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Happy New Year Colleagues :

The Archives for all of 2003 are now on-line at:

http://www.microscopy.com/MicroscopyListserver

Cheers...

Your Friendly Neighborhood SysOp
Nestor

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 1 22:02:03 2004

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Would someone point me to the listserver
for failure analysis discussion of metallurgical and
integrated circuit devices?

tnx,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 1 22:29:41 2004

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Gary:

The information is as follows:

====================== EDFAS Discussion List
=============================
This E-mail forum is a service exclusively for members of the
Electronic Device Failure Analysis Society, http://www.edfas.org

To reply or post a message to the whole group, send to:
edfas-at-mh.databack.com

To unsubscribe, send a message to: leave-edfas-at-mh.databack.com

For problems or questions, send an email to:
owner-edfas-at-mh.databack.com

Best regards-

David

--
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Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
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email: henriks-at-southbaytech.com

Celebrating 38 years of providing Materials Processing Solutions for Metallogaphy,
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The information contained in this message and any attachments is privileged and
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If you are not the intended recipient, please do not read, copy or disclose this
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delete this message from your system.

Gary Gaugler wrote:

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}
} Would someone point me to the listserver
} for failure analysis discussion of metallurgical and
} integrated circuit devices?
}
} tnx,
} gary g.

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 2 10:09:20 2004

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Hello all:

I've seen hot/cold stages from Deben that
look like they could hold a standard pin
stub specimen. However, they seem to
be optimized for low temperature work.
Does anyone know of some other supplier
that makes SEM specimen holders that will
heat up to about 200C and perhaps cool
to -25C?

The unit would need to mate to the stage
on a LEO Supra 55VP's specimen interchange
stage or on a FEI Sirion 400, under similar
circumstances.

Gatan makes a series of heated stages but
they seem more for stress testing and bulk
specimens. I will have an IC chip thermal
expoxy'd to a 12mm diameter Al pin stub. I need
to be able to heat this specimen in the SEM
and at any tilt and WD that the SEM will support.
Temperature stability could be as bad as +-5C.
That is OK.

Specimen holder and specimen changeout via
slide out chamber door is OK. Specimen interchange
lock does not have to be used.

thanks for any ideas and leads,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 2 11:27:25 2004

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In the latest issue of Microscopy Today there is an article on
pseudo-coloring of images. Since this is not something that I normally
do, I read the article with interest. I was surprised to find that the
author says that biologists nearly always use the "spectrum" color table
for the pseudo-coloring of grayscale images. I had thought that those
who study visual perception had found that among pseudo-color scales the
"thermal" scale is much better than all the others at providing a good
intuitive reading of the image. This is, I think, the scale that
Photoshop calls "Black Body". Can someone please clear up my confusion.
--
..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 2 11:58:48 2004

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Listers,

Here is the table of contents for the January/February 2004 issue of
Microscopy Today.

New Subscriptions via http://www.microscopy-today.com only, please.
New subscriptions will close on Thursday 8 January for this issue.

There has been a major change in subscription policies coming out of the MSA
Winter Council meeting.

Briefly: Canadians and Mexicans are now offered free subscriptions along
with microscopists in the USA.

MSA members anywhere have free subscriptions.

Non-MSA, non-North American subscriptions have been reduced from $80 or
$110US to $35US. Additional details in the magazine or on our web site.

THIS WILL BE THE LAST ISSUE NON-MSA MEMBER, NON-NORTH AMERICAN, UNSUBSCRIBED
OR NOT-CURRENTLY-SUBSCRIBED INDIVIDUALS WILL RECEIVE!

Listers,

Here is the table of contents for the November/December 2003 issue of
Microscopy Today. This issue is mailed with the Call for Papers for the 2004
Microscopy and Microanalysis meeting

New Subscriptions via http://www.microscopy-today.com only, please
New subscriptions will close on Tuesday 11 November for this issue.

There has been a major change in subscription policies coming out of the MSA
Winter Council meeting.

Briefly: Canadians and Mexicans are now offered free subscriptions along
with microscopists in the USA.

MSA members anywhere have free subscriptions.

Non-MSA, non-North American subscriptions have been reduced from $80 or
$110US to $35US. Additional details in the magazine or on our web site.

PURGING OF NON-MSA MEMBER, NON-NORTH AMERICAN, UNSUBSCRIBED OR
NOT-CURRENTLY-SUBSCRIBED INDIVIDUALS IS UNDERWAY!

January/February 2004
Carmichael: Correlating Fluorescence Microscopy with Electron Microscopy
P.E. Batson: Electron Microscopy Enters a New Era Using Aberration
__Correction
Paula Allan-Wojtas: Microscopy and Imaging of Foods— The Whys and Hows
Jerry Sedgewick: Image Stitching Using Photoshop
Michael Bode: A Few Thoughts About Image File Storage
Paul Beauregard: Behavior of Particle Size Distributions, Means and BET
__Values in Ideal and Non-Ideal Morphology Systems in a TEM
Katerina Moloni: The Moving Finger Writes: Carbon Nanotubes as AFM Probe
__Tips
Robert M. Zucker: Confocal Microscopy System Performance: Axial Resolution
Shane Roberts, Daniel Flatoff: Enhanced Sample Preparation of Cu Low-k
__Semiconductors via Mechanical Polishing and Ion Beam Etching
Luc Harmsen: The Year That Was! Microscopy in Southern Africa
Robert P. Apkarian: Comments on Cryo High Resolution Scanning Electron
__Microscopy
Jose A. Mascorro: Propylene Oxide: To Use or Not to Use in Biological
Tissue __Processing
M. T. Postek & A. E. Vladár: Is Low Accelerating Voltage Always the Best for
__Semiconductor Inspection and Metrology?

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 2 12:10:04 2004

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Yes it is unfortunately true that many (most?) biologists do use the
"spectrum" color scale, largely because it makes "prettier-looking"
images. It the cases where they are trying to illustrate
quantitative contrast this is not only grossly misleading but it is
usually plain wrong and can produce horrific artifacts! The worst
offenders are chiefly light microscopists who are trying to represent
weak flourescence contrast and for some reason think it shows up
"better" with a spectrum scale. In the STEM/X-Ray/EELS biological
microanalysis field most of us use some variation of the "black Body"
scale which of course more closely parallels the greyscale that is
intuitively quantitative anyway (black = 0, shades of grey through
white represent more positive values). Relative contrast or
non-linear scaling can be achieved by manipuating the scale either
continuously or by introducing discontinuities to other scales; of
course color then becomes essential (a) because the human eye can
perceive considerably more colors than levels of grey, and (b) one
can extend the scale over a far greater dynamic range(s); most
monitors only display 8-bit levels of grey (24-bit color) but data
are often 32-bit or more in dynamic range.

The topic of visual perception of data is a fascinating one indeed
and has been addressed in several treatises over the years. However
in my experience, I have found the most (subjectively) pleasing
results to come from visual artists (painters) who seem to have a
natural instinct for such representations. A visit to any good art
museum should convince most people of this!

Sorry if this is a rather brief and simplistic answer to your
question but maybe it helps some!

Peter

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
Peter Ingram
Sr. Physicist
Adj. Professor of Pathology,
Duke University Medical Center
Box 90319
LaSalle Street Extension
DURHAM NC USA 27708-0319

Tel: (919) 660-2695
Fax: (919) 660-2671
e-mail: p.ingram-at-cellbio.duke.edu
http://152.3.54.107/AEM_LAB.html

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 2 12:41:52 2004

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Hello Alwyn,

happy new year!

the most common use of Pseudo color is to enhance the contrast of the images
and make small details more visible.

A little background:

Computer monitors are normally set to "True Color". On most graphics cards
that means 32 bit of information per pixel, or "Millions of colors" as they
say. However, each pixel is represented by 3 colors (Red, Green, and Blue),
and each of these colors can take on an 8 bit value. 8 bits mean, that there
are 256 shades of each color available, which can be combined to give you
the "millions of colors" (256 x 256 x 256). What is not so obvious, that for
gray levels you need to combine the 3 colors in at the same strength, i.e.
black is 0,0,0, medium gray is 128,128,128 and white is 255,255,255. This
shows, that even if your monitor can display millions of colors, it can
usually only show 256 levels of gray. Take into account, that the human eye
can distinguish perhaps 50 or so levels of gray and modern cameras can
provide anywhere from 4000 to 64,000 levels of gray, and the need for
different color schemes becomes obvious.

Enter the pseudo colors.

There are as many pseudo color schemes as you can think of. Several have
become "standards". Among them definitely the "black body" scheme, and the
"spectrum" color scheme. The "black body" is perhaps more intuitive, as it
basically goes from Red to White. This provides a linear scale, which is
easy to understand to anybody who has seen a metal heated (and perhaps
burned himself or herself), and it is probably easier to discern small
contrasts both in the red and the bright parts of the spectrum than in b/w
images. However, it does not make full use of the capabilities of a monitor.
The "spectrum" pseudo color, on the other hand, makes full use of the
availble color spectrum, perhaps at the price of an intuitive understanding.
It may be better suited to images that have "many" gray levels, which all
need to be discerned. If used wrongly, however, the spectrum pseudo color
can also lead to misleading coloring.

I hope this helps.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Alwyn Eades [mailto:jae5-at-lehigh.edu]
Sent: Friday, January 02, 2004 10:28
To: MSA listserver

In the latest issue of Microscopy Today there is an article on
pseudo-coloring of images. Since this is not something that I normally
do, I read the article with interest. I was surprised to find that the
author says that biologists nearly always use the "spectrum" color table
for the pseudo-coloring of grayscale images. I had thought that those
who study visual perception had found that among pseudo-color scales the
"thermal" scale is much better than all the others at providing a good
intuitive reading of the image. This is, I think, the scale that
Photoshop calls "Black Body". Can someone please clear up my confusion.
--
.........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 3 07:27:59 2004

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Peter writes ...

} ...
} ... In the STEM/X-Ray/EELS biological microanalysis field
} most of us use some variation of the "black Body" scale
} which of course more closely parallels the greyscale that
} is intuitively quantitative anyway (black = 0, shades of
} grey through white represent more positive values).

I remember an M&M '99 session, which introduced a pseudo-color scale for
quantitative images (e.g., elemental distributions, maps). That is, ranges
of color for representing "orders of magnitude" ... or ranges we might refer
to as "major", "minor", "trace", or "undetected". The session was intended
to be its introduction, such that its color ranges would become familiar to,
and used by all, as so that quantitative images could be actually compared.
I thought it was interesting concept at the time, but also felt it needed
some refinement. Unfortunately my inadequate notetaking didn't allow for me
to ever find the color table and download it.

I have no idea if it was mentioned in the MT article, but the people who
had introduced the color scheme were from NIH (or, was it NIST?). I believe
it is too bad the color scheme never did rise to common use. That is, even
if I did feel it still needed some refinement, it would be a good thing if
quantitative images could all be compared.

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 3 10:27:30 2004

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} In Dec, 2001, a group of animal rights protestors in Cambridge announced that
} they intended to sue "Christianity as a whole" and anyone who celebrates
} Christmas. The shock announcement comes after years of protesting against
} Christmas which, they say, causes unnecessary cruelty to turkeys.

And ignore the use of reindeer as beasts of burden? Or use of swine as ham?
Sounds pretty discriminatory to me.

Some people think the New Year is when it is because it was the celebration of
Jesus's circumcision. If we think this is bad (e.g. castration ritual), do we
refuse to follow the calendar? BTW, the holiday of New Year has become almost
global.

This is a time of year when we should take some time off and relax. This
message is apropos to this bboard specifically because for a few days I didn't
think about microscopy at all. I read novels, slept, ate ham and argued with
family over the Iraq war and mostly trivial stuff. This is happy holidays.

Now, can we get back to microscopy and drop the holiday stuff? Even if some
of us won't be completing our Christmas celebrations until the 6th?

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 3 11:40:17 2004

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Email: faj-at-highway1.com.au
Name: Faye Taylor

Organization: Amateur

Education: Undergraduate College

Location: Perth, Western Australia

Question: Hello there,
I am a starter who wishes to get her grandchildren interested in a
world beyond TV & computer games. I started using computers when I
purchased my first 128K Mac back in 1985 . My present Mac is a G3
192MB ram & 40 GB hard drive.

I recently aquired a second hand
"MOTIC Biological Series B1 223A " but I have found that I cannot
use my lovely Fuji S602Z digital camera to take photos.

Do you have any ideas which will enable me to combine the use of the
hardware that I possess?
I feel that the hardest part is getting software that will enable me
to join up to the Macintosh even if I purchased a new camera.

I would really like to take the photos digitally but is it impossible
with my present configuration?
i would appreciate any comments please

Happy New Year Faye

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 3 13:32:14 2004

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} Email: faj-at-highway1.com.au
} Name: Faye Taylor
}
} Organization: Amateur
}
} Education: Undergraduate College
}
} Location: Perth, Western Australia
}
} Question: Hello there,
} I am a starter who wishes to get her grandchildren interested in a
} world beyond TV & computer games. I started using computers when I
} purchased my first 128K Mac back in 1985 . My present Mac is a G3
} 192MB ram & 40 GB hard drive.
}
} I recently aquired a second hand
} "MOTIC Biological Series B1 223A " but I have found that I cannot
} use my lovely Fuji S602Z digital camera to take photos.
}
} Do you have any ideas which will enable me to combine the use of the
} hardware that I possess?
} I feel that the hardest part is getting software that will enable me
} to join up to the Macintosh even if I purchased a new camera.
}
} I would really like to take the photos digitally but is it
} impossible with my present configuration?
} i would appreciate any comments please

Faye -

You don't say WHY you can't take photos with your equipment! I
suggest that you contact microscopeworld.com. They sell many Motic
scopes under the U.S. brand name "National", plus camera connectors,
so you should be able to get specific advice on your problem.

You'll find abundant microscopy resources for the grandkids at the
MICRO website; URL below.

Caroline

--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 3 15:23:11 2004

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Friends,
here is the table of content of the last 2003 issue of J.Microscopy
(OXF)
on Microscopy in the Nanobioscience.

215
Foreword
A. Diaspro

217
Polysaccharide properties probed with atomic force microscopy
N. I. Abu-Lail, T. A. Camesano

239
Encapsulated yeast cells inside Paramecium primaurelia: a model system
for protection capability of polyelectrolyte shells
S. Krol, O. Cavalleri, P. Ramoino, A. Gliozzi, A. Diaspro

244
Insights into the regulation of transcription by scanning force
microscopy
R. T. Dame, C. Wyman, N. Goosen

254
Monitoring enzymatic reactions in nanolitre wells
I. T. Young, R. Moerman, L. R. Van Den Doel, V. Iordanov, A. Kroon, H.
R. C. Dietrich, G. W. K. Van Dedem, A. Bossche, B. L. Gray, L. Sarro,
P. W. Verbeek, L. J. Van Vliet

264
The molecular machines of DNA repair: scanning force microscopy
analysis of their architecture
A. Janiijevi, D. Ristic, C. Wyman

273
TectoRNA and 'kissing-loop' RNA: atomic force microscopy of
self-assembling RNA structures
H. G. Hansma, E. Oroudjev, S. Baudrey, L. Jaeger

280
The nacre protein perlucin nucleates growth of calcium carbonate
crystals
S. Blank, M. Arnoldi, S. Khoshnavaz, L. Treccani, M. Kuntz, K. Mann,
G. Grathwohl, M. Fritz

292
Atomic force microscopy study of living diatoms in ambient conditions
I. C. Gebeshuber, J. H. Kindt, J. B. Thompson, Y. Del Amo,
H. Stachelberger, M. A. Brzezinski, G. D. Stucky, D. E. Morse, P.
K. Hansma

300
Self-assembly and recrystallization of bacterial S-layer proteins at
silicon supports imaged in real time by atomic force microscopy
E. S. Györvary, O. Stein, D. Pum, U. B. Sleytr

307
Fluorescent resolution target for super-resolution microscopy
P. R. H. Stark, L. J. Rinko, D. N. Larson

I hope is of interest

All my best
ALby

.......................................................................
...................................
.. non basta, resistere, resistere...resistere
^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
Alberto Diaspro
Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genoa, Italy
voice: +39-0103536426/480 fax 010314218
diaspro-at-fisica.unige.it, http://www.lambs.it
http://wiley.com/cda/product/0,,0471409200,00.html

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 4 17:50:49 2004

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Hi Mike!

I meant the "visual perception" of quantitation which is what
Alwyn's initial observation referred to. Of course I agree totally
with you that its easer to distinguish different colors from one
another than shades of any color or grey. The question is rather "is
bright green more or less than yellow?" Any quantitative color scale
must also have factored in parameters such as Hue, Saturation abd
Brightness; this is one of the main failings of the "spectrum scale"
- it doesn't!

Cheers etc

Peter

} Hello Peter,
}
} in actuality, the situation is a bit more complex than that. I am looking at
} the LUT right now that we have in our analySIS software, and you are of
} course right that a pixel with no intensity (intensity 0) is displayed as
} black (0,0,0). However, the intensity "1" is displayed as (R:41, G:0, B:0).
} Technically, it goes from black to white, but realistically, it goes from
} "dark red" to white.
}
} The situation becomes mor complex at the other end. To make yellow, you have
} to add in a green component, and to make white you also have to add in blue.
} So, it is not straightforward "black to white" or "red to white". Other
} colors get mixed in at the higher intensities to make yellow to white.
}
} As for qantitation: I am not sure, what you are referring to. Quantitaion is
} best done on the b/w images with the help of a computer, which has no
} problems distinguishing intensity 2976 from 2977. For the display of small
} contrasts for the human eye I agree with you, but there an even better
} choice is the spectrum LUT. It's easier to distinguish yellow from green
} than it is to distinguish "dark orange" from "darker orange".
}
} mike
}
}
}
} -----Original Message-----
} From: Peter Ingram [mailto:p.ingram-at-cellbio.duke.edu]
} Sent: Friday, January 02, 2004 12:03
} To: Mike Bode
} Subject: [Microscopy] RE: Psuedo color
}
}
}
} Actually the "black body" scale goes from black to white, albeit
} through red, orange and yellow, not simply red to white - a vital
} distinction when quantitation is involved!
}
} Peter
}
}
} } ---------------------------------------------------------------------------
} ---
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
Peter Ingram
Sr. Physicist
Adj. Professor of Pathology
Duke University Medical Center
Box 90319
DURHAM NC 27708-0319

Tel: 919 660-2695
Fax: 919 660-2671
Email: p.ingram-at-cellbio.duke.edu
Web: http://152.3.54.107/AEM_LAB.html

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 08:44:39 2004

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Gary-
I have been using a dual microprobe I purchased from Ernest F.
Fullam Inc.:

900 Albany Shaker Rd.
Latham
NY 12110-1491
800-833-4024, 518-785-5533

Part #15855 dual, o-ring sealed manipulator. They had suggested that I
purchase micromanipulators that had metal bellows rather than o-ring
seals since I have a FE-SEM, but since all of the other seals on my
specimen chamber were o-rings, including detectors that run in and out,
I opted for the less expensive o-ring sealed option, and I have had no
trouble with them. I cannot say if the microprobes I have will meet
your positioning accuracy requirements as I am currently using fairly
blunt tips. I also do not have verniers to check reproducibility. I
just watch where I am placing them using the SEM. The probes are
essentially the same as one might find on an electrical probe station
for testing devices. The one problem I do have with them is that since
I work with the probe tips near the pole piece, the probes induce a
significant aberration. I do not know if the set screws holding the tips
in are magnetic, making the problem worse or not. I do know that there
are magnetic knurled nuts about 2" up the shaft. You may need to
specify the materials you want the probe arms made out of, as well as
working at longer WD/higher kV. I haven't bothered to correct this, or
to move the probes further from the pole piece, as the resolution is
adequate for my experiments. I have found Fullam to be very helpful and
open to customizing their products for individual needs. They have a
web site at: http://www.fullam.com/. Good luck.

Sincerely,
Matthew Ervin, Ph.D.
(301)394-0017 phone, (301)394-1559 fax
MErvin-at-ARL.Army.mil

M/S: AMSRL-SE-RL
US Army Research Laboratory
2800 Powder Mill Road
Adelphi, MD 20783-1197

Disclaimer: The opinions and views expressed above are those of the
author and do not necessarily represent those of the U.S. Army Research
Laboratory or any other government agency

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Wednesday, December 31, 2003 10:11 PM
To: MSA listserver

Hi all:

Has anyone seen a source of micro probes for SEM that allow electrical
contact to a SEM chamber specimen? I need very precise
positioning--like within 0.15u or better and 0.05u repeatability and
stability.

I need two contact probes.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 09:42:19 2004

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Hello,

Our lab recently began using the "New Formulation" Kodak Electron
Microscope Film 4489 and employed a number of tips for developing this
film which we retrieved from the Listserver archive commencing Jan 2003

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 10:02:05 2004

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Phil,

I suggest that you check out "Polymer Microscopy", 2nd edition, by Sawyer &
Grubb. I believe that they addressed this issue.

Cheers,

"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

Philip Oshel
{peoshel-at-wisc.edu} To: Microscopy-at-sparc5.microscopy.com
cc:
Subject: [Microscopy] nylon SEM
12/23/03 02:55 PM

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Materials micromavens,

We have a user doing SEM of nylon, with embedded bits. We'd like to
chemically etch the nylon, which is something of an entertaining
problem, since nylon is used to mask things against etchants.
Does anyone have a recipe for something that will etch nylon and not
silica?
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 10:34:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,

Our lab recently began using the "New Formulation" Kodak Electron
Microscope Film 4489 and employed a number of tips for developing this
film which we retrieved from the Listserver archive commencing Jan 2003

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 10:44:59 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi, all-

We here at the Neurotoxicology Labs at Rutgers University have an
ancient Coolwell chiller for our Zeiss EM 10CA, and it appears to be
dying. Coolwell went out of business years ago, and Zeiss pointed me to
Lytron, Inc. as the company who bought Coolwell's stuff when it went
under. I have tried to contact Lytron online about repairs or a
possible replacement for this chiller, but they don't seem to be paying
much attention to their email. I am going to call them directly, of
course, but what I would like to know is if anyone can recommend another
company or particular chiller model that would be appropriate for our
EM, so that if Lytron continues to blow me off I will have other
sources that I can try.

Hope you all had a happy holiday!

Thanks in advance-
Kathleen Roberts
Principal Lab Technician
Neurotoxcology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 10:52:17 2004

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Nestor,

Many thanks to you for all your hard work over the past years. I very much
appreciate the service that you provide for the microscopy/microanalysis
community.

Cheers,

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

"Nestor J. Zaluzec"
{zaluzec-at-microscopy.c To: microscopy-at-ns.microscopy.com
om} cc:
Subject: [Microscopy] Administrivia: Archives for
2003 Now On-Line
01/01/04 10:37 AM

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Happy New Year Colleagues :

The Archives for all of 2003 are now on-line at:

http://www.microscopy.com/MicroscopyListserver

Cheers...

Your Friendly Neighborhood SysOp
Nestor

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 11:35:40 2004

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Dear Kathleen,

I have a Zeiss EM900 and my Coolwell also just bit the dust about
2months ago. I went with a Haskris Model 075 chiller, which includes
Option (K), a 220V interlock as specified by LEO. I have two other
Haskris chillers that have been very reliable (on a JEOL SEM and on a
Philips TEM).

Here is the contact info:

Doug Wagner
Haskris Co.
100 Kelly Street
Elk Grove Village, IL 60007
847-956-6420, x243 (tel)
847-956-6595 (fax)
doug-at-haskris.com

Good luck!
Ann

++++++++++++++++++++++++++++++++++++++
Ann Hein Lehman
Assistant Director, Electron Microscopy Facility
Mailstop: LSC-314
Trinity College
300 Summit Street
Hartford, CT 06106
v. 860-297-4289
e. ann.lehman-at-trincoll.edu
f. 860-297-2538
www.trincoll.edu/~alehman

-----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
Sent: Monday, January 05, 2004 11:54 AM
To: Microscopy-at-sparc5.microscopy.com

Hi, all-

We here at the Neurotoxicology Labs at Rutgers University have an
ancient Coolwell chiller for our Zeiss EM 10CA, and it appears to be
dying. Coolwell went out of business years ago, and Zeiss pointed me to

Lytron, Inc. as the company who bought Coolwell's stuff when it went
under. I have tried to contact Lytron online about repairs or a
possible replacement for this chiller, but they don't seem to be paying
much attention to their email. I am going to call them directly, of
course, but what I would like to know is if anyone can recommend another

company or particular chiller model that would be appropriate for our
EM, so that if Lytron continues to blow me off I will have other
sources that I can try.

Hope you all had a happy holiday!

Thanks in advance-
Kathleen Roberts
Principal Lab Technician
Neurotoxcology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 11:39:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Check out Haskris. I believe that they are the best on the market, in my
opinion, and they would make a model which would easily handle the Zeiss 10.

http://www.groupeinterconnexion.com/LaboratoryListingsAddPages/Chiller_Cryog
entics_Adds/HaskrisWaterChillerHA2953.htm

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 11:41:30 2004

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sorry, that website is: www.haskris.com

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 12:28:56 2004

Contents Retrieved from Microscopy Listserver Archives
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Hakris is a reasonably reliable chiller. I've had several on EM diff pumps. They also make a 115V version that I used on a Hitach S4500 FESEM since my lab had no chilled water supply. Unless strapped for cash, junk the old one. If it fails it can make a nasty mess of things. I think I spent 2K$ [American] for the one I bought 6 years ago.

Happy new year. [Can I say that?]

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Lehman, Ann [mailto:Ann.Lehman-at-trincoll.edu]
Sent: Monday, January 05, 2004 12:39 PM
To: Kathleen Roberts; Microscopy-at-sparc5.microscopy.com

Dear Kathleen,

I have a Zeiss EM900 and my Coolwell also just bit the dust about
2months ago. I went with a Haskris Model 075 chiller, which includes
Option (K), a 220V interlock as specified by LEO. I have two other
Haskris chillers that have been very reliable (on a JEOL SEM and on a
Philips TEM).

Here is the contact info:

Doug Wagner
Haskris Co.
100 Kelly Street
Elk Grove Village, IL 60007
847-956-6420, x243 (tel)
847-956-6595 (fax)
doug-at-haskris.com

Good luck!
Ann

++++++++++++++++++++++++++++++++++++++
Ann Hein Lehman
Assistant Director, Electron Microscopy Facility
Mailstop: LSC-314
Trinity College
300 Summit Street
Hartford, CT 06106
v. 860-297-4289
e. ann.lehman-at-trincoll.edu
f. 860-297-2538
www.trincoll.edu/~alehman

-----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
Sent: Monday, January 05, 2004 11:54 AM
To: Microscopy-at-sparc5.microscopy.com

Hi, all-

We here at the Neurotoxicology Labs at Rutgers University have an
ancient Coolwell chiller for our Zeiss EM 10CA, and it appears to be
dying. Coolwell went out of business years ago, and Zeiss pointed me to

Lytron, Inc. as the company who bought Coolwell's stuff when it went
under. I have tried to contact Lytron online about repairs or a
possible replacement for this chiller, but they don't seem to be paying
much attention to their email. I am going to call them directly, of
course, but what I would like to know is if anyone can recommend another

company or particular chiller model that would be appropriate for our
EM, so that if Lytron continues to blow me off I will have other
sources that I can try.

Hope you all had a happy holiday!

Thanks in advance-
Kathleen Roberts
Principal Lab Technician
Neurotoxcology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 13:07:58 2004

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Ann-

Oooh, thank you! You just made things a lot easier for me. :o) I
guess I should talk to LEO as well to see what options I need, unless
your Zeiss and mine are similar enough?

God, how I love listservs....thank you, Nestor!

Thanks again-
Kathleen
Neurotoxicology Labs
Rutgers University

Lehman, Ann wrote:

} Dear Kathleen,
}
} I have a Zeiss EM900 and my Coolwell also just bit the dust about
} 2months ago. I went with a Haskris Model 075 chiller, which includes
} Option (K), a 220V interlock as specified by LEO. I have two other
} Haskris chillers that have been very reliable (on a JEOL SEM and on a
} Philips TEM).
}
} Here is the contact info:
}
} Doug Wagner
} Haskris Co.
} 100 Kelly Street
} Elk Grove Village, IL 60007
} 847-956-6420, x243 (tel)
} 847-956-6595 (fax)
} doug-at-haskris.com
}
} Good luck!
} Ann
}
} ++++++++++++++++++++++++++++++++++++++
} Ann Hein Lehman
} Assistant Director, Electron Microscopy Facility
} Mailstop: LSC-314
} Trinity College
} 300 Summit Street
} Hartford, CT 06106
} v. 860-297-4289
} e. ann.lehman-at-trincoll.edu
} f. 860-297-2538
} www.trincoll.edu/~alehman
}
}
} -----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
} Sent: Monday, January 05, 2004 11:54 AM
} To: Microscopy-at-sparc5.microscopy.com
} Subject: [Microscopy] chiller for Zeiss EM 10CA
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 13:11:23 2004

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Pat-

Yes, Dr. Bonder is still at Rutgers-I just did a search for him on
Rutgers' website. I don't know him personally, though, as he is on the
Newark campus, where I have never been, and I am on the New Brunswick
campus. Worlds apart... :o)

Kathleen

Pat Connelly wrote:

} Kathleen,
} WE have been using a Haskris Co. water chiller (RO 75) since 1996 for
} my Phillips 200 TEM. It works very well and the only complaint that I
} have had is that we use a timer to shut down our ancient scope at
} night and the one on the chiller keeps dying - it just stays on.
}
} This company was recommended to me when our previous chiller, also a
} Haskris,died after 25 years or so, by a refrigeration specialist who
} does some contract work here.
}
} Do you know if Dr. Ed Bonder is still at Rutgers? He was in EM the
} last time I had heard from him but I do not know the exact department
} - Biology? He was a grad student here at Penn a few decades ago!
}
} Pat Connelly
} Research Specialist

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 13:21:08 2004

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To all who wrote in reply to my question-
}
} Thank you for the information, you all have made my life much easier. :o)
}
} Now I can sit down with my boss and be able to give him some real
} information about replacing this poor thing, instead of "I'm still
} searching for a source..."
}
} Thanks again-
} Kathleen
} Neurotoxicology Labs
} Rutgers University

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 13:26:57 2004

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Ouch! That is an expensive repair...would LEO install a temp. sensor on
a 'scope that is so old? My impression was that LEO didn't service
Zeiss 'scopes anymore.

Thanks for the information-
Kathleen

Ken Tiekotter wrote:

} Dear Kathleen,
}
} I just had a major life change as my Coolwell went down, was repaired, and
} crashed again for the third and final time. The issue was exasperated by a
} series of facilities failures. The outcome was about an $18k repair bill to
} include a new Haskris chiller (~$5600.00)
}
} Unfortunately, the Zeiss EM 10CA does not a temperature sensor to determine
} glycol temperature, but rather only flow rate. The repair included a
} complete overhaul of the column because oil vapors were not condensing in
} the diffusion pump and consequently went everywhere in the column.
}
} After almost 20 years with my beloved EM10, the hospital decided to donated
} the scope and close my lab. You may want to check with Zeiss (LEO) about
} installing a temperature sensor and automatic relay to shut the HV value if
} the circulator temperature gets too high.
}
} Best wishes to you and your EM10!
} Ken
}
} _______________________________________
} Kenneth L. Tiekotter, Adjunct Professor
} The University of Portland
} Department of Biology
} 5000 N Willamette Blvd.
} Portland, OR 97203 USA
}
} Director, MicroImaging Dx Center
} Legacy Portland Hospitals
} Legacy Holladay Park Medical Center
} 1225 NE 2nd Avenue
} Portland, OR 97232 USA
}
} Tel.: 503.413.5391
}
}
}
}
}
} On 1/5/04 8:54 AM, "Kathleen Roberts" {kgrobert-at-rci.rutgers.edu} wrote:
}
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 13:40:57 2004

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Joel-

I will admit that I am not entirely sure what is wrong with it. All I
know is that when I turn the 'scope on, it's fine for the first half
hour or so...then a buzzer goes off-there is no indicator light to say
what that buzzer is for on the 'scope, but my boss tells me that it's an
overtemp alarm. If you look at the temp gauge on the chiller, it's
reading way above the overtemp limit.

There was one occasion when a pump in the house distilled water system
was dying, and when it was replaced, the 'scope stopped buzzing. Now,
however, the distilled water system appears to be fine, and the 'scope
is buzzing again, so I am assuming that it is the chiller.

I did get a local HVAC repair guy in (from the same company that
resurrected our old cryostat), but he said that he couldn't do anything
without the refrigeration and other specifications for that chiller. I
managed to get a couple of diagrams from someone else on this list (his
name escapes my memory for the moment, but thanks again anyway!), but
the HVAC guy said that it wasn't enough. As Lytron isn't willing to
help, I'm going to give up and get a new chiller, as this one is pretty
old anyway.

Thanks,
Kathleen
Neurotoxicology Labs
Rutgers University

McClintock, Joel wrote:

} Kathleen,
}
} I take care of a Zeiss 902 with a coolwell chiller. I have fixed this thing several times. What is the problem with it? Often the temp sensor goes haywire. I have found it is often the switch. I have replaced it for around $7. As others have recommended Haskris is my favorite. If money is tight I may be able to direct you to a used one.
}
} Joel McClintock
} EM Specialist
} U of Kentucky
} 859-257-1242
}
} -----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
} Sent: Mon 1/5/2004 11:54 AM
} To: Microscopy-at-sparc5.microscopy.com
} Cc:
} Subject: [Microscopy] chiller for Zeiss EM 10CA
}
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi, all-
}
} We here at the Neurotoxicology Labs at Rutgers University have an
} ancient Coolwell chiller for our Zeiss EM 10CA, and it appears to be
} dying. Coolwell went out of business years ago, and Zeiss pointed me to
} Lytron, Inc. as the company who bought Coolwell's stuff when it went
} under. I have tried to contact Lytron online about repairs or a
} possible replacement for this chiller, but they don't seem to be paying
} much attention to their email. I am going to call them directly, of
} course, but what I would like to know is if anyone can recommend another
} company or particular chiller model that would be appropriate for our
} EM, so that if Lytron continues to blow me off I will have other
} sources that I can try.
}
} Hope you all had a happy holiday!
}
} Thanks in advance-
} Kathleen Roberts
} Principal Lab Technician
} Neurotoxcology Labs
} Dept of Pharmacology & Toxicology
} Ernest Mario School of Pharmacy
} Rutgers University
} 41 B Gordon Rd
} Piscataway, NJ 08854
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 13:47:21 2004

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Gary,
I have seen presentation on two micro-manipulator type systems: Zyvex - a MEMS based system (www.zyvex.com), and Klendiek (http://kleindiek.com, http://www.ascendinstruments.com/product_nanoprober.asp) a micro-motor based system distributed in USA by Ascend Instruments. They are geared to manipulate specimen inside a FIB or SEM chamber and both can be used for electrical measurements. The problem is that they are expensive (~100K). Since I have not actually used either one of them I cannot recommend them. We are thinking of a versatile solution that would allow TEM sample extraction, transfer, in DB-FIB and also allow us to perform occasional electrical measurements on powered devices.

Regards and Happy New Year to all.

Jerzy

PS: If you get other replies, please post them since I would also be interested in a less expensive system but with less flexibility. I do not have any vested interest in either company, we only had sales presentations from both distributors.

******************************************************
Jerzy Gazda, Ph.D. Advanced Micro Devices
Supervising Engineer 5204 E. Ben White Blvd. - MS 512
PCAL - AIM Section Austin, TX 78741
TEL: 1-800-538-8450, Ext. 51453
jerzy.gazda-at-amd.com
******************************************************

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Wednesday, December 31, 2003 9:11 PM
To: MSA listserver

Hi all:

Has anyone seen a source of micro probes for SEM that allow electrical
contact to a SEM chamber specimen? I need very precise
positioning--like within 0.15u or better and 0.05u repeatability and
stability.

I need two contact probes.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 16:05:53 2004

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Another source is Omniprobe, http://www.omniprobe.com/. Click the Products nav button. They can do electrical testing, TEM lift-out, mechanical testing, etc.
I have no financial interest in the company.

jerzy.gazda-at-amd.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Gary,
} I have seen presentation on two micro-manipulator type systems: Zyvex - a MEMS based system (www.zyvex.com), and Klendiek (http://kleindiek.com, http://www.ascendinstruments.com/product_nanoprober.asp) a micro-motor based system distributed in USA by Ascend Instruments. They are geared to manipulate specimen inside a FIB or SEM chamber and both can be used for electrical measurements. The problem is that they are expensive (~100K). Since I have not actually used either one of them I cannot recommend them. We are thinking of a versatile solution that would allow TEM sample extraction, transfer, in DB-FIB and also allow us to perform occasional electrical measurements on powered devices.
}
} Regards and Happy New Year to all.
}
} Jerzy
}
} PS: If you get other replies, please post them since I would also be interested in a less expensive system but with less flexibility. I do not have any vested interest in either company, we only had sales presentations from both distributors.
}
} ******************************************************
} Jerzy Gazda, Ph.D. Advanced Micro Devices
} Supervising Engineer 5204 E. Ben White Blvd. - MS 512
} PCAL - AIM Section Austin, TX 78741
} TEL: 1-800-538-8450, Ext. 51453
} jerzy.gazda-at-amd.com
} ******************************************************
}
}
} -----Original Message-----
} } From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Wednesday, December 31, 2003 9:11 PM
} To: MSA listserver
} Subject: [Microscopy] micro probes
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi all:
}
} Has anyone seen a source of micro probes for SEM that allow electrical
} contact to a SEM chamber specimen? I need very precise
} positioning--like within 0.15u or better and 0.05u repeatability and
} stability.
}
} I need two contact probes.
}
} gary g.

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 16:34:46 2004

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--------------------------------------------------------------------------

Email: letitsnow-at-antelecom.net
Name: Elizabeth Colvin

Organization: Homeschool

Education: 9-12th Grade High School

Location: Pearblossom, CA-L.A. county

Question: I have obtained several unstained blood smears. I have
Wright's stain and methylene blue available. Can you please tell me
how long to leave the stain on the slide before rinsing. And do I
rinse with distilled water. Thank you.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 16:52:04 2004

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Kathleen,

Good question from Joel. The alarm (buzzer)you are hearing more than
likely is the chiller fluid flow indicator on the EM10. The pressure
must be maintained at 1.5 - 2liters per minute. The flow indicator is
located on the right-hand side of the column inside the gray hinged
'door'. These is a small glass window to show where the float is in
relationship to the flow of fluid: the higher the float, the greater
the number of liters/minute.

On the front of the Coolwell chiller is also a flow indicator, which
should be adjusted to meet the 1.5 - 2 liter flow on the microscope.
Also check to see if the temperature gauge on the Coolwell remains the
same or fluctuates. It could be the chiller is fine, but the pump is
going out.

Ken

Kathleen Roberts wrote:

}
}
} ------------------------------------------------------------------------
------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

---------------------------------------
Kenneth L, Tiekotter, Adjunct Professor
Dept. of Biology
The University of Portland
5000 N Willamette Blvd,
Portland, OR 97203 USA

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 17:16:32 2004

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Dear List,
I am posting the following for Dr. Jensen, the head of our cryo-EM
group:

------------------------------------------------------------------------
------------------------
I'm looking for an image processing scientist/computer programmer to
help with our expanding biological electron tomography projects here at
Caltech. We are currently imaging many specimens including cells,
viruses, and purified protein complexes with a state-of-the-art 300kV,
helium-cooled, energy-filtered, automated, FEG TEM. We are in the
process now of purchasing a large new supercomputer for the structural
biology groups. Duties would include applying existing programs as well
as developing new software for image processing needs, handling large
amounts of image data, managing processes on our supercomputer, working
with students to help them solve image processing problems, and being a
creative member of a growing scientific team. Minimum qualifications
are a bachelor’s degree, strong programming skills, mathematical
aptitude, an ability to work well with others, and enthusiasm for
biology research. Graduate education or extended experience in related
fields is preferred. Interested persons seeking either a post-doctoral
position or a permanent staff position are encouraged to apply. Salary
will be commensurate with qualifications. CalTech is located in
Pasadena, California (a suburb of Los Angeles) next to the San Gabriel
mountains, and offers an extraordinarily rich intellectual environment
for computationally-inclined scientists, all within a sunny, affordable,
diverse community that will make you want to stay. Please send CV and
three letters of reference to jensen-at-caltech.edu or

Dr. Grant Jensen
California Institute of Technology
Biology Division, Mailcode 114-96
1200 E. California Blvd.
Pasadena, CA 91125
------------------------------------------------------------------------
--------------------------

Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 17:40:32 2004

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Kathleen,

Just to add to what Ken said just below, if the flow alarm is in fact what
you are hearing, then just check the various filters in the cooling water
system, probably one in the chiller tank, probably another one on the input
side to the microscope. Or, the lines may be plugged up somewhere with crud
such as algae or corrosion products. After checking the filters and cleaning
or replacing them, if problem persists may have to have scope and/or
delivery lines flushed to clear them. I had to do that once for in an SEM's
interior cooling lines.

Hope this helps!
--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra
----------------------------------------------------------------------------
} Kathleen,
}
} Good question from Joel. The alarm (buzzer)you are hearing more than
} likely is the chiller fluid flow indicator on the EM10. The pressure
} must be maintained at 1.5 - 2liters per minute. The flow indicator is
} located on the right-hand side of the column inside the gray hinged
} 'door'. These is a small glass window to show where the float is in
} relationship to the flow of fluid: the higher the float, the greater
} the number of liters/minute.
}
} On the front of the Coolwell chiller is also a flow indicator, which
} should be adjusted to meet the 1.5 - 2 liter flow on the microscope.
} Also check to see if the temperature gauge on the Coolwell remains the
} same or fluctuates. It could be the chiller is fine, but the pump is
} going out.
}
} Ken
} } Kathleen Roberts wrote:
} } ------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ------------------------------------------------------------------------
} } Joel-
} }
} } I will admit that I am not entirely sure what is wrong with it. All I
} } know is that when I turn the 'scope on, it's fine for the first half
} } hour or so...then a buzzer goes off-there is no indicator light to say
} } what that buzzer is for on the 'scope, but my boss tells me that it's
} an
} } overtemp alarm. If you look at the temp gauge on the chiller, it's
} } reading way above the overtemp limit.
} }
} } There was one occasion when a pump in the house distilled water system
} } was dying, and when it was replaced, the 'scope stopped buzzing. Now,
} } however, the distilled water system appears to be fine, and the 'scope
} } is buzzing again, so I am assuming that it is the chiller.
} }
} } I did get a local HVAC repair guy in (from the same company that
} } resurrected our old cryostat), but he said that he couldn't do anything
} } without the refrigeration and other specifications for that chiller. I
} } managed to get a couple of diagrams from someone else on this list (his
} } name escapes my memory for the moment, but thanks again anyway!), but
} } the HVAC guy said that it wasn't enough. As Lytron isn't willing to
} } help, I'm going to give up and get a new chiller, as this one is pretty
} } old anyway.
} }
} } Thanks,
} } Kathleen
} } Neurotoxicology Labs
} } Rutgers University
} }

} ---------------------------------------
} Kenneth L, Tiekotter, Adjunct Professor
} Dept. of Biology
} The University of Portland
} 5000 N Willamette Blvd,
} Portland, OR 97203 USA

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 5 17:41:59 2004

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Hello Peter,

I did not want to imply that the "spectrum" scale is "perfect". There are
many color scales and depending on what you want to see or show, one or the
other might be better.

You bring up a good point, though: familiarity with the scale. Everybody can
interpret a black and white scale, and the thermal scale is also very
intuitive. Once we get to more colors, I would say that the spectrum scale
is familiar to most people, red on one end, blue on the other. Other scales
need more explanation or a color scale bar on the Image.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Peter Ingram [mailto:p.ingram-at-cellbio.duke.edu]
Sent: Sunday, January 04, 2004 16:54
To: Mike Bode
Cc: Microscopy-at-MSA.Microscopy.Com

Steven;
I was kidding about being a Raelian. I am agnostic. I celebrate the spirit of Christmas, not the religious part. My wife is Turkish, and is a Moslem. She loves Christmas, as does our daughter. We are presently being visited by my wife's mother and sister. Despite the fact that they are both Moslem, and neither of them speaks English, they loved their first Christmas. When my wife celebrates her holidays, I celebrate with her. My brother's wife is Jewish (another mixed marriage-agnostic and Jewish). Their family celebrates both Hanukah and Christmas. Their two kids love having two holidays to celebrate.
As for the spirit of Christmas, I am sorry to hear that it has eluded you. You can give gifts to loved ones any time, not just Christmas. You can try to bring more cheer into peoples lives any time, not just Christmas. You can get together with your family any time, not just Christmas. You can put up special decorations any time, not just Christmas, and you can listen to wonderful music any time, not just Christmas. It's just that human nature is such that we sometimes need a special stimulus to prioritize all this in a hectic world, and Christmas does just that-and more. Finally, if you have ever looked in to the eyes of a young child contemplating Santa Claus' imminent arrival, and shared that wonder, then you would know that this a wonderful thing to have. Steven, you have some homework to do. You need to find out what Christmas Spirit is. If you do it right, you will have a Happy New Year.

John Mardinly
408-765-2346
877-277-1182

-----Original Message-----
} From: Steven E. Slap [mailto:siksik03-at-comcast.net]
Sent: Monday, January 05, 2004 5:01 AM
To: Mardinly, John; Microscopy-at-sparc5.microscopy.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 01:59:15 2004

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On Mon, 5 Jan 2004, Mike Bode wrote:

} You bring up a good point, though: familiarity with the scale.

And one (little) cent more : I had a look a few weeks ago to the biology
manual
from my daughter (secondary school, french 3°, i. e. 15 years old), an all
the EM and SEM pictures were in pseudo color, whith different color rules
from one picture to an other and without any mention that it was "false
colors" and that the true signal was a monochrome level variation ! I've
than understood why a student asked my once, why we dont't have color
images on the SEM ... " Not enough monney to pay it ?" asked he !
Familarity with a "false" color scale, can be an obstacle to understand
the way the images was obtained (and to understand the image itself,
perheps).

So pseudo color, why not of coarse, but with a color scale along a border
of the picture, like the micron bar, as is often done on AFM images.

J. Faerber
IPCMS
Strasbourg France

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 03:36:16 2004

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John
I was thinking, it's only my family is "so creative". When we came to US
my kids very quickly figured out what to do: ever since we do celebrate
everything. Catholic Christmas, New Year, then Russian Christmas, then
Russian "Old" New Year... The whole point there was to have gifts for
every holiday... As far as I remember my kids also enjoyed some Jewish
holidays when they had school off... I really like you description: "the
spirit of Christmas". I think, good spirit should unify us, not separate
by religious believe... Sergey.

At 11:48 PM 1/5/2004 -0800, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 05:30:26 2004

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Kathleen -

I'll also put in my $.02 worth (Cdn) for Haskris chillers. I've
owned both Haskris and Neslab ones over the years, but what I really like
about the Haskris models I've used is the fact that the water tank/reservoir
has a removable lid, so you can always look inside and visually inspect the
condition of the water. The Neslab one we have now, though reasonably
reliable and all, has a completely sealed water tank with just a narrow
little filler neck, so you can never see what's going on inside.
Interestingly, both companies use the same water pumps supplied by a third
company somewhere in Indiana, I believe. These pumps are rebuildable and
replaceable of course, as are the electric motors that power them, so it's
often possible to keep a chiller running for a very long time before it
actually has to be replaced.
To choose an appropriate model for your particular application you
just need to know how much water (usually gallons/minute) and at what
temperature your particular instrument needs it, then match that up to the
model listing. There's not much point in greatly exceeding the needs of your
instrument with a bigger chiller than necessary, since the motor/pump will
be running constantly anyway.
Some folks will let one big chiller cool several instruments. No
doubt this is pretty cost-effective, but the down-side is apparent when the
chiller craps out and you now have several instruments down instead of just
one.......

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
Sent: Monday, January 05, 2004 12:54 PM
To: Microscopy-at-sparc5.microscopy.com

Hi, all-

We here at the Neurotoxicology Labs at Rutgers University have an
ancient Coolwell chiller for our Zeiss EM 10CA, and it appears to be
dying. Coolwell went out of business years ago, and Zeiss pointed me to
Lytron, Inc. as the company who bought Coolwell's stuff when it went
under. I have tried to contact Lytron online about repairs or a
possible replacement for this chiller, but they don't seem to be paying
much attention to their email. I am going to call them directly, of
course, but what I would like to know is if anyone can recommend another
company or particular chiller model that would be appropriate for our
EM, so that if Lytron continues to blow me off I will have other
sources that I can try.

Hope you all had a happy holiday!

Thanks in advance-
Kathleen Roberts
Principal Lab Technician
Neurotoxcology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 05:50:44 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello everyone,

I'm searching for some decent disposable blades for our Leica Microtome to
get sections of living hearts.
I heard that Feather Blades should do the trick. Has anyone experience with
getting sections of living cardiomyoctes and could give me an address of a
supplier of blades, preferrably in Germany/Europe ?

Thanks

Michael Didié

--
+++ GMX - die erste Adresse für Mail, Message, More +++
Neu: Preissenkung für MMS und FreeMMS! http://www.gmx.net

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 07:29:15 2004

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Although these are debates that should take place somewhere, this is not the forum for them. Unless one can tie a microscope to this line of remarks I would rather not see this on this listserver.

Just my opinion.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, January 06, 2004 2:48 AM
To: Steven E. Slap; Microscopy-at-sparc5.microscopy.com
Cc: Microscopy-at-MSA.Microscopy.Com

Steven;
I was kidding about being a Raelian. I am agnostic. I celebrate the spirit of Christmas, not the religious part. My wife is Turkish, and is a Moslem. She loves Christmas, as does our daughter. We are presently being visited by my wife's mother and sister. Despite the fact that they are both Moslem, and neither of them speaks English, they loved their first Christmas. When my wife celebrates her holidays, I celebrate with her. My brother's wife is Jewish (another mixed marriage-agnostic and Jewish). Their family celebrates both Hanukah and Christmas. Their two kids love having two holidays to celebrate.
As for the spirit of Christmas, I am sorry to hear that it has eluded you. You can give gifts to loved ones any time, not just Christmas. You can try to bring more cheer into peoples lives any time, not just Christmas. You can get together with your family any time, not just Christmas. You can put up special decorations any time, not just Christmas, and you can listen to wonderful music any time, not just Christmas. It's just that human nature is such that we sometimes need a special stimulus to prioritize all this in a hectic world, and Christmas does just that-and more. Finally, if you have ever looked in to the eyes of a young child contemplating Santa Claus' imminent arrival, and shared that wonder, then you would know that this a wonderful thing to have. Steven, you have some homework to do. You need to find out what Christmas Spirit is. If you do it right, you will have a Happy New Year.

John Mardinly
408-765-2346
877-277-1182

-----Original Message-----
} From: Steven E. Slap [mailto:siksik03-at-comcast.net]
Sent: Monday, January 05, 2004 5:01 AM
To: Mardinly, John; Microscopy-at-sparc5.microscopy.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:12:53 2004

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Email: lookerr-at-battelle.org
Name: Ron Looker

Organization: Battelle

Education: Graduate College

Location: Columbus, OH

Question: I am looking for procedures for various microchemical tests
such as protein. Where would be a good resource for finding such
procedures? Thanks you for your time,

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:21:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

How can I resist!

A number of years ago I took a SEM course and I was told the following:

It seems a number of students comment to their professor that they would
like a real time false color display on the SEM. At the time this was not
a inexpensive request or total practical. The next day the students found
a coffee mug full of Sharpie color markers next to the glass CRT screen and
a note welcoming them to "Sharpie Color Technology."

Stay Safe................

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:36:44 2004

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Hi All, I know we are not a theological forum ( and I'm not one, I'm
just a SEM tech)
I agree with the last mail about unifying us.
This is only a way as we can Unify Religion with Science including
Microscopy
Microscopy and Science has discovered a world full of distinctive marks
of intelligent design so we can not deny the chance of the existence of a
creator, so if we want to give honor to him we have to make sure that we
are worshipping him in a good way.

As much of us are from different cultures, we also have to be united,
an example of unity is the language, in this case English. But What about
religions, does exist a language in which we agree about belief? Even
when some religious people have influenced wars, Yes, does exist : is the
True. And I'm not being ambiguous I'm talking about the true about the
date of Christ birth ( where Christmas is originated), the true about
Mexican traditions, I mean all of them over the world, dates, even about
the origin of the live (because religions talk about the creator).
Knowing the true about our own traditions and beliefs and talk about
them to others will unify us.

I agree about giving gifts, I enjoy accepting them and I deeply appreciate
when people give them at any day of the year, without expectation.

Sincerely

Rafael Peńa
SEM Tech
Process Enginering
Tel 83297100
Ext 4721
Monterrey Nl Mexico

----- Forwarded by Rafael Pena/MONT3/MFG/KEMET/US on 01/06/04 08:29 AM
-----

"Tomic, Peter (Peter)" {ptomic-at-agere.com}
01/06/04 07:32 AM

To: {Microscopy-at-sparc5.microscopy.com}
cc: {Microscopy-at-MSA.Microscopy.Com} , (bcc: Rafael Pena/MONT3/MFG/KEMET/US)
bcc: Rafael Pena/MONT3/MFG/KEMET/US
Subject: [Microscopy] RE: RE: Dec. 25

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Although these are debates that should take place somewhere, this is not
the forum for them. Unless one can tie a microscope to this line of
remarks I would rather not see this on this listserver.

Just my opinion.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, January 06, 2004 2:48 AM
To: Steven E. Slap; Microscopy-at-sparc5.microscopy.com
Cc: Microscopy-at-MSA.Microscopy.Com

Steven;
I was kidding about being a Raelian. I am agnostic. I
celebrate the spirit of Christmas, not the religious part. My wife is
Turkish, and is a Moslem. She loves Christmas, as does our daughter. We
are presently being visited by my wife's mother and sister. Despite the
fact that they are both Moslem, and neither of them speaks English, they
loved their first Christmas. When my wife celebrates her holidays, I
celebrate with her. My brother's wife is Jewish (another mixed
marriage-agnostic and Jewish). Their family celebrates both Hanukah and
Christmas. Their two kids love having two holidays to celebrate.
As for the spirit of Christmas, I am sorry to hear that
it has eluded you. You can give gifts to loved ones any time, not just
Christmas. You can try to bring more cheer into peoples lives any time,
not just Christmas. You can get together with your family any time, not
just Christmas. You can put up special decorations any time, not just
Christmas, and you can listen to wonderful music any time, not just
Christmas. It's just that human nature is such that we sometimes need a
special stimulus to prioritize all this in a hectic world, and Christmas
does just that-and more. Finally, if you have ever looked in to the eyes
of a young child contemplating Santa Claus' imminent arrival, and shared
that wonder, then you would know that this a wonderful thing to have.
Steven, you have some homework to do. You need to find out what Christmas
Spirit is. If you do it right, you will have a Happy New Year.

John Mardinly
408-765-2346
877-277-1182

-----Original Message-----
} From: Steven E. Slap [mailto:siksik03-at-comcast.net]
Sent: Monday, January 05, 2004 5:01 AM
To: Mardinly, John; Microscopy-at-sparc5.microscopy.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:36:44 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi All, I know we are not a theological forum ( and I'm not one, I'm
just a SEM tech)
I agree with the last mail about unifying us.
This is only a way as we can Unify Religion with Science including
Microscopy
Microscopy and Science has discovered a world full of distinctive marks
of intelligent design so we can not deny the chance of the existence of a
creator, so if we want to give honor to him we have to make sure that we
are worshipping him in a good way.

As much of us are from different cultures, we also have to be united,
an example of unity is the language, in this case English. But What about
religions, does exist a language in which we agree about belief? Even
when some religious people have influenced wars, Yes, does exist : is the
True. And I'm not being ambiguous I'm talking about the true about the
date of Christ birth ( where Christmas is originated), the true about
Mexican traditions, I mean all of them over the world, dates, even about
the origin of the live (because religions talk about the creator).
Knowing the true about our own traditions and beliefs and talk about
them to others will unify us.

I agree about giving gifts, I enjoy accepting them and I deeply appreciate
when people give them at any day of the year, without expectation.

Sincerely

Rafael Peńa
SEM Tech
Process Enginering
Tel 83297100
Ext 4721
Monterrey Nl Mexico

----- Forwarded by Rafael Pena/MONT3/MFG/KEMET/US on 01/06/04 08:29 AM
-----

"Tomic, Peter (Peter)" {ptomic-at-agere.com}
01/06/04 07:32 AM

To: {Microscopy-at-sparc5.microscopy.com}
cc: {Microscopy-at-MSA.Microscopy.Com} , (bcc: Rafael Pena/MONT3/MFG/KEMET/US)
bcc: Rafael Pena/MONT3/MFG/KEMET/US
Subject: [Microscopy] RE: RE: Dec. 25

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Although these are debates that should take place somewhere, this is not
the forum for them. Unless one can tie a microscope to this line of
remarks I would rather not see this on this listserver.

Just my opinion.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, January 06, 2004 2:48 AM
To: Steven E. Slap; Microscopy-at-sparc5.microscopy.com
Cc: Microscopy-at-MSA.Microscopy.Com

Steven;
I was kidding about being a Raelian. I am agnostic. I
celebrate the spirit of Christmas, not the religious part. My wife is
Turkish, and is a Moslem. She loves Christmas, as does our daughter. We
are presently being visited by my wife's mother and sister. Despite the
fact that they are both Moslem, and neither of them speaks English, they
loved their first Christmas. When my wife celebrates her holidays, I
celebrate with her. My brother's wife is Jewish (another mixed
marriage-agnostic and Jewish). Their family celebrates both Hanukah and
Christmas. Their two kids love having two holidays to celebrate.
As for the spirit of Christmas, I am sorry to hear that
it has eluded you. You can give gifts to loved ones any time, not just
Christmas. You can try to bring more cheer into peoples lives any time,
not just Christmas. You can get together with your family any time, not
just Christmas. You can put up special decorations any time, not just
Christmas, and you can listen to wonderful music any time, not just
Christmas. It's just that human nature is such that we sometimes need a
special stimulus to prioritize all this in a hectic world, and Christmas
does just that-and more. Finally, if you have ever looked in to the eyes
of a young child contemplating Santa Claus' imminent arrival, and shared
that wonder, then you would know that this a wonderful thing to have.
Steven, you have some homework to do. You need to find out what Christmas
Spirit is. If you do it right, you will have a Happy New Year.

John Mardinly
408-765-2346
877-277-1182

-----Original Message-----
} From: Steven E. Slap [mailto:siksik03-at-comcast.net]
Sent: Monday, January 05, 2004 5:01 AM
To: Mardinly, John; Microscopy-at-sparc5.microscopy.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:49:58 2004

Contents Retrieved from Microscopy Listserver Archives
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} The next day the students found a coffee mug full of
} Sharpie color markers next to the glass CRT screen and
} a note welcoming them to "Sharpie Color Technology."

Ah, yes... Interactive computer graphics.

Bruce Girrell

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:54:27 2004

Contents Retrieved from Microscopy Listserver Archives
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To the listserver,
Is there an easier way to make holey
carbon (small 1.5 um) films, other than
steaming formvar/evaporating carbon and
dissolving formvar with solvents? If not
who sells good small holed pure carbon
films.

thanks
mike d

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 08:58:33 2004

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Michael Didié wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

} I heard that Feather Blades should do the trick. Has anyone experience with
} getting sections of living cardiomyoctes and could give me an address of a
} supplier of blades, preferrably in Germany/Europe ?
}
} Thanks
}
} Michael Didié
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 09:40:53 2004

Contents Retrieved from Microscopy Listserver Archives
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Handbook of Chemical Microscopy, Vol II. (1940) E. M. Chamot and C. W. Mason

(1989 Reprints available from McCrone Research Institute, Chicago, IL.)

Karl Hagglund
(513) 634-0146

} From: lookerr-at-battelle.org (by way of Ask-A-Microscopist) on 01/06/2004 02:15 PM
GMT

lookerr-at-battelle.org To: microscopy-at-ns.microscopy.com
(by way of Cc: (bcc: Karl Hagglund-KW/PGI)
Ask-A-Microscopist) Subject: [Microscopy] AskAMicroscopist:
microchemical tests

01/06/2004 09:15 AM

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Email: lookerr-at-battelle.org
Name: Ron Looker

Organization: Battelle

Education: Graduate College

Location: Columbus, OH

Question: I am looking for procedures for various microchemical tests
such as protein. Where would be a good resource for finding such
procedures? Thanks you for your time,

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 10:01:17 2004

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Michael,
Assuming your message has lost a little in translation you might like to
go to the Leica's own web site www.leica-microsystems.com.
They their own (feather) microtome blades but are you actually using a
vibratome?

I have just seen an ad in Microscopy and analysis Jan 2004 for a new live
cell cutting module for their microdissection kit for live tissue
cultures.
(I have no commercial interest)

Gill Brown

GlaxoSmithKline Medicines Research Centre,
STEVENAGE,

""Michael Didié"" {Michael.Didie-at-gmx.de}

06-Jan-2004 11:53

To: Microscopy

cc:
Subject: [Microscopy] Feather Blades

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Hello everyone,

I'm searching for some decent disposable blades for our Leica Microtome to
get sections of living hearts.
I heard that Feather Blades should do the trick. Has anyone experience
with
getting sections of living cardiomyoctes and could give me an address of a
supplier of blades, preferrably in Germany/Europe ?

Thanks

Michael Didié

--
+++ GMX - die erste Adresse für Mail, Message, More +++
Neu: Preissenkung für MMS und FreeMMS! http://www.gmx.net

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 10:04:41 2004

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There is a thoughtful, well-presented magazine called Science & Spirit
that addresses the intersection under discussion, which may be an
appropriate venue for this dialogue. (It might make a good article for
them if anyone wants to pursue it!)

--
***************************************************************
Do not publicly post any of my correspondence without permission

Dee Breger
Mgr. SEM/EDX Facility
Lamont-Doherty Earth Observatory
61 Route 9W
Palisades, NY 10964 USA
T: 845/365-8640
F: 845/365-8155

http://www.ldeo.columbia.edu/micro
Journeys in Microspace (Columbia University Press, 1995)
http://www.lsc.org/antarctica/front.html

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 10:10:32 2004

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Joel-

Well, knowing my boss, he will want to start with the smaller stuff -all
the suggestions of what to check on the Coolwell that you and everyone
else has been sending me (thank you oh so VERY much, everyone!)-and then
when all those have been exhausted, go buy a Haskris. So, if it is not
too much trouble, could you please dig up & send me that Grainger part
number, just in case?

I will check everyone's suggestions and see if they work. At the very
least, it would be nice to be at least somewhat functional until we get
the new chiller in, assuming that the Facilities people here can figure
the Coolwell out without diagrams. :o)

Muchas gracias,
Kathleen
Neurotoxicology Labs
Rutgers University

McClintock, Joel wrote:

} Kathleen,
}
} This sounds real familiar. I suspect the switch is your problem with this chiller. No matter what chiller you have the compressor comes on then off, back and forth. On the front of this chiller right in the middle should be a temp adjustment, don't recall exact wording, but if you take a flat blade screw driver and move it around you should hear the cmpressor come on. If you do watch the temperature and see if it goes down. If so the compressor is working. Your problem then is something is not telling it ot come on properly. In my experience it is the switch from the thermocouple. Coolwells are really sensitive and when operating correctly keep the water temp pretty steady. THe compressor comes off and on, on and off quite often. The thermocouple initiates this. The thermocouple is stuck in the water and a copper line with a flat copper plate at it's end. This plate buts up to a switch. The switch has a little button on it and is pretty sensitive. As the water temp changes the copper swells and shrinks turning the switch off and on respectively. If the switch is sticky or fails things don't work. Doesn't take much as you might imagine the copper moves very little. I can dig up the number for this switch if you need it as I got it through a company called Grainger. Sound like you are going with a new one though. Good luck.
}
} One thing to keep in mind is whether you have a Haskris chiller or coolwell over time maintenance and/or repair will be necessary. Over the years I have called Haskris many times and their phone support is very very good. The only way to get any help on a Coolwell is if you had a time machine and even then I would not be hopeful. The design of Haskris is service friendly.
}
} Joel
}
} -----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
} Sent: Mon 1/5/2004 2:50 PM
} To: McClintock, Joel; Microscopy-at-sparc5.microscopy.com
} Cc:
} Subject: [Microscopy] Re: chiller for Zeiss EM 10CA
}
}
}
} Joel-
}
} I will admit that I am not entirely sure what is wrong with it. All I
} know is that when I turn the 'scope on, it's fine for the first half
} hour or so...then a buzzer goes off-there is no indicator light to say
} what that buzzer is for on the 'scope, but my boss tells me that it's an
} overtemp alarm. If you look at the temp gauge on the chiller, it's
} reading way above the overtemp limit.
}
} There was one occasion when a pump in the house distilled water system
} was dying, and when it was replaced, the 'scope stopped buzzing. Now,
} however, the distilled water system appears to be fine, and the 'scope
} is buzzing again, so I am assuming that it is the chiller.
}
} I did get a local HVAC repair guy in (from the same company that
} resurrected our old cryostat), but he said that he couldn't do anything
} without the refrigeration and other specifications for that chiller. I
} managed to get a couple of diagrams from someone else on this list (his
} name escapes my memory for the moment, but thanks again anyway!), but
} the HVAC guy said that it wasn't enough. As Lytron isn't willing to
} help, I'm going to give up and get a new chiller, as this one is pretty
} old anyway.
}
} Thanks,
} Kathleen
} Neurotoxicology Labs
} Rutgers University

}
} McClintock, Joel wrote:
}
} } Kathleen,
} }
} } I take care of a Zeiss 902 with a coolwell chiller. I have fixed this thing several times. What is the problem with it? Often the temp sensor goes haywire. I have found it is often the switch. I have replaced it for around $7. As others have recommended Haskris is my favorite. If money is tight I may be able to direct you to a used one.
} }
} } Joel McClintock
} } EM Specialist
} } U of Kentucky
} } 859-257-1242
} }
} } -----Original Message-----
} } From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
} } Sent: Mon 1/5/2004 11:54 AM
} } To: Microscopy-at-sparc5.microscopy.com
} } Cc:
} } Subject: [Microscopy] chiller for Zeiss EM 10CA
} }
} }
} }
} }
} }
} } ------------------------------------------------------------------------------
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} } -------------------------------------------------------------------------------
} }
} } Hi, all-
} }
} } We here at the Neurotoxicology Labs at Rutgers University have an
} } ancient Coolwell chiller for our Zeiss EM 10CA, and it appears to be
} } dying. Coolwell went out of business years ago, and Zeiss pointed me to
} } Lytron, Inc. as the company who bought Coolwell's stuff when it went
} } under. I have tried to contact Lytron online about repairs or a
} } possible replacement for this chiller, but they don't seem to be paying
} } much attention to their email. I am going to call them directly, of
} } course, but what I would like to know is if anyone can recommend another
} } company or particular chiller model that would be appropriate for our
} } EM, so that if Lytron continues to blow me off I will have other
} } sources that I can try.
} }
} } Hope you all had a happy holiday!
} }
} } Thanks in advance-
} } Kathleen Roberts
} } Principal Lab Technician
} } Neurotoxcology Labs
} } Dept of Pharmacology & Toxicology
} } Ernest Mario School of Pharmacy
} } Rutgers University
} } 41 B Gordon Rd
} } Piscataway, NJ 08854
} }
} }
} }
} }
} }
} }
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 11:05:49 2004

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Group,
FYI, I have posted the availability of a Kevex Sigma Gold EDS processor and
a Kevex 4855 Digital Beam Control Interface to the surplus equipment list.
Cheers,
Tom

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 11:07:24 2004

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Morning Elizabeth,
If you have Wright's Stain you should do the following.
1. find two glass rods that will reach across a dish/bowl on
which you can support a slide with smear up.
2. Wright's Stain is dissolved in methanol (or should be! - 0.5g
Wright's in 100ml (~ { 3oz) - mixed by 'trituration' (grinding with the
end of a round-bottom test tube) in small amounts of the alcohol until
all is dissolved!). It is delivered on the horizontal dry smear slowly,
with a dropper, so that a puddle of stain covers the smear (& perhaps
the entire slide). Leave for 2.5 min.
3. Add water dropwise to the surface of the stain until IT forms
a puddle that covers about 1/2 of the slide. Then blow gently,
back-and-forth, on the surface of the water-stain until the two are
mixed well. Total time should be about 4.5 min.
4. Rinse the water-stain off the slide in gently running water
and stand the slide against an inverted glass to dry - with smear down.
[If at home, DO ALL staining, rinsing and drying on aluminum foil. The
dye will stain Formica surfaces. Removal requires another email.] When
completely dry, a coverglass can be applied using appropriate care with
a permanent mountant.
5. You can also view the smear directly with an oil immersion
lens (that's the way it is done in pathology labs). Oil is placed
directly on the smear and then differential counting is performed.
Count 100 white blood cells, identifying each, and record the
distributions. A normal smear will show something like the following:
1 basophil, 2 eosinophils, 38 neutrophils (each of the previous
identified by cytoplasmic granules that are dark blue, bright red and
the latter pink with a segmented nucleus respectively), and 59
lymphocytes (small cells with a round nucleus and a thin rim of
cytoplasm). All red blood cells should be orange and without nuclei.

The theory is this.
Methylene blue (base) and eosin (acid) are mixed in water (1:1) and
combine to form a precipitate. The precipitate is dried and then
dissolved(?) in methanol. After the dye thoroughly penetrates the cells
in the smear, the water causes the precipitate to dissociate (based on
mass action). The methylene blue and eosin are then simultaneously
accessible to cellular constituents and are attracted according to their
individual affinities. The rinse in excess water then removes all
unbound dye. Applying the dyes separately requires much more work and
gives much less satisfactory results. The above dyes belong to a group
of blood dyes called "Romanovsky Stains".

Coverslipping.
If you do not have an oil immersion lens, you can do the following
so that you can view cells with a 40X dry objective. This will work
though you will have to remove the coverslip and the oil to store the
smear. To keep an oiled smear, absorb the excess oil with the tip of a
piece of paper towel.

Try this site:

http://www.mcl.tulane.edu/classware/pathology/Krause/Blood/Blood.html

DO NOT use alcohol (will leach dyes!) to remove the rest. Wrap the
slide once with good quality paper and NO Scotch tape!

DO NOT try to look at the cells when dry. The image will be saturated
with diffraction rings that arise through the interaction of the
microscope light and the curved surfaces of the cells - which are whole
in a smear (remember?).

Hope this helps,

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:letitsnow-at-antelecom.net]
Sent: Monday, January 05, 2004 5:38 PM
To: microscopy-at-ns.microscopy.com

------------------------------------------------------------------------
--

Email: letitsnow-at-antelecom.net
Name: Elizabeth Colvin

Organization: Homeschool

Education: 9-12th Grade High School

Location: Pearblossom, CA-L.A. county

Question: I have obtained several unstained blood smears. I have
Wright's stain and methylene blue available. Can you please tell me
how long to leave the stain on the slide before rinsing. And do I
rinse with distilled water. Thank you.

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 11:58:33 2004

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All right! I can't TAKE it anymore!

Please, PLEASE, can the next person to add to this thread spell PSEUDO correctly!
..please...
(if it's not too much to ask...)
(whimper)
:-)

Mike O'Keefe

Bruce Girrell wrote:

} ------------------------------------------------------------------------------
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}
} } The next day the students found a coffee mug full of
} } Sharpie color markers next to the glass CRT screen and
} } a note welcoming them to "Sharpie Color Technology."
}
} Ah, yes... Interactive computer graphics.
}
} Bruce Girrell

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 12:12:03 2004

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Our lab recently began using the "New Formulation" Kodak Electron
Microscope Film 4489 and employed a number of tips for developing this
film
which we retrieved from the Listserver archive commencing Jan 2003 .

We use a manual processing method (no nitrogen-burst agitation).
Although
we have now managed to essentially eliminate the background fog and
"mottled" appearance, the negatives appear darker (denser) than with
the previous formulation.

These darker negatives can be printed satisfactorily in the darkroom.
However, we digitize our images and archive them on-line. With the
"New
Formulation" film and denser negative we have noticed scan lines in our

digitized images. The darker the negative, the more apparent the scan
lines.
We are currently investigating the plate camera emulsion selector
positions on
our TEM with the hope that concurrent adjustments of exposure
time/emulsion setting/darkroom technique will result in a 'less dense'
negative.

Has anyone else run in to this problem when digitizing their "denser"
negatives? Does anyone have any thoughts beyond what we are trying?

Thank you in advance for your assistance.

Catherine Powell

Catherine Powell, Ph.D.
Division of Surgical Pathology
Department of Laboratory Medicine, Saint John Regional Hospital
P.O. Box 2100, Saint John, NB Canada E2K 4G9
phone (506) 648-7183 FAX (506) 648-6514
email powca-at-reg2.health.nb.ca

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 12:55:28 2004

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Hi,

We've been through the ringer with this film and have finally come to
terms with it. However, during the last three changes of D-19 developer
we have gotten significantly darker negatives (including the data bar,
which is added by the scope independently of negative exposure in our
JEOL 1200EX), for some reason we don't yet understand. We didn't change
anything in the way we mixed our developer or exposed our films, and we
have no reason to think the developer has been changed. We solved this
in the meantime by diluting the developer, since the first batch of
negatives had already been exposed and it's not a good idea to shorten
already short developing times---four minutes in our case. We added
about 25% more water (i.e., another quart per gallon of developer), ran
a couple test negatives, then proceeded normally with regard to
time/temperature/agitation. This worked well for us. Of course,
changing developer dilutions can affect the tonal response of films, but
in this case the results were fine. If you try this, always run your
own tests, of course.

We've had no problems with "scan lines". That's puzzling. They must be
coming from the scanner, itself, which maybe indicates that some of the
scanning elements (sorry, I forget the terminology---are they called
pixels?) aren't doing their thing and are causing lines in the digitized
image.

Good luck.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

-----Original Message-----
} From: Dr. Catherine Powell [mailto:POWCA-at-reg2.health.nb.ca]
Sent: Tuesday, January 06, 2004 12:15 PM
To: Microscopy-at-MSA.Microscopy.Com

Our lab recently began using the "New Formulation" Kodak Electron
Microscope Film 4489 and employed a number of tips for developing this
film which we retrieved from the Listserver archive commencing Jan 2003

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 13:19:33 2004

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Catherine,

Regarding the denser negs, anytime you change film in any camera system you
usually need to re-calibrate camera exposure and film development. Sounds
like you have done that and are getting a less dense neg that can be nicely
digitized.

Regarding the scan lines flaw, you didn't mention if you are using an actual
negative scanner, or a flatbed scanner to digitize the negs. But in either
case, you may just need to lubricate the moving parts. In my case, I use a
UMAX Vista-S8 and about once a year I need to pull the glass surfaces off to
get inside and lubricate the metal bar that the scanner heads move on. They
just get dry, so then they don't slide smoothly and "skip" a line here and
there. Use a clean lint-free cloth with a dab of a fine oil on it, or 3-in-1
oil is what I use. In fact, I just did this lube job yesterday, and it
worked!

Good luck!

Gib
--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra

} Our lab recently began using the "New Formulation" Kodak Electron
} Microscope Film 4489 and employed a number of tips for developing this
} film which we retrieved from the Listserver archive commencing Jan 2003 .
}
} We use a manual processing method (no nitrogen-burst agitation).
} Although
} we have now managed to essentially eliminate the background fog and
} "mottled" appearance, the negatives appear darker (denser) than with
} the previous formulation.
}
} These darker negatives can be printed satisfactorily in the darkroom.
} However, we digitize our images and archive them on-line. With the
} "New Formulation" film and denser negative we have noticed scan lines in our
} digitized images. The darker the negative, the more apparent the scan
} lines.
} We are currently investigating the plate camera emulsion selector
} positions on
} our TEM with the hope that concurrent adjustments of exposure
} time/emulsion setting/darkroom technique will result in a 'less dense'
} negative.
}
} Has anyone else run in to this problem when digitizing their "denser"
} negatives? Does anyone have any thoughts beyond what we are trying?
}
} Thank you in advance for your assistance.
}
} Catherine Powell
} Catherine Powell, Ph.D.
} Division of Surgical Pathology
} Department of Laboratory Medicine, Saint John Regional Hospital
} P.O. Box 2100, Saint John, NB Canada E2K 4G9
} phone (506) 648-7183 FAX (506) 648-6514
} email powca-at-reg2.health.nb.ca

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 13:32:52 2004

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I haven't had any issues scanning in the darker negatives. We have an
Agfa Duoscan T2500 that works well enough with these newer negatives at
1000 and 2500 ppi (the two resolutions I've tried). Before the holiday
break I put together a group of images (digitally scanned ones) that had
both new and old negatives included with no discernable differences
between them. Other than having the scanner support discontinued its
been a great and reliable scanner for lecture slides and TEM negatives
(if anyone has a driver for it that works with the latest Mac OS 10.3 I
would be very interested in hearing about it). As you have mentioned,
it would probably be worth trying a emulsion setting series to see if
that improves your results. But alas I cannot say that I've tried this
yet to attempt to get the old and new density similar on the negatives.

HTH,

Geoff Williams
Microscopy Facility Supervisor

Central Michigan University Biology Department Microscopy Facility
http://www.cst.cmich.edu/centers/microscopy/

} -----Original Message-----
} From: Dr. Catherine Powell [mailto:POWCA-at-reg2.health.nb.ca]
} Sent: Tuesday, January 06, 2004 1:15 PM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] TEM -Need help with scanning EM film 4489
}
}
}
}
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} ----
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
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} -----
}
} Our lab recently began using the "New Formulation" Kodak Electron
} Microscope Film 4489 and employed a number of tips for developing this
} film
} which we retrieved from the Listserver archive commencing Jan 2003 .
}
} We use a manual processing method (no nitrogen-burst agitation).
} Although
} we have now managed to essentially eliminate the background fog and
} "mottled" appearance, the negatives appear darker (denser) than with
} the previous formulation.
}
} These darker negatives can be printed satisfactorily in the darkroom.
} However, we digitize our images and archive them on-line. With the
} "New
} Formulation" film and denser negative we have noticed scan lines in
our
}
} digitized images. The darker the negative, the more apparent the scan
} lines.
} We are currently investigating the plate camera emulsion selector
} positions on
} our TEM with the hope that concurrent adjustments of exposure
} time/emulsion setting/darkroom technique will result in a 'less dense'
} negative.
}
} Has anyone else run in to this problem when digitizing their "denser"
} negatives? Does anyone have any thoughts beyond what we are trying?
}
} Thank you in advance for your assistance.
}
} Catherine Powell
}
}
}
} Catherine Powell, Ph.D.
} Division of Surgical Pathology
} Department of Laboratory Medicine, Saint John Regional Hospital
} P.O. Box 2100, Saint John, NB Canada E2K 4G9
} phone (506) 648-7183 FAX (506) 648-6514
} email powca-at-reg2.health.nb.ca

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 13:34:03 2004

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Thanks, Mike, for pointing out the proper spelling. The correct pronunciation
of â€psuedoâ€™ is as in â€blue psuedo shoes.â€™ And thereâ€™s nothing all that
astonishing about using colored markers on the screen. When we first introduced a
computer (one of the original upright Macs) in the department office a couple
of decades ago, to a secretary firmly set in the old ways, we had to take
turns each night cleaning the whiteout correction fluid off the screen. {;-)

Anyway, to the use and abuse of pseudo color;...

It is certainly true that human vision can only distinguish a few dozen
shades of grey brightness on a display screen, as compared to a few hundred colors.
Note that both of these values are far less than the 256 shades of brightness
or â€śmillionsâ€ť of colors that the hardware typically controls. It is also
true that trying to direct someoneâ€™s attention to the â€śkind of darkish grey
spotâ€ť is a lot less helpful than â€śthe yellow-orange spotâ€ť in an image (but of
course, human words for colors arenâ€™t terribly consistent or widely agreed,
either - look at any set of paint chips in the turquoise-teal-seagreen-etc.
family). Pseudo- or false-color certainly has some valid uses. But it is also easily
misunderstood, widely abused, and often hides more in the image than it
reveals. And if the viewer is one of the 5-10% of men (or the very tiny percentage
of women) who have defective color vision, it is inappropriate in any case.

Firstly, of course, the table must be shown along with a numerical scale that
translates it. But even then, simple spectrum lookup table is rarely if ever
a good choice. The problem is that the table is typically constructed with
uniform steps in hue, going around the color wheel. But human vision is notably
insensitive to changes in hue in the green part of the spectrum, and much more
so at the red and blue ends and through the red-to-blue purples. A
perceptually uniform hue scale (which I have never seen used) would stretch these out and
compress the greens and could probably produce more than a hundred
discernible colors.

More colors could be seen if they were NOT fully saturated. Changing
saturation and hue in a spiral pattern, or also altering brightness along with hue and
saturation, can produce color tables that varied in a gradual way and
produced greater ability to distinguish changes. The gradual part is important - if
the colors jump around too much in discontinuous ways, the image is badly
broken up (camouflaged, in effect) and the overall sense of structure, the gestalt
of the image, is hidden. To some extent this happens even with a good, gradual
table. The use of the â€śheatâ€ť or â€śthermoâ€ť scale is an example of a gradual
and visually attractive scale, which does not break up the content of the
image. But it does not actually add very much to the ability to visually
distinguish small changes - perhaps a 20-40% improvement over straight grey scale (which
is why color tints are also used in photographic printing, to gain the same
increase). Note that the brightness increases monotonically in this scale, and
that it is by contributing more steps at the dark end that the increase is
obtained.

For selected purposes, carefully constructed color scales can be useful to
help the viewer perceive subtle differences or make comparisons from one part of
an image to another. But they need to be documented, and in most cases it is
also important to show the original data as well in case the color scale can
produce misinterpretation or hide other information.

It has been my experience that people are not generally assisted very much by
pseudo color scales, as compared to other ways to reveal subtle detail. One
of the best of these is to render the surface with elevation representing the
original grey scale value. We have millions of years of evolution in our brain
wiring that knows how to interpret surface images, in terms of shape and
roughness. Using computer graphics to generate properly rendered images with
correct perspective, and adjustable viewpoints, surface characteristics, and
illumination is easy with current technology and communicates very effectively. The
AFM folks use this trick too, along with color scales, although in most cases
in only limited ways.

John Russ
(see www.DrJohnRuss.com for a schedule of upcoming workshops on image
analysis)

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 13:50:49 2004

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The recent thread about the use and abuse of pseudo color is only one of many
issues that have to do with an important topic that underlies just about
everything that we as microscopists do - namely, we LOOK AT images. But while we
are typically very concerned with the performance and specifications of our
microscopes, we take for granted the performance of our visual systems, to our
peril.

Over the past 5 years or so I have been invited several times to give a talk
on human vision and how it impacts what microscopists see (and fail to see) in
images. At the repeated urging of many people, Iâ€™ve prepared the lecture in
written form. Anyone who wants to read it can download the "Seeing the
Scientific Image" pdf file from my website (www.DrJohnRuss.com). If someone thinks
there is a logical place to publish it (too long for Microscopy Today, and not a
research paper for Microscopy and Microanalysis) please let me know.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 14:12:58 2004

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Tina-

Silly me, in all my crabbing about this chiller, I didn't give the
model? The model # is SE-075W CZ. I got some diagrams from Eckhart
Dorneich, and a manual is on the way from Joel McClintock (thank you
both!), but I'll take yours too, if they match my chiller. I figure you
can never have too much information, and it's always good, in this lab,
to have extra copies. :o)

Thank you very much-
Kathleen
Neurotoxicology Labs
Rutgers University

Tina Carvalho wrote:

} Hi-
}
} What model chiller do you have? I might have the wiring and plumbing
} diagrams.
}
} I have a 10/A and have struggled to keep the chiller going. The scope was
} down for a couple of years - oil and then water in the column! - while we
} used our new LEO 912 EFTEM. The expensive new instrument can be very
} frustrating, and was down once for nearly 5 months! So we got the 10/A
} going again, including the chiller. We all had forgotten what a gem it is,
} and right now I'd sell the new one and keep the old if I had a
} choice.
}
} We have Hakris chillers on our other two instruments, and they are
} fine. We got the very first one that Haskris built for Zeiss/LEO, and they
} had a fit trying to include both a pressure and flow gauge plus that
} interlock that keeps it going to cool down the diff pump after you turn
} off the scope, but they are quite used to it, now. They're pretty reliable
} and, fortunately, not prone to that temperature sensor screwing up like
} the Coolwell.
}
} Over the years I've found out there are a whole lot of closet Zeiss 10s
} out there - the most reliable backup even if you have a fancy new
} instrument! Keep it going. My next trick is to outfit it with a digital
} camera.
}
} Aloha,
} Tina
}
} ****************************************************************************
} * Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
} * Biological Electron Microscope Facility * (808) 956-6251 *
} * University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
} ****************************************************************************
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 15:03:50 2004

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Dear Catherine,
I found the new formulation film was more sensitive and adjusted my auto
settings in the TEM to compensate.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "Dr. Catherine Powell" {POWCA-at-reg2.health.nb.ca}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Tuesday, January 06, 2004 10:14 AM

Scanning very dense negatives can cause problems related to the scanner if
your scanner is using a CCD rather than a PMT. With a CCD you can not
crank up the current to boost the signal like you can with a PMT. The
result is that there is not enough light i.e. signal getting to the camera
array. If that is the case then you must either slow down the scan speed
so that the camera can collect enough signal or if this is impossible make
your negatives less dense. Our ZI Photoscan 2000 has problems with
negatives above an OD of 2.3 or so. Above this lines like what you
described appear. I hope this helps. Good luck.

Bob Grassucci

At 02:14 PM 1/6/04 -0400, Dr. Catherine Powell wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Robert Grassucci
Howard Hughes Medical Institute at The Wadsworth Center
Empire State Plaza
Albany, NY 12201-0509
Phone: (518)474-5821
Fax: (518)486-2191
E-Mail: bobg-at-wadsworth.org

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 17:31:44 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (alchung-at-ucla.edu) from
http://www.msa.microscopy.com/Ask-A-Microscopist.html on Tuesday,
January 6, 2004 at 16:51:57
---------------------------------------------------------------------------

Email: alchung-at-ucla.edu
Name: Albert Chung

Organization: UCLA

Education: Graduate College

Location: Los Angeles, CA USA

Question: I am having issues with the silicon monoxide film tearing
in the TEM. I have called Ted Pella about this problem and they are
making a new batch as we speak, but I have about 50 silicon monoxide
films on copper grids for which I cannot use. Any suggestions on how
to approach this problem is greatly appreciated. I am operating the
JEOL 100CX and the typical current saturation is about 80 mA.

If you need additional information, please let me know.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 18:13:31 2004

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There is another one:
you may bombard thin nylon film by some heavy ions (argon may be good) in
the accelerator. It will produce very uniform holes. The size of holes
strictly dependent from the energy and type of particle used. But, still:
you need to eveporate carbon over and dissolve nylon (have no idea how to
do so). As a matter of fact this technology widely used to produce filters
for ultrafiltration.

Sergey

At 07:03 AM 1/6/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 6 19:20:48 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

-- [ From: Garber, Charles A. * EMC.Ver #3.1a ] --

Albert Chung wrote:
========================================================================
Question: I am having issues with the silicon monoxide film tearing in the
TEM. I have called Ted Pella about this problem and they are making a new
batch as we speak, but I have about 50 silicon monoxide films on copper
grids for which I cannot use. Any suggestions on how to approach this
problem is greatly appreciated. I am operating the JEOL 100CX and the
typical current saturation is about 80 mA.
========================================================================
Support films of SiOx can be too thick or too thin or could have other
features about them that render them unstable in the electron beam. This is
of course exactly the same for carbon coated grids. That is why it is
imperative to have in-house, as part of the grid coating process, a TEM for
batch inspection purposes so that the customer does not end up being
responsible for their own QC. And does not end up preparing a large number
of grids only to find them unusable.

In the case of carbon replica films that were prepared but which are too
thin, we have in the past, been able to resurrect them by applying another
coating of carbon to strengthen them and to make grids that were once
unstable, now stable. We have never done this with SiOx filmed grids but in
theory, it might work the same way.

Disclaimer: SPI Supplies produces SiOx firmed grids as a part of our
business and to our knowledge, we have not had any problems with film
stability in the electron beam. On occasion, we do make a batch that
flunks our own in-house TEM inspection process but those grids never make it
into the hands of customers.

Chuck

PS: Remember that we are 100% paperless and the only way we can keep track
of this kind of correspondence is if you reply using the reply feature of
your e-mail software. That way the entire string of correspondence will be
in one place.

============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 00:09:32 2004

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Catherine;
One of my favorite web sites, Imaging Resources http://www.imaging-resource.com
has reviewed numerous film scanners. Scanning extremely dense film has always been an acid test for a scanner. The following link is to a negative scanned with a Minolta Dimage Scan Elite II Film & Slide Scanner that failed the acid test in some dark regions, and the effect there seems similar to what you describe. The site tests many other scanners with the same negatives, and many do not exhibit this artifact.
http://www.imaging-resource.com/SCAN/DSEII/DSETRAA602PS.HTM

John Mardinly
Intel

-----Original Message-----
} From: Dr. Catherine Powell [mailto:POWCA-at-reg2.health.nb.ca]
Sent: Tuesday, January 06, 2004 10:15 AM
To: Microscopy-at-MSA.Microscopy.Com

Our lab recently began using the "New Formulation" Kodak Electron
Microscope Film 4489 and employed a number of tips for developing this
film
which we retrieved from the Listserver archive commencing Jan 2003 .

We use a manual processing method (no nitrogen-burst agitation).
Although
we have now managed to essentially eliminate the background fog and
"mottled" appearance, the negatives appear darker (denser) than with
the previous formulation.

These darker negatives can be printed satisfactorily in the darkroom.
However, we digitize our images and archive them on-line. With the
"New
Formulation" film and denser negative we have noticed scan lines in our

digitized images. The darker the negative, the more apparent the scan
lines.
We are currently investigating the plate camera emulsion selector
positions on
our TEM with the hope that concurrent adjustments of exposure
time/emulsion setting/darkroom technique will result in a 'less dense'
negative.

Has anyone else run in to this problem when digitizing their "denser"
negatives? Does anyone have any thoughts beyond what we are trying?

Thank you in advance for your assistance.

Catherine Powell

Catherine Powell, Ph.D.
Division of Surgical Pathology
Department of Laboratory Medicine, Saint John Regional Hospital
P.O. Box 2100, Saint John, NB Canada E2K 4G9
phone (506) 648-7183 FAX (506) 648-6514
email powca-at-reg2.health.nb.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 06:34:24 2004

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Posting this for a friend.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

Hi All,

I am doing some housecleaning & have the following EDS Systems free to
anyone:

Kevex 8000
Kevex Delta
PGT System 4
Tracor 5500

Happy New Year All.

Earl Weltmer
eweltmer1-at-cox.net
Scanservice Corp.

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 08:12:53 2004

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Hi all

We have too 2 Kevex Delta avavaible, one complete, with detector (10mm2,
138 eV, warm, but was working in July)), the other only the electronic,
for spares, with 8" and 5"1/4 Bernouilli.

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 08:23:57 2004

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If anyone has a mechanical lab balance they would like to dispose of, I
could use one. I collect/repair antique phonographs as a hobby and would
like to be able to true up governor weights from time to time. I've looked
at E-bay but I am leery since, if a balance moves up and down, the general
public thinks it works. Some units offered are missing parts. etc.

Thanks,

Ron

-----Original Message-----
} From: qualityimages [mailto:qualityimages-at-netrax.net]
Sent: Wednesday, January 07, 2004 7:37 AM
To: Microscopy

Posting this for a friend.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

Hi All,

I am doing some housecleaning & have the following EDS Systems free to
anyone:

Kevex 8000
Kevex Delta
PGT System 4
Tracor 5500

Happy New Year All.

Earl Weltmer
eweltmer1-at-cox.net
Scanservice Corp.

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 09:29:29 2004

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Hi Listers

As many of you may know I run a training organisation that travels world
wide spreading the word on SEM, TEM and EDS operation. I also have a deep
interest in "Quality in Electron Microscopy"as those who picked up our paper
last year would know?

Now to the point. Once again I am picking up respected journals and finding
examples of what I would call poor microscopy, but in truth it also
demonstrates poor quality control!

To bring one image to mind. The micrograph is of a structure which is
described as being an example of a smooth surface on a biological material.
But, the micrograph was taken at 20kV, where the vast majority of the
information will have come from beneath the surface softening the true
surface detail.

First to remove the training aspect . Operators of SEM should be taught that
by manipulation of kV and working distance one may subdue or enhance surface
features. To use more than 10kV on most biological samples is asking for
sub surface detail, ignore this and comments on surface irregularities are
null and void in my mind. (I have to say I would probably try to use 2 to
5kV if the microscope used was produced in the last 15 years!)

Now the quality aspect. By the time a paper is published a number of steps
should have been taken. Working backwards, the publisher should have the
paper vetted by knowledgeable scientists who would be able to pick out the
problems that I see and have them corrected prior to going to print. Next
back in the chain is the laboratory that was involved with the scientist;
did they check the quality of the work leaving their EM unit? Stepping back
again did the scientist take the micrographs or did they receive help?
Either way the training of staff and operators should overcome this type of
problem! But if the results the staff and visiting operators produce are
not assessed how do you know that their training is inadequate?

As the pressure to perform increases and funding decreases only the cream of
our laboratories will remain. In industry there is no question about
following rigid "Quality" procedures and it is not too far off that this
will hit the world's EM units too! I know that this is my baby but is it
not about time that we woke up to these facts?

There is an area where I believe we have room for discussion; what do you
think?

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0) 7711 606967
www.emcourses.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 10:49:04 2004

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Steve,
Your post (whose spirit I agree with totally) prompted a
question. If I have a biological sample sputter coated with metal,
isn't all the contrast coming from the metal? Does the underlying
carbon based material scatter anything much? If the carbon isn't
scattering much then wouldn't the problem you used for illustration
matter only at high mags where distances on the order of the coat
thickness are being resolved?

As ever,
Tobias

} ------------------------------------------------------------------------------
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--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
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/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 12:39:30 2004

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Steve,
I agree entirely with you in that training (perhaps educating is a
better word) is key to good and reliable results. The example you sited
happens constantly. I take great pains to not only lecture about, but prove
through lab exercises, the effects that varying microscope parameters have
on the final image.

Unfortunately many "trained" people ask to use our facility and are denied
because their training was inadequate. They are either retrained so they
have the theory to go along with twiddling the knobs or rely on our
"service" option (trained staff does the actual imaging). The reputation of
our facility is very important.

We cannot guarantee to get perfect results with every research system on the
first try but we do our best and learn from our mistakes. At least if we
understand our instruments we can concentrate on sample prep to get the best
possible final results...not what the investigator thinks is there but what
is ACTUALLY there.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 1/7/04 9:42 AM, "Steve Chapman" {protrain-at-emcourses.com} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Hi Listers
}
} As many of you may know I run a training organisation that travels world
} wide spreading the word on SEM, TEM and EDS operation. I also have a deep
} interest in "Quality in Electron Microscopy"as those who picked up our paper
} last year would know?
}
} Now to the point. Once again I am picking up respected journals and finding
} examples of what I would call poor microscopy, but in truth it also
} demonstrates poor quality control!
}
} To bring one image to mind. The micrograph is of a structure which is
} described as being an example of a smooth surface on a biological material.
} But, the micrograph was taken at 20kV, where the vast majority of the
} information will have come from beneath the surface softening the true
} surface detail.
}
} First to remove the training aspect . Operators of SEM should be taught that
} by manipulation of kV and working distance one may subdue or enhance surface
} features. To use more than 10kV on most biological samples is asking for
} sub surface detail, ignore this and comments on surface irregularities are
} null and void in my mind. (I have to say I would probably try to use 2 to
} 5kV if the microscope used was produced in the last 15 years!)
}
} Now the quality aspect. By the time a paper is published a number of steps
} should have been taken. Working backwards, the publisher should have the
} paper vetted by knowledgeable scientists who would be able to pick out the
} problems that I see and have them corrected prior to going to print. Next
} back in the chain is the laboratory that was involved with the scientist;
} did they check the quality of the work leaving their EM unit? Stepping back
} again did the scientist take the micrographs or did they receive help?
} Either way the training of staff and operators should overcome this type of
} problem! But if the results the staff and visiting operators produce are
} not assessed how do you know that their training is inadequate?
}
} As the pressure to perform increases and funding decreases only the cream of
} our laboratories will remain. In industry there is no question about
} following rigid "Quality" procedures and it is not too far off that this
} will hit the world's EM units too! I know that this is my baby but is it
} not about time that we woke up to these facts?
}
} There is an area where I believe we have room for discussion; what do you
} think?
}
} Steve Chapman
} Senior Consultant Protrain
} Electron Microscopy Training and Consultancy World Wide
} Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0) 7711 606967
} www.emcourses.com
}
}
}

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Put into TEM at low mag but still with an objective aperture in
place, and 100 kV. Really spread the beam and turn up slowly. You may
find that by gradually increasing the electron dose, you'll "harden"
the film. This approach certainly works with formvar films and
biological resin sections but I've never tried it with silicon
monoxide, so I can't guarantee it'll work.
--
Larry Stoter
NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 15:12:05 2004

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Happy New Year

Does anyone have a circuit diagram for an oldish Leitz microscope lamp power supply
Type 301-314.001?

It's a beige box with an analog voltmeter, a mains switch, and a brighness adjust knob
on the front panel.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 15:24:34 2004

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Email: jamielange-at-wi.rr.com
Name: jamie lange

Organization: university of wisconsin

Education: Graduate College

Location: milwaukee, wi. usa

Question: we used a spurr's resin prep on a sample of nematodes,
after staining and heat-fixing the sections, we see dark ribbon-like
structures on several specimens. Are these artifacts caused by air
bubbles and can they be avoided? thank you,
jamie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 15:59:17 2004

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Re: Silicon monoxide film

We believe the problem may have been caused by weak film. Silicon monoxide
film should be as fresh as possible. Some of our customers have requested
thicker coatings but this doesn't help. We make our film up the day it is
requested by the customer to insure this problem doesn't occur. We suggest
you purchase the minimum amount required at one time because new batches can
be made up in a day or so.

John Arnott
Disclaimer: Ladd Research produces a wide variety of EM supplies including
substrates, such as silicon monoxide.

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com
----- Original Message -----
} From: "Larry Stoter" {larry-at-cymru.freewire.co.uk}
To: "by way of Ask-A-Microscopist" {alchung-at-ucla.edu} ;
{Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, January 07, 2004 3:27 PM

Steve, et al.:

I agree there is a definte problem in terms of (some of) the microscopy
work being used and published. Steve hits a very good case where failure to
understand the technique can easy lead to poor data. (by microscopy I mean
in the broadest sense: SEM, TEM, LM, SPM, etc. . . Anyone dealing with
molecular biolgists labling molecules and wanting to use a confocal
microscope already knowing exactly what kind of "picture" they want to get
knows what I mean)

One of the really frightening aspects is that very very few people wish to
learn microscopy - become microscopists - today. I have been watching this
trend for several years now where users (students and faculty in my case)
simple want images. They want to push a button out comes an image - that's
all. If they could have the microscope automatically load the sample that
would be even better. Now granted there are times when a simple click image
will sufice - but more and more often researchers are failing to realize how far
they are trying to push the capabilities of a microscopy technique. I have
been told specifically they do NOT want to learn the microscope they want an
image. And then you try and turn around and tell them the data they are
collecting is bad science?

} Next back in the chain is the laboratory that was involved with the
} scientist; did they check the quality of the work leaving their EM unit?
} Stepping back again did the scientist take the micrographs or did they
} receive help? Either way the training of staff and operators should overcome
} this type of problem! But if the results the staff and visiting operators
} produce are not assessed how do you know that their training is inadequate?
}

There is a time you can attempt to argue with the "users" over scienfic
quality, but running and EM Lab you can not dictate it - certainly not in
academia, and not even in industry - yes, you can be asked for an evaluation
of the data (and that is what peer review also does) but no one can really
control what the data is used for after it leaves the lab.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 16:48:19 2004

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We are having one of those debates that we microscopists seem to obsess
about. The question is whether to store our saturated uranyl acetate
solution (in dH2O) at room temp or at 4 C. Opinions, especially those
backed by data, would be welcome. Happy New Year. Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 17:36:49 2004

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Richard

With huge headache I've established procedure in my Lab that everyone, who
uses equipment in the Lab should go through mandatory training. Without
this training, person just could not enter the facility (digital lock). My
training course includes intense training on data collection,
interpretation and sample preparation. So, it does not insure from the
"bad science", but at least I felt people knows what they doing. It means,
if they will present "bad data" I know, they did it on purpose... My
course is about week long (2h/day) and people's reaction are very
different. Nevertheless, I noticed that majority of the users finally
enjoyed "good electron microscopy", because it save them time and the
quality of their images is good (and confidence is great). In general, I
do agree: people becomes more and more "lazy" - they want to have results
doing nothing (best scenario - machine will do). It's very pity and made
me very skeptical on quality of many data published. Sergey

P.S. Knowledge is power.

At 02:20 PM 1/7/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 17:48:07 2004

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More important - to store in the dark! At +4oC you will have lower
concentration because of solubility. I prefer to store most of the
chemical solutions at cold temperature.
Sergey

At 02:49 PM 1/7/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 7 17:54:43 2004

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If it makes all of you feel any better, the phenomenon of users not
wanting to learn how to use something, just wanting the results, is not
limited to microscopy, and is a dangerous trend. This trend is
ironically aided by the very advancing technologies that make truly
understanding the theories and principles of what is happening more
important than ever.

Too many devices, instruments and other systems have become "too easy to
use". The advances in human interfaces, automation, computer controls,
etc. have made it very easy for just about anyone to get results. The
danger is that there is no way for someone who doesn't truly understand
what's going on to know if the results are meaningful or not. "I got
the answer, and it's what I was expecting, so it must be right!"

The problem is also not limited to "sophisticated" technology. We have
users who no longer know that there is a darkness adjustment on a copy
machine, much less how to use it. Not that long ago, you couldn't get
two copies in a row to turn out without tweaking the adjustment. If
someone does take the thing off "auto" and sets it dark, everyone else
thinks the thing is broken...

If someone finds a "real" cure for this phenomenon, please share it with
the world, because the problem is pretty universal.

John W. Raffensperger, Jr.
IS Manager
Helwig Carbon Products, Inc.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 03:26:44 2004

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I fully agree with this fact that the problem is universal,
and it is not only limited to microscopy. However, before one
finds the "cure for this phenomenon", one should look for the cause
of this problem.

If the new generation, i.e. the younger students and others, "are just
wanting results", is it not the consequence of the ATTITUDE OF THE
LARGE MAJORITY of those who trained them?

Those who trained the last two generations are now collecting the
results of what they have done.
The biggest reference for this generation is having rapid success,
which means gaining large amounts of money and if possible a quick fame.

No university professor considers the students for their interest for
science and their will to do something for the sake of humanity.
They rank them on their good marks, without worrying about how they
obtained it. And even if they do so, it is to REPRIMAND the student and
not for TEACHING them the importance of honesty.
A large percentage of students learn just to obtain a good mark, without
thinking about why's and how's. And those few who do, are not
appreciated
by the professors, may be since they need more time that is not
available.

A professorship is the art of teaching many things including highest
human values to the students, I can not name many who have done that, or
even
have thought to do it. If they do not reflect such thoughts, at least
they
should avoid to discourage the very few who do have such values (and
have truly come to learn something that can be helpful for the society)
by treating them as naives and dealing with irony with them.

Some students tell me that the science professors are so arrogant that
the students have no more appeal for scientific branches.
} From my discussions with some undergraduate science students, their
feeling is
that if they go for science in their graduate school they could ruin
their future and they will loose the chances of success!

I agree that the danger is real and from my understanding the solution
to the problem is to reverse the trend from now on by changing the
teaching philosophy. However, one should have the certitude of the
importance of such a training to be able to have an impact on one's
student.

Sousan Abolhassani, Ph.D.
Laboratory for Materials Behaviour
Paul Scherrer Institut
5232 Villigen PSI
Switzerland

Tel.: + 41 56 310 2191
Fax.: + 41 56 310 2205
E-mail: sousan.abolhassani-at-psi.ch

"John W. Raffensperger, Jr." wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} If it makes all of you feel any better, the phenomenon of users not
} wanting to learn how to use something, just wanting the results, is not
} limited to microscopy, and is a dangerous trend. This trend is
} ironically aided by the very advancing technologies that make truly
} understanding the theories and principles of what is happening more
} important than ever.
}
} Too many devices, instruments and other systems have become "too easy to
} use". The advances in human interfaces, automation, computer controls,
} etc. have made it very easy for just about anyone to get results. The
} danger is that there is no way for someone who doesn't truly understand
} what's going on to know if the results are meaningful or not. "I got
} the answer, and it's what I was expecting, so it must be right!"
}
} The problem is also not limited to "sophisticated" technology. We have
} users who no longer know that there is a darkness adjustment on a copy
} machine, much less how to use it. Not that long ago, you couldn't get
} two copies in a row to turn out without tweaking the adjustment. If
} someone does take the thing off "auto" and sets it dark, everyone else
} thinks the thing is broken...
}
} If someone finds a "real" cure for this phenomenon, please share it with
} the world, because the problem is pretty universal.
}
} John W. Raffensperger, Jr.
} IS Manager
} Helwig Carbon Products, Inc.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 04:32:18 2004

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Our old camera has to be replaced and I am offered a new one for 1200 euros.
This may not be too expensive but I wonder if I can get the same results
with a cheaper webcam attached to the microscope. I understand it is just a
question of removing the camera objective lense or to make it focus
infinity.

My question is: can I expect a really better performance from a more
expensive, purpose-built camera? Quite likely the camera will not be the
limiting factor in the quality of micrographs, but other factors in the
microscope and the preparation...

And, which factors should I cosider in the camera? I am thinking of
sensitivity to poor light, gain, and so.

Thanks for all your comments,

Antonio D. Molina-García
Inst. del Frio (CSIC) Madrid, Spain

PD. My main purpose for video recording from a microscope is to study ice
crystal evolution during growth and recrystallization. Image is so, not too
sharp ever, as the contrast between ice crystals is small. Also the sample
thickness is larger than when using other sample types and, when the size
of
crystals is small, it is even difficult to get any light through...

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 04:54:16 2004

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Second Announcement
From Microscopy to Nanoscopy, Genoa, 9-11 February 2004.
The 5th Practical and Intensive Workshop on 3D Confocal Microscopy will
be held in Genoa, at LAMBS, Department of Physics, Via Dodecaneso 33,
16146 Genoa.
The aim of the workshop, as usual, is to introduce researchers to
Confocal Microscopy and related methods. This year we would like to
show how it is possible to move from Microscopy to Nanoscopy, according
to a Stefan Hell’s recent paper (Natur.Biotech., 21 (11), 2003, p.1347).
2004 Program includes: lessons on basic aspects of fluorescence and
confocal microscopy (February 9th, 10 a.m.- 1 p.m.), lectures on
applications of confocal microscopy and related methods (February 9th,
2 p.m.-7 p.m. with coffe break), experimental sessions on confocal and
multiphoton architectures, experimental sessions with image analysis,
processing, visualization and deconvolution software, roundtables with
speakers (February 10th-11th, 8,30 a.m. - 7 p.m., including lunch
break). Lecturers: Tony Wilson, Erik Manders, Alberto Diaspro, Mario
Faretta, Cesare Usai.
The workshop is limited to 20 students served on first-in-first-out
basis. Only Monday afternoon lectures are open.
The workshop fee is 250 Euros. Some grants will be available on the
basis of real need.
Please register or request information sending an e-mail to
diaspro-at-fisica.unige.it using "confocal 5 - genoa" as subject. Please,
specify if you want to attend the Workshop or only Monday afternoon
lectures. Logistic help can be provided upon request. Poster can be
sent upon request in pdf format.
Main sponsor of the Workshop is Nikon Italia, SpA, Firenze. News on the
workshop can be found at www.lambs.it, from January 13th 2004.
Further sponsorship can be proposed to diaspro-at-fisica.unige.it using as
subject "confocal 5 - sponsor".
All my best
Alberto Diaspro
.......................................................................
...................................
.. non basta, resistere, resistere...resistere
^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
Alberto Diaspro
Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genoa, Italy
voice: +39-0103536426/480 fax 010314218
diaspro-at-fisica.unige.it, http://www.lambs.it
http://wiley.com/cda/product/0,,0471409200,00.html

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 06:43:27 2004

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Electron Microscopist/Laboratory Manager Position
Department of Materials Science and Engineering
Drexel University, Philadelphia, PA 19010

We are seeking a candidate to supervise a microscopy laboratory,
which includes an FEI/Phillips XL30 field emission environmental
scanning electron microscope with an EDAX-EDS and TSL-OIM, an Amray
1830/D4, and a basic TEM (we outsource most TEM work), optical
microscopes, sample preparation facilities, two X-ray
diffractometers, etc. We are moving towards a centralized facilities
model for the entire university and anticipate the move of many of
our laboratories to a new research building by 2005. In addition to
instrument maintenance, user scheduling, supervising and training
users, the person in this position is expected to participate in the
planning and execution of tasks related to the centralized materials
testing and characterization facilities and the relocation of the
labs to the new building. Candidates should have demonstrated
experience with electron microscopy and preferably a degree in
Materials, Physics or Biology. Salary will be commensurate with
qualifications and experience.

The successful candidate will join a technical staff of three within
the department. Detailed information about the department can be
found at http://www.materials.drexel.edu, a copy of our recent
newsletter can be found at
http://www.materials.drexel.edu/Newsletter/fall_03.pdf and our last
annual report at
http://www.materials.drexel.edu/annualreports/Annual%20Report%202002.pdf.
Candidates interested in this position should please submit a CV and
a short career plan to: Microscopy Hiring Committee, Drexel
University, Department of Materials Science and Engineering, 3141
Chestnut Street, Philadelphia, PA 19104.

Dr. Richard Knight
--
"And the men who hold high places, must be the ones to start..."

Richard Knight, Ph.D., FASM, Auxiliary Professor,
Center for the Plasma Processing of Materials [CPPM],
Drexel University, Dept. of Materials Science & Engineering,
3141 Chestnut Streets, Philadelphia, PA 19104

"A Ben Franklin Center of Engineering Excellence"

Tel: [215] 895-1844; FAX: [215] 895-2332;
E-mail: knightr-at-drexel.edu [Slow]; knightr-at-coe.drexel.edu [More Reliable]
Web: http://www.materials.drexel.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 06:54:50 2004

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A most interesting thread, and one that is near and dear to my heart.......

I frequently get people new to SEMs, either through personnel changes at
a customer's site or through someone's acquisition of a "new" (used)
SEM. Half of my business is still servicing ETEC Autoscans and as the
new systems get more and more automated, I get more and more comments on
how user unfriendly the Autoscan is. My standard reply is that it is
not at all unfriendly if you understand how an SEM works.

I always start a new user out by building an SEM on paper and guess
what? A scanning electron microscope is not a microscope at all! The
only image formed in its optics is a DEmagnified image of the tip of the
filament! So, what is it? It's a signal generator with one or more
signal processors attached. What I really love about SEMs, especially
with an EDS attached, is that you can tell me what you want to see and I
can probably show it to you. Then we have to sit down and have a long
talk about what is real. Don't tell me, "the computer said...". The
computer doesn't know squat. And I haven't even gotten to specimen
preparation!

The problem goes beyond the need for instant gratification, but may be
related to the definition of success. People aren't interested in
becoming microscopists because organizations no longer hire
microscopists. One must pay too much for the knowledge and experience.
Most are looking for "machine operators" that can be transferred
between different pieces of equipment at will or they simply equate a
microscope with a copier or personal computer. It's merely another tool
to be used in getting the job done. We no longer have someone
designated as the "copier specialist" in the office and having a degree
in computer science is not a prerequisite for operating a computer on
your desktop.

In part, there is simply so much more to know about any piece of
equipment or area of interest, and the areas of interest and expertise
are so intertwined, that one cannot be an expert in all areas, and in
part it is the "Walmartization" of the world. The dive to the bottom,
the least common denominator, the lowest cost, the lowest price. Of
course, if everyone worked for Walmart, no one could afford to do much
shopping............

I don't have any answers. I've always liked to understand any equipment
that I use, whether it's a microscope or an automobile or a dishwasher,
but then, I repair things for a living. I make a living this way
because other people have different interests and drives (and that often
does NOT include an interest or ability to repair things). A hundred
years ago, most people who owned an automobile also had a mechanic in
their employ, and the mechanic often traveled with, or even drove, the
car.

I believe our problem in science will also get worked out. It's
probably going to take some disaster related to bad science to get
people's attention, but in the end, some kind of accommodation will be
worked out. It will be interesting to watch it unfold.

In the mean time, we can all keep trying to spread our knowledge and our
concerns. We subscribe to this listserver because we care. Keep caring!

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 07:15:40 2004

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Dear Antonio,

I would be careful with using a webcam for professional microscopy. Indeed,
you can adjust a webcam this way that it can be attached to a microscope
(remove the lens and put the ccd in the focuspoint of the lightbeam), but
most webcams are very limited. Limited in shutterspeed, colorrange and fo
sure in pixelresolution. Webcams are often used for amateur-microscopy and
astronomy and give nice results, but if you really want to start analysing
the (live) images or use them for publication, I'm afraid you might get
dissapointed. Also: more expensive, professional camera's will last longer
,give you nicer resultes and a better support after sale will be offered.
Best regards,

Sven Terclavers

On 08-01-2004 23:33, "Antonio Molina" {ifrm111-at-if.csic.es} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Our old camera has to be replaced and I am offered a new one for 1200 euros.
} This may not be too expensive but I wonder if I can get the same results
} with a cheaper webcam attached to the microscope. I understand it is just a
} question of removing the camera objective lense or to make it focus
} infinity.
}
} My question is: can I expect a really better performance from a more
} expensive, purpose-built camera? Quite likely the camera will not be the
} limiting factor in the quality of micrographs, but other factors in the
} microscope and the preparation...
}
} And, which factors should I cosider in the camera? I am thinking of
} sensitivity to poor light, gain, and so.
}
} Thanks for all your comments,
}
} Antonio D. Molina-García
} Inst. del Frio (CSIC) Madrid, Spain
}
} PD. My main purpose for video recording from a microscope is to study ice
} crystal evolution during growth and recrystallization. Image is so, not too
} sharp ever, as the contrast between ice crystals is small. Also the sample
} thickness is larger than when using other sample types and, when the size
} of
} crystals is small, it is even difficult to get any light through...
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 07:31:01 2004

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I very much agree with Sousan about what drives students and their reward systems. However, consider the fact that universities often reflect what is going on in private industry. I would bet that many researchers, scientists and engineers report to people that have scant knowledge of the science they ostensibly oversee. I call this the "MBA Phenomenon." I've observed this trend not only in microscopy. How often must someone in the lab. explain to their "management" exactly what an image is telling them? Quality should start with quality management and that means the management ought to know what they are managing.

Peter Tomic
Agere Systems

Disclaimer: I am happy to report that the above conditions do not apply to me at the moment.

-----Original Message-----
} From: Sousan Abolhassani [mailto:sousan.abolhassani-at-psi.ch]
Sent: Thursday, January 08, 2004 4:29 AM
To: John W. Raffensperger, Jr.
Cc: microscopy-at-MSA.Microscopy.com

I fully agree with this fact that the problem is universal,
and it is not only limited to microscopy. However, before one
finds the "cure for this phenomenon", one should look for the cause
of this problem.

If the new generation, i.e. the younger students and others, "are just
wanting results", is it not the consequence of the ATTITUDE OF THE
LARGE MAJORITY of those who trained them?

Those who trained the last two generations are now collecting the
results of what they have done.
The biggest reference for this generation is having rapid success,
which means gaining large amounts of money and if possible a quick fame.

No university professor considers the students for their interest for
science and their will to do something for the sake of humanity.
They rank them on their good marks, without worrying about how they
obtained it. And even if they do so, it is to REPRIMAND the student and
not for TEACHING them the importance of honesty.
A large percentage of students learn just to obtain a good mark, without
thinking about why's and how's. And those few who do, are not
appreciated
by the professors, may be since they need more time that is not
available.

A professorship is the art of teaching many things including highest
human values to the students, I can not name many who have done that, or
even
have thought to do it. If they do not reflect such thoughts, at least
they
should avoid to discourage the very few who do have such values (and
have truly come to learn something that can be helpful for the society)
by treating them as naives and dealing with irony with them.

Some students tell me that the science professors are so arrogant that
the students have no more appeal for scientific branches.
} From my discussions with some undergraduate science students, their
feeling is
that if they go for science in their graduate school they could ruin
their future and they will loose the chances of success!

I agree that the danger is real and from my understanding the solution
to the problem is to reverse the trend from now on by changing the
teaching philosophy. However, one should have the certitude of the
importance of such a training to be able to have an impact on one's
student.

Sousan Abolhassani, Ph.D.
Laboratory for Materials Behaviour
Paul Scherrer Institut
5232 Villigen PSI
Switzerland

Tel.: + 41 56 310 2191
Fax.: + 41 56 310 2205
E-mail: sousan.abolhassani-at-psi.ch

"John W. Raffensperger, Jr." wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} If it makes all of you feel any better, the phenomenon of users not
} wanting to learn how to use something, just wanting the results, is not
} limited to microscopy, and is a dangerous trend. This trend is
} ironically aided by the very advancing technologies that make truly
} understanding the theories and principles of what is happening more
} important than ever.
}
} Too many devices, instruments and other systems have become "too easy to
} use". The advances in human interfaces, automation, computer controls,
} etc. have made it very easy for just about anyone to get results. The
} danger is that there is no way for someone who doesn't truly understand
} what's going on to know if the results are meaningful or not. "I got
} the answer, and it's what I was expecting, so it must be right!"
}
} The problem is also not limited to "sophisticated" technology. We have
} users who no longer know that there is a darkness adjustment on a copy
} machine, much less how to use it. Not that long ago, you couldn't get
} two copies in a row to turn out without tweaking the adjustment. If
} someone does take the thing off "auto" and sets it dark, everyone else
} thinks the thing is broken...
}
} If someone finds a "real" cure for this phenomenon, please share it with
} the world, because the problem is pretty universal.
}
} John W. Raffensperger, Jr.
} IS Manager
} Helwig Carbon Products, Inc.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 08:13:05 2004

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----- Original Message -----
} From: jamielange-at-wi.rr.com (by way of
MicroscopyListServer)

The power of semantics

I am convinced that one of the reasons for a decline in the quality of
microscopy, especially in industry, is semantic. Over the last few
years it has become fashionable for managers to refer to instruments as
"tools". They no longer distinguish between different kinds of
equipment - they are all tools. Tools include: lathes, electron
microscopes, fork lift trucks, x-ray diffraction units,.....

When a person using a tool leaves or is promoted, you need another
person to operate the tool. So you take a person from this tool and put
them on to that tool. Give them a couple of hours to read the manual
and away you go.

I can only assume that machinists are complaining about the decline in
the quality of work done in machine shops. All the ex-SEM operators
must be doing a lousy job of operating the milling machines.

--
..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 08:39:34 2004

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In a message dated 1/8/04 9:28:40 AM, jae5-at-lehigh.edu writes:

} I can only assume that machinists are complaining about the decline in
}
} the quality of work done in machine shops. All the ex-SEM operators
} must be doing a lousy job of operating the milling machines.

Alwyn, I don't think the analogy holds. Machine tools have gotten "smarter"
in recent years. Numerical control and feedback devices have made it possible
for information to flow directly from the design computers and CAD programs
(which in turn have replaced the traditional draftsman) to control the machining
process. In some cases the "operators" aren't even present, or just keep watch
over a large array of machines in case of malfunctions or to load raw
material. As the microscopes have evolved, they have for the most part not become
easier to operate. Oh sure, some "little" things like adjusting astigmatism,
saturating filaments, even focusing, have been automated. But not the "big" things
like taking a meaningful picture. In fact, it has arguably become more
complicated to use the modern microscopes because they offer a much broader range of
possibilities than the old ones did. More imaging modes, more types of
detectors, etc., create a greater demand for insight and knowledge on the part of
the operator.

John Russ
(visit www.DrJohnRuss.com for a schedule of upcoming image analysis workshops
and other information)

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 08:50:32 2004

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8 January 2004

Mike Delannoy asked whether there is an easier way to make holey carbon
films than Formvar, steam, create the holes in the damaged Formvar film,
carbon coat the holey Formvar and dissolve the Formvar away to leave the
holey carbon film. If there is, we'd like to know about it! This is the
easiest method about which we know.

I must stress, however, that making holey and lacey carbon coated grids is
pure art. People who have decades of experience making support films still
have difficulty at times with the reproducibility of the method, and the
details are entirely a matter of getting the "feel" of the method. Details
of our methods are described on

http://www.2spi.com/catalog/grids/cusctgrd.html

and the pages linked to it.

An easier way to obtain holey carbon support films with a known and precise
distribution of holes is the Quantifoil Micromachined Holey Carbon Grids,
described on

http://www.2spi.com/catalog/grids/quantifoil-carbon-films.html

Disclaimer: SPI Supplies has a very active business making coated grids for
customers throughout the world. We also sell grids and other supplies for
customers who prefer to coat their own grids, and we sell the Quantifoil
Holey Carbon Grids.

Andy

Andrew W. Blackwood, Ph.D.
Vice President, Technical
SPI Supplies
P.O. Box 656
West Chester, PA 19381-0656
Ph: 1 610 436 5400 X108
FAX: 1 610 436 5755
e-mail: ablackwood-at-2spi.com
WWW: http://www.2spi.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 09:25:16 2004

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John,

While I see your point, it is much easier to at produce something with
today's "tools", even your "tools". We can now use PhotoShop or some other
application, load up some Image Tool filters and away you go with image
analysis. My first IA package was very cumbersone and it took some major
training just to load the images and navigate through the software.
Presumably, you would pick some understanding of the subject matter through
osmosis, solid state diffusion or entropy while learning how to operate the
software. Now the software is so easy, anyone can sit down and after a few
minutes start cranking out numbers.... for as meaningful or meaningless as
they may be.

With SEMs, my first one filled a room and producing a photo was a real
chore. You had to have an intimate knowledge of the controls and operating
conditions to get even a poor quality photo. Now you can train a chipmunk
(borrowed from one of my associates) to run an SEM. We have seen PhD's
operate the SEM as a machine and have absolutely zero fundamental knowledge
of the images or EDS data. I am thankful that I can sit down at my SEM and
get a great photo in 5 minutes, but that means anyone else can too.

Al Stone
ASTON

ps. no offense to anyone with a PhD, the point is that just because you can
drive a car doesn't mean you understand the rules of the road or know how
to travel cross country

At 08:42 AM 1/8/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 09:25:52 2004

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My favorite quote fits well in this discussion:
"It is not enough to believe what you see. You must also understand
what you see.
- Leonardo da Vinci"

I think it has to do a bit with what John just brought up in regards to
the evolution of the microscopes. They have become "easier" to operate,
and in doing so (computer control, mouse operated saturation...) there
is a great disconnect with how the 'system' works. Users learning on an
old EM300 for example have more interactions with the parameters on the
microscope and thus are in a better position to 'understand' what they
are doing in the process of collecting an image.

It is difficult to stress integrity, understanding when teaching. Even
harder is the problem educators have in providing evaluation of the
process, esp when there is a definitive end product (a lab report with
images for example). I would much prefer to be able to grade students
on their process than on the end results, and to provide an objective
progress evaluation that translates onto a final grade. The biggest
problem is that each student is different, has different learning
speeds, different ways of coming to the same end point. So many
variables to deal with. I find that the most effective and simple
question I can present to students and faculty using the facility is
"How do you know [ That ] is what you are looking at?" And sometimes it
becomes a significant frustration level when the individual cannot
convince me. But when they CAN convince me they wind up becoming much
more confident and it forces them to find supporting evidence that they
were too lazy or busy to look for earlier, and then they (more often
than not) are much better at looking (literature sourcing) BEFORE
starting their next project.

Well it is a new year and for some of us a new Semester. Time to start
doing what ever we can do to reverse the trend!

Geoff Williams
Microscopy Facility Supervisor

Central Michigan University Biology Department Microscopy Facility
http://www.cst.cmich.edu/centers/microscopy/

} -----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
} Sent: Thursday, January 08, 2004 9:42 AM
} To: jae5-at-lehigh.edu; microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Re: Re: Knowledge and Quality
}
}
}
}
------------------------------------------------------------------------
--
} ----
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
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} -----
}
}
} In a message dated 1/8/04 9:28:40 AM, jae5-at-lehigh.edu writes:
}
} } I can only assume that machinists are complaining about the decline
in
} }
} } the quality of work done in machine shops. All the ex-SEM operators
} } must be doing a lousy job of operating the milling machines.
}
} Alwyn, I don't think the analogy holds. Machine tools have gotten
} "smarter"
} in recent years. Numerical control and feedback devices have made it
} possible
} for information to flow directly from the design computers and CAD
} programs
} (which in turn have replaced the traditional draftsman) to control the
} machining
} process. In some cases the "operators" aren't even present, or just
keep
} watch
} over a large array of machines in case of malfunctions or to load raw
} material. As the microscopes have evolved, they have for the most part
not
} become
} easier to operate. Oh sure, some "little" things like adjusting
} astigmatism,
} saturating filaments, even focusing, have been automated. But not the
} "big" things
} like taking a meaningful picture. In fact, it has arguably become more
} complicated to use the modern microscopes because they offer a much
} broader range of
} possibilities than the old ones did. More imaging modes, more types of
} detectors, etc., create a greater demand for insight and knowledge on
the
} part of
} the operator.
}
} John Russ
} (visit www.DrJohnRuss.com for a schedule of upcoming image analysis
} workshops
} and other information)

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 09:28:16 2004

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-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Thursday, January 08, 2004 8:42 AM

In a message dated 1/8/04 9:28:40 AM, jae5-at-lehigh.edu writes:

} I can only assume that machinists are complaining about the decline in
}
} the quality of work done in machine shops. All the ex-SEM operators
} must be doing a lousy job of operating the milling machines.

Alwyn, I don't think the analogy holds. Machine tools have gotten
"smarter"
in recent years.

-Reply:

I agree with Alwyn. This is the exact phenomenon I was referring to,
and Machine Tools are one of the specific examples I had in mind with my
original comments to this thread.

As you stated, there are shops where those involved truly understand
what's going on, and things work very well.

In other shops, while these "tools" have indeed become "smarter", the
quality of the output has decreased. This is because, as another post
stated, these newer machines are viewed as a "tool", and an "operator"
is assigned. Because of the intelligence of the machine, the "operator"
who is no longer a "machinist" can get a result. It is often not an
optimal result, either in terms of quality, and/or in terms of
production rate. But a result was obtained. Compounding this,
management has seen this situation "evolve" gradually, so they don't
realize how much the "lower priced" help is actually costing them vs. a
"real" machinist.

Add CAM instructions coming from an engineer who has never even operated
a machine, and things get even more fun. Ask me about the $100,000+
damage one of these "wonder kids" did when they crashed a brand new
machining center. The simulation ran perfectly. Too bad the engineer
forgot that something had to hold the work piece, and this something was
2" think...

John W. Raffensperger, Jr.
IS Manager
Helwig Carbon Products, Inc.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 09:36:59 2004

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We have a Zeiss 109 TEM available. Scope includes the unique SEM attachment (gives SEM capability with two SEM stages that fit standard Zeiss pin mounts). Turbo pumped; extra gun assembly, filaments, water chiller, manuals, and original orange paint on column included. Has been under full Zeiss/Leo service contract and in use until last month.

Needs to be removed as soon as possible to make room for a new scope.

Preference given to academic institutions. If you want it, you need to make arrangements for shipping, or pick it up in New London, CT. Contact me offline for further information.

Page Owen

************************
T. Page Owen, Jr., Chair
Department of Botany
Connecticut College
New London, CT 06320
860-439-2147
tpowe-at-conncoll.edu
************************

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 09:46:30 2004

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Hi Jamie:

Without a picture of what you are seeing advice is difficult. My
guess is that the section is not flat on the slide and water/stain is
getting underneath a wrinkle in the section and the result is the
"ribbon" you are seeing. Suggestions to solve the problem:

1. A sharp knife. If you are using glass knives use only knives made
"fresh". Glass, being a super-cooled liquid, flows and older knives are
less sharp. Try it!
2. De-wrinkle the sections with 1,2 dicholorethane or chloroform.
3. Float the sections on a larger drop of water on a hot plate. The
larger drop will take longer to evaporate and give the section more time
to be expanded/dewrinkled by heat.
4 Thinner sections? I don't know how thick your sections are but 1-2
microns is the range to shot for.

Geoff

by way of MicroscopyListServer wrote:

} Email: jamielange-at-wi.rr.com
} Name: jamie lange
}
} Organization: university of wisconsin
}
} Education: Graduate College
}
} Location: milwaukee, wi. usa
}
} Question: we used a spurr's resin prep on a sample of nematodes, after
} staining and heat-fixing the sections, we see dark ribbon-like
} structures on several specimens. Are these artifacts caused by air
} bubbles and can they be avoided? thank you,
} jamie
}
} ---------------------------------------------------------------------------
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 09:52:27 2004

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Hi

This certainly is a f.a.q.!

First of all EVERYONE must realise that the image that they see (even though
they pressed the SE or SEI button) is a mixed SE+BSE image. This means
surface detail from the SE and sub surface detail from the BSE. As you put
the kV up the BSE dominates more and of course as you take the kV down the
BSE are reduced allowing the SE to dominate. I should point out that you
will often see BSE information even at 2kV or less; this being the result of
the SE3 contribution.

Place a thin coating on the surface of a specimen and you increase the
coefficient of emission, the metal being the SE emitter rather than the
original biological material. You do image the specimen surface as that
topography has been followed by the coating procedure. However the BSE come
from a far greater depth below the surface and at any kV, under the wrong
circumstances of WD and spot size, these electrons will contribute to the
image. Should there be structure of differing density, by way of the BSE,
this will show as "shadows" in the background or may even dominate the
image.

In a field emission instrument, of the type where the above lens detector is
available, it is possible to screen out the BSE contribution and display a
pretty pure SE image. I have to say in my 40 years in the business we have
more often gone for "information" rather than "resolution" therefore I do
try to include a degree of BSE to add contrast to the image.

Hope this helps?

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob 07711 606967
www.emcourses.com

----- Original Message -----
} From: "Tobias Baskin" {baskin-at-bio.umass.edu}
To: "Steve Chapman" {protrain-at-emcourses.com} ;
{microscopy-at-MSA.microscopy.com}
Sent: Wednesday, January 07, 2004 4:51 PM

It appears we have a change in how quality is monitored over the years of
SEM evolution. As may be the case where older SEMs require understanding of
how a SEM works to get an image, to the extent that newer SEMs do not
require this, those operating newer SEMs may not require the prior extent of
knowledge to produce images. Where once the decision to take images were
made by those who knew enough to understand and self monitor quality, that
appears not to be the case anymore. Advances in technology have allowed
images to be taken by operators who do not understand what they are looking
at; one can not expect an unknowing individual to monitor quality.

We can address the quality issue with education or attitude (as proposed by
others on this board). This is a head on approach; a less direct method
would be to change the decision rights or incentives. For example, operators
should not be given the decision right of what to take an image of. For
example, operators should not be rewarded simply on the number of images
taken.

The point is that monitoring of quality has changed, so we should consider
changing decision rights and incentives/rewards. If these three components
of organizational architecture are not in balance, results will be
unsatisfactory.

Sincerely,
John Moore
Montara Industries
919-434-8457

Disclaimers:
1) This framework is described in a book titled "Managerial Economics and
Organizational Architecture", a text that I studied while obtaining my MBA
at the University of Rochester, Class of 2000.

2) In defense of my education and this technique, I cite first that the
poster from Agere on this topic reported not suffering certain difficulties,
and second that in my recent job search I found Agere to be hiring MBA's
(see monster.com directemployers.com, hotjobs.com or flipdog.com).

3) I am not a SEM expert, nor do I have direct experience in this field. I
began following this message board in the interest of selling a defect
review tool that I made a speculative investment in: a SEMVision by Applied
Materials.

----- Original Message -----
} From: "Sousan Abolhassani" {sousan.abolhassani-at-psi.ch}
To: "John W. Raffensperger, Jr." {johnr-at-helwigcp.com}
Cc: {microscopy-at-MSA.Microscopy.com}
Sent: Thursday, January 08, 2004 4:28 AM

I fully agree with this fact that the problem is universal,
and it is not only limited to microscopy. However, before one
finds the "cure for this phenomenon", one should look for the cause
of this problem.

If the new generation, i.e. the younger students and others, "are just
wanting results", is it not the consequence of the ATTITUDE OF THE
LARGE MAJORITY of those who trained them?

Those who trained the last two generations are now collecting the
results of what they have done.
The biggest reference for this generation is having rapid success,
which means gaining large amounts of money and if possible a quick fame.

No university professor considers the students for their interest for
science and their will to do something for the sake of humanity.
They rank them on their good marks, without worrying about how they
obtained it. And even if they do so, it is to REPRIMAND the student and
not for TEACHING them the importance of honesty.
A large percentage of students learn just to obtain a good mark, without
thinking about why's and how's. And those few who do, are not
appreciated
by the professors, may be since they need more time that is not
available.

A professorship is the art of teaching many things including highest
human values to the students, I can not name many who have done that, or
even
have thought to do it. If they do not reflect such thoughts, at least
they
should avoid to discourage the very few who do have such values (and
have truly come to learn something that can be helpful for the society)
by treating them as naives and dealing with irony with them.

Some students tell me that the science professors are so arrogant that
the students have no more appeal for scientific branches.
} From my discussions with some undergraduate science students, their
feeling is
that if they go for science in their graduate school they could ruin
their future and they will loose the chances of success!

I agree that the danger is real and from my understanding the solution
to the problem is to reverse the trend from now on by changing the
teaching philosophy. However, one should have the certitude of the
importance of such a training to be able to have an impact on one's
student.

Sousan Abolhassani, Ph.D.
Laboratory for Materials Behaviour
Paul Scherrer Institut
5232 Villigen PSI
Switzerland

Tel.: + 41 56 310 2191
Fax.: + 41 56 310 2205
E-mail: sousan.abolhassani-at-psi.ch

"John W. Raffensperger, Jr." wrote:
}
} --------------------------------------------------------------------------
----
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} --------------------------------------------------------------------------
-----
}
} If it makes all of you feel any better, the phenomenon of users not
} wanting to learn how to use something, just wanting the results, is not
} limited to microscopy, and is a dangerous trend. This trend is
} ironically aided by the very advancing technologies that make truly
} understanding the theories and principles of what is happening more
} important than ever.
}
} Too many devices, instruments and other systems have become "too easy to
} use". The advances in human interfaces, automation, computer controls,
} etc. have made it very easy for just about anyone to get results. The
} danger is that there is no way for someone who doesn't truly understand
} what's going on to know if the results are meaningful or not. "I got
} the answer, and it's what I was expecting, so it must be right!"
}
} The problem is also not limited to "sophisticated" technology. We have
} users who no longer know that there is a darkness adjustment on a copy
} machine, much less how to use it. Not that long ago, you couldn't get
} two copies in a row to turn out without tweaking the adjustment. If
} someone does take the thing off "auto" and sets it dark, everyone else
} thinks the thing is broken...
}
} If someone finds a "real" cure for this phenomenon, please share it with
} the world, because the problem is pretty universal.
}
} John W. Raffensperger, Jr.
} IS Manager
} Helwig Carbon Products, Inc.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 10:39:09 2004

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To Joel, Eckhart, Kenneth, Peter, and anyone else who gave me advice-

OK, I finally had a chance to sit down and fiddle with the chiller, and
here is what I have.

I turned on my Zeiss EM 10CA and checked the flowmeter in the column:
about 2.2 L/min, if I am reading it right. There was no gauge for the
chiller flow rate, but there is a pressure gauge on the front of the
chiller, and it read about 39 psi. This reading did not change through
the entire test, and neither did the EM flowmeter.

Chiller temperature reading was about 75 degrees F at start. It needs
to be 68 degrees F, according to the EM's manual. Only the "Cool" light
was on...all others, including the "Compressor" light, were off.

I turned the temperature screw to the left to lower the temp setting.
No response from the compressor. Turned it down a second time....still
no response. After about 5 minutes the Compressor light turned on, and
the temperature started to drop, finally. The temperature went all the
way down to 53 degrees F, at which point the "Lo Temp" light went on,
the "Compressor" light went off, and the "Heat" light went on. I turned
up the temp screw a little bit.

At about 60 degrees F, the "Heat" and "Lo Temp" lights went off and the
"Cool" and "Pump" lights are on (actually the "Pump" light never turned
off). It rose to 68 degrees F....and continued to rise. I let it get
to about 79 degrees F, and the compressor never turned back on. I tried
turning the screw back to the left to drop the temp setting...it never
went back on.

At this point, I decided to turn the EM 'scope off....though the flow
rate never dropped, and the buzzer never went off. The temperature
gauge on the chiller continued to rise, even after turning the 'scope
off. It was reading about 90 degrees F when I left to come write all of
you.

Just now went back in to check the thing...the compressor finally came
on...it's reading about 53 degrees F and the "Lo Temp" light is on, and
the "Compressor" light is off.

So I think it's the switch....or perhaps the "Hi Temp" sensor? Or
both? I have no idea how all the sensors and switches are
connected...even with the diagrams and manual that were sent, as I have
no idea how to read such things (been eons since I did circuits in
Physics class...). What do you all think?

Thank you all so much for your help-
Kathleen
Neurotoxicology Labs
Rutgers University

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 12:23:55 2004

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I've been reading the iterations on this thread and it seems to me that it
would be useful to separate the chiller from the TEM to test the
chiller. Kathleen, if you have a carbon evaporator that has a diffusion
pump you can cool it with the Coolwell long enough to tell if the Coolwell
has a problem. If the Coolwell tests okay on another heat load (the carbon
evaporator) then your problem is in the TEM.

Owen

Owen P. Mills
Electron Optics Engineer
Materials Science & Engineering
Michigan Technological University
Rm 512 M&M Bldg.
Houghton, MI 49931
PH 906-369-1875
FAX 906-487-2934
mailto:opmills-at-mtu.edu
http://www.mm.mtu.edu/~opmills

At 11:48 AM 1/8/2004 -0500, Kathleen Roberts wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Owen P. Mills
Electron Optics Engineer
Materials Science & Engineering
Michigan Technological University
Rm 512 M&M Bldg.
Houghton, MI 49931
PH 906-369-1875
FAX 906-487-2934
mailto:opmills-at-mtu.edu
http://www.mm.mtu.edu/~opmills

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 13:00:36 2004

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Hi Listers

Well some interesting stuff, I was particularly taken by Peter Tomic's
comments

"Quality should start with quality management and that means the management
ought to know what they are managing."

Via MSA and mostly privately I have had mail from, judging by the mailers
enthusiasm, pretty good EM units. However I have probably visited more EM
units in the world than most of you and I have to say in very many cases
they are just not up to the standards that I would set. Here Peter's
comment hits home to me! You see, as an example, in most units people were
trained when the SEM, TEM or EDS system first arrived in the lab. Now they
have new equipment and I bet they have rarely been trained to operate using
the techniques opened up by the new SEM or TEM? Once trained you know how
to use them is what I see. Guess what, a customer born on a Cambridge 100
SEM still used their new sexy Field Emission SEM in just the same way. A
thick gold coating and 20kV plus was the way to do it, quote "we have
always done it this way". We produced amazing results uncoated at 150,000X
at 1.5kV! Do I make my point? This was a very highly rated government
research laboratory that by perception would be rated as in the top 5 in a
country very well respected for its EM work!

We all believe we run a good unit, my point would be "how do you know?" Do
you have management procedures that are up to date, do you routinely check
the performance of your staff, do you look at the output your users produce,
etc etc? Take a look at www.iaaem.com/mppa1 here you will find a quality
procedure that has been proposed by a group of scientists and Quality
experts from across the world. Answer the questions and total up the points
for your laboratory and lets see how far you area away from Total Quality
Management. What would you suggest is included and maybe together we will
be able to develop procedures that would help sort out what you all, almost,
seem to agree is a bit of a mess!

I am working overseas (Egypt) for the next week so have fun on your own for
a little while.

Regards

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob 07711 606967
www.emcourses.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 13:44:05 2004

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Hello Listers,

I want to give away the following to a university or non-profit lab or
group:

Plexiglass racks for holding 3.25" x 4" (TEM) and 4" x 5" (Polaroid)
negative film; and
hard rubber tanks for processing negatives.

Interested parties should contact me off-line. Commercial/industrial users
need not respond.

Thanks,

"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 14:04:04 2004

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Owen-

Good idea, except that I don't have a carbon evaporator. :o)

Thanks anyway,
Kathleen
Neurotox Labs
Rutgers University

Owen P. Mills wrote:

} I've been reading the iterations on this thread and it seems to me
} that it would be useful to separate the chiller from the TEM to test
} the chiller. Kathleen, if you have a carbon evaporator that has a
} diffusion pump you can cool it with the Coolwell long enough to tell
} if the Coolwell has a problem. If the Coolwell tests okay on another
} heat load (the carbon evaporator) then your problem is in the TEM.
}
} Owen
}
} Owen P. Mills
} Electron Optics Engineer
} Materials Science & Engineering
} Michigan Technological University
} Rm 512 M&M Bldg.
} Houghton, MI 49931
} PH 906-369-1875
} FAX 906-487-2934
} mailto:opmills-at-mtu.edu
} http://www.mm.mtu.edu/~opmills
}
} At 11:48 AM 1/8/2004 -0500, Kathleen Roberts wrote:
}
}
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } To Joel, Eckhart, Kenneth, Peter, and anyone else who gave me advice-
} }
} } OK, I finally had a chance to sit down and fiddle with the chiller,
} } and here is what I have.
} }
} } I turned on my Zeiss EM 10CA and checked the flowmeter in the column:
} } about 2.2 L/min, if I am reading it right. There was no gauge for
} } the chiller flow rate, but there is a pressure gauge on the front of
} } the chiller, and it read about 39 psi. This reading did not change
} } through the entire test, and neither did the EM flowmeter.
} } Chiller temperature reading was about 75 degrees F at start. It
} } needs to be 68 degrees F, according to the EM's manual. Only the
} } "Cool" light was on...all others, including the "Compressor" light,
} } were off.
} }
} } I turned the temperature screw to the left to lower the temp setting.
} } No response from the compressor. Turned it down a second
} } time....still no response. After about 5 minutes the Compressor
} } light turned on, and the temperature started to drop, finally. The
} } temperature went all the way down to 53 degrees F, at which point the
} } "Lo Temp" light went on, the "Compressor" light went off, and the
} } "Heat" light went on. I turned up the temp screw a little bit.
} }
} } At about 60 degrees F, the "Heat" and "Lo Temp" lights went off and
} } the "Cool" and "Pump" lights are on (actually the "Pump" light never
} } turned off). It rose to 68 degrees F....and continued to rise. I
} } let it get to about 79 degrees F, and the compressor never turned
} } back on. I tried turning the screw back to the left to drop the temp
} } setting...it never went back on.
} }
} } At this point, I decided to turn the EM 'scope off....though the flow
} } rate never dropped, and the buzzer never went off. The temperature
} } gauge on the chiller continued to rise, even after turning the 'scope
} } off. It was reading about 90 degrees F when I left to come write all
} } of you.
} }
} } Just now went back in to check the thing...the compressor finally
} } came on...it's reading about 53 degrees F and the "Lo Temp" light is
} } on, and the "Compressor" light is off.
} } So I think it's the switch....or perhaps the "Hi Temp" sensor? Or
} } both? I have no idea how all the sensors and switches are
} } connected...even with the diagrams and manual that were sent, as I
} } have no idea how to read such things (been eons since I did circuits
} } in Physics class...). What do you all think?
} }
} } Thank you all so much for your help-
} } Kathleen
} } Neurotoxicology Labs
} } Rutgers University
} }
} }
}
} Owen P. Mills
} Electron Optics Engineer
} Materials Science & Engineering
} Michigan Technological University
} Rm 512 M&M Bldg.
} Houghton, MI 49931
} PH 906-369-1875
} FAX 906-487-2934
} mailto:opmills-at-mtu.edu
} http://www.mm.mtu.edu/~opmills
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 14:12:46 2004

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In my experience, CCTV cameras as used in security applications work better than
webcams, but the resolution of both is not that great and you may spend considerable
time on the mechanical aspects of the interfacing and be disappointed with the result.

1200 euros may be well worth it for something that you can just unpack from the box
and be using in a few minutes.

cheers

rtch

Send reply to: "Antonio Molina" {ifrm111-at-if.csic.es}
} From: "Antonio Molina" {ifrm111-at-if.csic.es}
To: {Microscopy-at-MSA.Microscopy.Com}

Most people store UA in the refrigerator perhaps without
understanding why. UA is photosensitive and degraded by light
(especially fluorescent lighting that contains UV). If you store
aqueous solutions in the light they will eventually precipitate
--first long the sides of the container and then on the bottom. I
have no data, just based on observation.

} We are having one of those debates that we microscopists seem to
} obsess about. The question is whether to store our saturated uranyl
} acetate solution (in dH2O) at room temp or at 4 C. Opinions,
} especially those backed by data, would be welcome. Happy New Year.
} Tom
}
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 14:31:49 2004

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Steve;

Thank you for the honorable mention. If my boss is on this listserver I'll have to polish up the old resume. It's so much fun to be quoted. I feel like Hemingway.

Once again, I don't have ANY of these issues HERE.

I needed a good laugh today.

Peter Tomic
Unknown Corporation, Inc.
Anytown, USA

-----Original Message-----
} From: Steve Chapman [mailto:protrain-at-emcourses.com]
Sent: Thursday, January 08, 2004 1:59 PM
To: MSA

Hi Listers

Well some interesting stuff, I was particularly taken by Peter Tomic's
comments

"Quality should start with quality management and that means the management
ought to know what they are managing."

Via MSA and mostly privately I have had mail from, judging by the mailers
enthusiasm, pretty good EM units. However I have probably visited more EM
units in the world than most of you and I have to say in very many cases
they are just not up to the standards that I would set. Here Peter's
comment hits home to me! You see, as an example, in most units people were
trained when the SEM, TEM or EDS system first arrived in the lab. Now they
have new equipment and I bet they have rarely been trained to operate using
the techniques opened up by the new SEM or TEM? Once trained you know how
to use them is what I see. Guess what, a customer born on a Cambridge 100
SEM still used their new sexy Field Emission SEM in just the same way. A
thick gold coating and 20kV plus was the way to do it, quote "we have
always done it this way". We produced amazing results uncoated at 150,000X
at 1.5kV! Do I make my point? This was a very highly rated government
research laboratory that by perception would be rated as in the top 5 in a
country very well respected for its EM work!

We all believe we run a good unit, my point would be "how do you know?" Do
you have management procedures that are up to date, do you routinely check
the performance of your staff, do you look at the output your users produce,
etc etc? Take a look at www.iaaem.com/mppa1 here you will find a quality
procedure that has been proposed by a group of scientists and Quality
experts from across the world. Answer the questions and total up the points
for your laboratory and lets see how far you area away from Total Quality
Management. What would you suggest is included and maybe together we will
be able to develop procedures that would help sort out what you all, almost,
seem to agree is a bit of a mess!

I am working overseas (Egypt) for the next week so have fun on your own for
a little while.

Regards

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob 07711 606967
www.emcourses.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 14:48:50 2004

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Yes, alas, we have also seen the "take the picture and run" mentality
here as well.

Like most microscopists who came up through the system, most of us
eagerly learned everything related to microscopy (specimen prep,
knife making, ultramicrotomy, alignment, optimization of the scope,
darkroom, image interpretation, etc). It was fun and we enjoyed
learning and making discoveries. Now, it seems the thrill is gone and
the object is to get into the job market and make big bucks....

MONEY is the motivator and it can be used to influence people. For
example, I point out that microscopy is a marketable skill and I
prove it by giving the names of our former students (in biological
and physical sciences) who got jobs in their discipline since they
could do microscopy. An employer will generally hire the individual
with the better set of skills. Unless they are incredibly naive or
just plain stupid (in which case you wouldn't want them using your
equipment anyway) they will realize the value in learning the
discipline.

More immediately, I point out that it is CHEAPER for them to do their
own microscopy than to hire it out.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 15:10:24 2004

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Hello:

I was wondering if someone knows where I can find an
monochromator for spectral scanning 400-700 nm
that can be attached to a Zeiss microscope (Axioskop) for
transmitted light imaging ( scanning microphotometry).

Any help will be greatly appreciated.

Thanks,
Fatima

{} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {}

Fatima Merchant, Ph.D.
Lead Research Engineer
Advanced Digital Imaging Research, LLC (Formerly PSI, Inc.)

2450 South Shore Blvd., Suite 305
League City, Texas 77573

Telephone: (281) 535-1889 Ext. 425

Facsimile: (281) 538-7596
Email: merchant-at-adires.com

{} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {} {}

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 15:14:05 2004

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On Jan 8, 2004, at 6:42 AM, DrJohnRuss-at-aol.com wrote:

} Alwyn, I don't think the analogy holds. Machine tools have gotten
} "smarter"
} in recent years. Numerical control and feedback devices have made it
} possible
} for information to flow directly from the design computers and CAD
} programs
} (which in turn have replaced the traditional draftsman) to control the
} machining
} process. In some cases the "operators" aren't even present, or just
} keep watch
} over a large array of machines in case of malfunctions or to load raw
} material.
Dear John,
So now the machine tools are capable of performing as well as the
automated tomography packages we use? In our case, we have to watch
the progress of the program carefully to see that the auto-tracking,
auto-focussing, etc. is working properly, and lately we have also found
that the file made from the tilt series has values that do not match
the exposure we set (to the extent that some of the images were blank).
The take-home lesson is that there still must be knowledgeable
oversight, especially with regard to automated processes, to assure the
quality of the results.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 15:14:33 2004

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A lab user has asked me to find some place he can get freeze fracture work
done. Close to San Francisco bay area would be best. Reply to me and I will
pass on the contact info.

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 15:34:44 2004

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Dear Kathleen,
I have had good luck getting a local HVAC (Heating, Ventilation and Air
conditioning) or Air Conditioning repair shop to fix my Haskris water chillers.
Haskris are good but they do occasionally break down. Sounds like one of your
sensors or accuators is stuck.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Kathleen Roberts" {kgrobert-at-rci.rutgers.edu}
To: {Microscopy-at-sparc5.microscopy.com}
Sent: Thursday, January 08, 2004 8:48 AM

Thank you for the advice...I figure $10 isn't too much to spend to try
and fix this thing....if the repair cost starts to escalate, we'll junk
it and call Haskris. :o)

Kathleen
Neurotoxicology Labs
Rutgers University

Webster, Paul wrote:

} Hi Kathleen,
}
} A word of warning if you plan to try to fix the chiller. We spent nearly $7,000 in a year of repairing our Coolwell chiller before it finally failed for good and we had to buy a new machine. When the second one started giving problems, we used the repair money to buy a new one immediately.
}
} The first one started by developing a leak in the compressor, then the pump failed and finally the thermostat switch. Getting a similar thermostat switch to the one that failed was impossible. We searched through Grainger, talked with refrigeration engineers and could only come up with a close approximation of what we needed.
}
} We had to suffer as the less sensitive thermostat switch attempted to hold the water temperature steady but with much less control. In the end it was when some other part of the machine failed that we decided to replace it. Looking back, the time and expense needed to repair the machine was not worth it.
}
} If you do find your chiller has only a small problem then try fixing it and hope the costs don't escalate.
}
} Regards,
}
} Paul Webster.
}
}
}
}
} Paul Webster, Ph.D.
} House Ear Institute
} 2100 West Third Street
} Los Angeles
} CA 90057
} phone (213) 273 8026
} fax (213) 413 6739
} email: pwebster-at-hei.org
}
}
}
}
} } ----------
} } From: Kathleen Roberts
} } Sent: Thursday, January 8, 2004 12:13 PM
} } To: Owen P. Mills
} } Cc: Microscopy-at-sparc5.microscopy.com
} } Subject: [Microscopy] Re: Coolwell chiller testing
} }
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 8 16:00:34 2004

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Owen-

Nope, no SEM and no BIG waterbath. I'm going to call Facilities here at
RU-they may be able to devise something to test it.

Thanks-
Kathleen
Neurotoxicology Labs
Rutgers University

Owen P. Mills wrote:

} Kathleen,
}
} Any heat source that can be water cooled will work, anything with a a
} diffusion pump. SEM? Got a BIG hot water bath? Coil copper tubing
} in the bath, turn the bath heat way up, connect the chiller lines to
} the ends of the coil of copper tubing. Should be a low tech test of
} the chiller.
}
} Owen
}
} At 03:13 PM 1/8/2004 -0500, you wrote:
}
} } Owen-
} }
} } Good idea, except that I don't have a carbon evaporator. :o)
} } Thanks anyway,
} } Kathleen
} } Neurotox Labs
} } Rutgers University
} }
} } Owen P. Mills wrote:
} }
} } } I've been reading the iterations on this thread and it seems to me
} } } that it would be useful to separate the chiller from the TEM to test
} } } the chiller. Kathleen, if you have a carbon evaporator that has a
} } } diffusion pump you can cool it with the Coolwell long enough to tell
} } } if the Coolwell has a problem. If the Coolwell tests okay on
} } } another heat load (the carbon evaporator) then your problem is in
} } } the TEM.
} } }
} } } Owen
} } }
} } } Owen P. Mills
} } } Electron Optics Engineer
} } } Materials Science & Engineering
} } } Michigan Technological University
} } } Rm 512 M&M Bldg.
} } } Houghton, MI 49931
} } } PH 906-369-1875
} } } FAX 906-487-2934
} } } mailto:opmills-at-mtu.edu
} } } http://www.mm.mtu.edu/~opmills
} } }
} } } At 11:48 AM 1/8/2004 -0500, Kathleen Roberts wrote:
} } }
} } }
} } } } ------------------------------------------------------------------------------
} } } }
} } } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } } America
} } } } To Subscribe/Unsubscribe --
} } } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } On-Line Help
} } } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } } -------------------------------------------------------------------------------
} } } }
} } } }
} } } } To Joel, Eckhart, Kenneth, Peter, and anyone else who gave me advice-
} } } }
} } } } OK, I finally had a chance to sit down and fiddle with the chiller,
} } } } and here is what I have.
} } } }
} } } } I turned on my Zeiss EM 10CA and checked the flowmeter in the
} } } } column: about 2.2 L/min, if I am reading it right. There was no
} } } } gauge for the chiller flow rate, but there is a pressure gauge on
} } } } the front of the chiller, and it read about 39 psi. This reading
} } } } did not change through the entire test, and neither did the EM
} } } } flowmeter.
} } } } Chiller temperature reading was about 75 degrees F at start. It
} } } } needs to be 68 degrees F, according to the EM's manual. Only the
} } } } "Cool" light was on...all others, including the "Compressor" light,
} } } } were off.
} } } }
} } } } I turned the temperature screw to the left to lower the temp setting.
} } } } No response from the compressor. Turned it down a second
} } } } time....still no response. After about 5 minutes the Compressor
} } } } light turned on, and the temperature started to drop, finally. The
} } } } temperature went all the way down to 53 degrees F, at which point
} } } } the "Lo Temp" light went on, the "Compressor" light went off, and
} } } } the "Heat" light went on. I turned up the temp screw a little bit.
} } } }
} } } } At about 60 degrees F, the "Heat" and "Lo Temp" lights went off and
} } } } the "Cool" and "Pump" lights are on (actually the "Pump" light
} } } } never turned off). It rose to 68 degrees F....and continued to
} } } } rise. I let it get to about 79 degrees F, and the compressor never
} } } } turned back on. I tried turning the screw back to the left to drop
} } } } the temp setting...it never went back on.
} } } }
} } } } At this point, I decided to turn the EM 'scope off....though the
} } } } flow rate never dropped, and the buzzer never went off. The
} } } } temperature gauge on the chiller continued to rise, even after
} } } } turning the 'scope off. It was reading about 90 degrees F when I
} } } } left to come write all of you.
} } } }
} } } } Just now went back in to check the thing...the compressor finally
} } } } came on...it's reading about 53 degrees F and the "Lo Temp" light
} } } } is on, and the "Compressor" light is off.
} } } } So I think it's the switch....or perhaps the "Hi Temp" sensor? Or
} } } } both? I have no idea how all the sensors and switches are
} } } } connected...even with the diagrams and manual that were sent, as I
} } } } have no idea how to read such things (been eons since I did
} } } } circuits in Physics class...). What do you all think?
} } } }
} } } } Thank you all so much for your help-
} } } } Kathleen
} } } } Neurotoxicology Labs
} } } } Rutgers University
} } } }
} } }
} } } Owen P. Mills
} } } Electron Optics Engineer
} } } Materials Science & Engineering
} } } Michigan Technological University
} } } Rm 512 M&M Bldg.
} } } Houghton, MI 49931
} } } PH 906-369-1875
} } } FAX 906-487-2934
} } } mailto:opmills-at-mtu.edu
} } } http://www.mm.mtu.edu/~opmills
} }
} }
}
} Owen P. Mills
} Electron Optics Engineer
} Materials Science & Engineering
} Michigan Technological University
} Rm 512 M&M Bldg.
} Houghton, MI 49931
} PH 906-369-1875
} FAX 906-487-2934
} mailto:opmills-at-mtu.edu
} http://www.mm.mtu.edu/~opmills
}

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In a message dated 1/8/04 4:44:05 PM, tivol-at-caltech.edu writes:

} The take-home lesson is that there still must be knowledgeable
} oversight, especially with regard to automated processes, to assure the
} quality of the results

You'll get no argument from me about that! The point I was trying to make is
that as the tools have become more complex, many of the tasks that we once
dealt with manually (I learned electron microscopy on a Siemens 1A, right on the
Caltech campus, back in the '50's - and as a result I really know what
alignment means, not just how to push a button) are now so automated that they are
hard to control. We may (but may not) be able to spot problems, but the casual
user (shudder) will not know how to correct them.

I think this thread has been interesting primarily in that everyone who has
commented has been in basic agreement that far too many people who use
microscopes understand them, or the ancillary techniques of specimen preparation,
image analysis, etc., well enough to keep out of trouble or get really optimum
results. Clearly they have other priorities than learning all that stuff. I've
taught image analysis courses now to something approaching 3500 people. Even
assuming they all learned everything I wanted them to, that is a drop in the
bucket. And the people who really need it most don't come - at best they send a
technician whom they can subsequently tell to do the work. But that's another
rant.

John Russ

John Russ

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On Jan 8, 2004, at 1:11 PM, Jon Krupp wrote:

} A lab user has asked me to find some place he can get freeze fracture
} work
} done. Close to San Francisco bay area would be best. Reply to me and I
} will
} pass on the contact info.
}
Dear Jon,
If Kent McDonald does not have freeze-fracture, he probably knows
someone in or near Berkeley who does. I don't have his email address
immediately at hand.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

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Steve and to all other Listers

The same is with EPMA (Electron Probe Microanalysis) with EDS.
Unfortunately m o s t manufacturers moved their goals and tried to
develop calculation machines as 'black box'. Because of the giant
improvements in calculation speed of our computers (in last decades),
only one button hit is necessary to display the complete analysis result
(in most cases computer needs a tiny part of a second). The unskilled or
less skilled operators believe in these results, without any concern.
Even element concentration result errors of 0.1% and less are taken from
the computer display as the truth. But such a very high 'accuracy' must
be only the statistical part! The computer speed and modern easy to use
software interfaces cover the very complex and not linear relations
between measured signal and element concentration in specimen. The
iteration process to get result convergence and the systematic and
statistic errors with their error propagation during computing process
are not visible.

I think for future, a more open software is going to be a trend. There
must be a possibility to interact between the knowledge of the
microanalyst and the computer program. A visible and easy
understandable feedback for all computing steps is necessary. Of course,
a higher skilled level of the operator is then necessary. This makes
sense only, if the software give the possibility to share the knowledge
with the operator, which is then really become a microanalyst.

A couple of years ago, I found in a very old German book of C. Remigius
Fresenius "Anleitung zur Qualitativen Chemischen Analyse" ("Guidance to
the Qualitative Chemical Analysis") - Braunschweig 1874:

"Es muss daher ein Halbwissen, wie überall
so ganz besonders hier, für schlimmer als ein Nichtwissen erachtet
und vor oberflächlicher Beschäftigung mit der chemischen Analyse
ganz vorzüglich gewarnt werden."

Translation (I hope the feeling is transfered):
Therefore a partial knowledge, like everywhere so particularly here,
must be worse than even ignorance. It should be warned before
superficial concern with the chemical analysis completely and
excellently here.

These words are still valid and can be used nowadays for EPMA and
Electron Microscopy including image interpretation, as well.

Frank Eggert

Steve Chapman wrote:

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 9 05:35:11 2004

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My two cents worth on a subject that has quite a few here tossing their own
around.

Having spent 25 years in this area, I've had the opportunity to see the
initial investigations of this practical application of sub-atomic particle
physics in basic research labs as well as its resultant spread to a wide
variety of industries. The use of SEM analysis has become a commodity
because it is so successful in so many areas. Decades ago, many were
researching the potential applications, and in virtually each case, they
found the usefulness.

I can't begin to tell you the variety of areas where my customers have
found the SEM useful. From missle guidance systems to electron beam
lithography. Particulate analysis of howitzer oils to particulate
contaminant analysis of sausage casings. The taxonomical classification of
emerging bacterial species to process control for the laser produced
hologram labels used for software copyright and federal IDs.

The fact is that the SEM has perhaps been too successful. We still hold in
reverence the atomic physicists who can design an atomic bomb or understand
the results from particle accelerators. But the SEM is a child of these
processes that has found wide spread use and the demands for its
application greatly exceed the number of those who really understand the
underlying processes, much less the proper application of the various
subtleties of its application.

I've had to deal with this over the years as the operators I deal with have
changed from those individuals who first brought an SEM into a lab to the
'checklist' operators who know nothing about the instruments other than the
written sequence of actions to turn it on and get an image. One of the
challenges in my work is to try to encourage the SEM operators to learn and
think more about the consequences of each turn of a knob or click of a
mouse. As a maintenance provider, it certainly helps me if my customers
have some understanding of their machines - but more importantly, it helps
them do better work. SEMs aren't the only problems here - x-ray
spectroscopy in fluorescence or the SEM based microanalysis is another area
where operators are often fooled into thinking that results are a simple
matter of a set routine.

The computerization of the instruments is furthering the problem. While
the manufacturers are seeking only to play to the market, how many
operators really understand what's happening when they tell their computer
to bring up an FE gun? It really started with simple improvements such as
electronic gun adjustments. When an operator had to physically move the
gun assembly around, it made some sense that the position of the gun was
important to aim the beam down the column. How many really understand the
use of magnetic fields in the gun to tilt and shift the beam to alignment?
Most that I see at first only know that they have to tweak these knobs and
watch for an improvement in the signal.

Like it or not, this trend will continue. But it is not selective to SEMs
- I see similar trends in every analytical instrument. As these
instruments become more 'user friendly', they are actually lulling users
into thinking that all that is needed is a brief glimpse at the user
manual, which usually only describes how to push the buttons. IR, GC, LC,
MS, ICP and many other techniques that involve complex physics have been
reduced to a simplicity that masks their proper use primarily because those
using them and buying them want simple answers. A material scientist
investigating ceramics doesn't want to have to learn the sub-atomic
particle interactions involved, he just wants pretty pictures that explain
a manufacturing fault and justify the expense of the SEM, not to mention
his job.

'Ease of use' is a marketing tool, and as such, it is a primary goal of
manufacturers. I don't mean to focus on them, because it is a vicious
circle - the customers are demanding it, the manufacturers simply provide
it. In this process, though, what gets lost is that the proper use and
interpretation of these instruments requires more than the customers are
wanting to afford and more than the manufacturers are wanting to admit to.

Now Steve's attention is a little more esoteric - the quality control of a
reviewed paper. But doesn't that just follow from the above? The results,
rather than the process, are what matter most now. More and more we see
examples in studies that are published, only to be later refuted. NASA's
claim a couple of years ago about evidence of ancient bacteria in Mars
based rock found in the Antarctic has, last I knew, been lost in dispute.
Pons and Fleischman, and Gallo, are of course extremes, but how much of
what is accepted as reputable science has later fallen as poor science. A
brief look at medical headlines over the past decade or two can give a good
glimpse. Science itself is supposed to ensure honest and accurate results,
and the assumption of most people, scientists included, is that anything
purporting to be science, promoted by supposed scientists, has some truth.
Innocent until proven guilty, so to say.

Whether authored by lack of knowledge of instrumental techniques, lack of
personal integrity or poor selection of measured variables, many papers get
published that should have been caught by reviewers. That's assuming that
those reviewers are well versed in all aspects of a particular paper. But
given the wide variety of instrumental techniques available today, it can
be a daunting task to find a single person expert in all of the
instrumental techniques presented in a paper, not to mention the basic
field of the paper and mathmatical aspects. If a reviewer isn't well
versed in all aspects and techniques of a particular paper, can he be
expected to catch the kind of cross-discipline problem in your example?
Since much goes unsaid in virtually any paper, should reviewers be
required to request all details of sample provenance - the collection,
preparation and analysis?

By the way, Steve, was there any mention, in the example you cited, whether
the sample was coated or not, or is it an assumption of yours that is
wasn't?

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174
ph. (630) 513-7093 fax (630) 513-7092 web http://www.sem.com

-----Original Message-----
} From: Steve Chapman [SMTP:protrain-at-emcourses.com]
Sent: Wednesday, January 07, 2004 6:42 AM
To: MSA

Hi Listers

As many of you may know I run a training organisation that travels world
wide spreading the word on SEM, TEM and EDS operation. I also have a deep
interest in "Quality in Electron Microscopy"as those who picked up our
paper
last year would know?

Now to the point. Once again I am picking up respected journals and
finding
examples of what I would call poor microscopy, but in truth it also
demonstrates poor quality control!

To bring one image to mind. The micrograph is of a structure which is
described as being an example of a smooth surface on a biological material.
But, the micrograph was taken at 20kV, where the vast majority of the
information will have come from beneath the surface softening the true
surface detail.

First to remove the training aspect . Operators of SEM should be taught
that
by manipulation of kV and working distance one may subdue or enhance
surface
features. To use more than 10kV on most biological samples is asking for
sub surface detail, ignore this and comments on surface irregularities are
null and void in my mind. (I have to say I would probably try to use 2 to
5kV if the microscope used was produced in the last 15 years!)

Now the quality aspect. By the time a paper is published a number of steps
should have been taken. Working backwards, the publisher should have the
paper vetted by knowledgeable scientists who would be able to pick out the
problems that I see and have them corrected prior to going to print. Next
back in the chain is the laboratory that was involved with the scientist;
did they check the quality of the work leaving their EM unit? Stepping
back
again did the scientist take the micrographs or did they receive help?
Either way the training of staff and operators should overcome this type of
problem! But if the results the staff and visiting operators produce are
not assessed how do you know that their training is inadequate?

As the pressure to perform increases and funding decreases only the cream
of
our laboratories will remain. In industry there is no question about
following rigid "Quality" procedures and it is not too far off that this
will hit the world's EM units too! I know that this is my baby but is it
not about time that we woke up to these facts?

There is an area where I believe we have room for discussion; what do you
think?

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0) 7711 606967
www.emcourses.com

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 9 08:38:55 2004

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Hi Faye,

I cannot help you with your MAC and the software but
if you need an adapter for your Fuji S602Z and a microscope
I can help you. We have adapters for all kind of digital
cameras either for C-Mount or eye-pieces. Let me know if
you want to know more about it.

Unfortunately our web site is not in english yet. However
you can find the list of digital cameras we support here:

www.klughammer.de - enter the german pages, then open
"Kameraadapter" - "für dig. Kameras" - go to the bottom of
this page there you find "Kameraübersicht (PDF)", open it
and then you get an overview of cameras.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

bwoAAM} ------------------------------------------------------------------------------
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bwoAAM} Email: faj-at-highway1.com.au
bwoAAM} Name: Faye Taylor

bwoAAM} Organization: Amateur

bwoAAM} Education: Undergraduate College

bwoAAM} Location: Perth, Western Australia

bwoAAM} Question: Hello there,
bwoAAM} I am a starter who wishes to get her grandchildren interested in a
bwoAAM} world beyond TV & computer games. I started using computers when I
bwoAAM} purchased my first 128K Mac back in 1985 . My present Mac is a G3
bwoAAM} 192MB ram & 40 GB hard drive.

bwoAAM} I recently aquired a second hand
bwoAAM} "MOTIC Biological Series B1 223A " but I have found that I cannot
bwoAAM} use my lovely Fuji S602Z digital camera to take photos.

bwoAAM} Do you have any ideas which will enable me to combine the use of the
bwoAAM} hardware that I possess?
bwoAAM} I feel that the hardest part is getting software that will enable me
bwoAAM} to join up to the Macintosh even if I purchased a new camera.

bwoAAM} I would really like to take the photos digitally but is it impossible
bwoAAM} with my present configuration?
bwoAAM} i would appreciate any comments please

bwoAAM} Happy New Year Faye

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 9 12:46:37 2004

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Dear Jon,
Caroline sent this to me; please pass it along to your colleague.

Begin forwarded message:

} Bill -
}
} Kent gave my old machine to a woman in SF who is running it for hire;
} I don't know anything about her or the quality of her work. Look at
} www.nanoanalytical.netfirms.com .
}
} Caroline
}
} --
} Caroline Schooley
} Project MICRO Coordinator
} Microscopy Society of America
} Box 117, 45301 Caspar Point Road
} Caspar, CA 95420
} Phone/FAX (707)964-9460
} Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
}
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 9 14:49:55 2004

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Email: srw6y-at-virginia.edu
Name: Steven

Organization: UVA School of Medicine

Title-Subject: [Microscopy] [Filtered] Scion Image "Set Scale"

Question: The lab where I currently work uses Scion Image, a freeing
distributed graphical editing program. I have been having a problem
with the "Set Scale" option under the "Analyze" tab. After taking a
snapshot of a known scale under the microscope, I set the scale
accordingly by typing in the known distance and setting the units to
micrometers. When I switch to a different image and wish to use the
same scale, the scale I have just calibrated has been reset to the
default. Also, I have gone under the "file" tab and clicked on
"record preferences," which seems to do nothing. No save box opens,
and I am left with my cursor. In addition, the "revert to save
option," also under the "file tab" is never illuminated.

How can I set the scale so it will be calibrated for all images open
in the editing session?

Thanks and I hope someone out there has some answers.

Steven

---------------------------------------------------------------------------

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Good morning,

I am trying to help a plant biology student with some plant histology on
mango saplings. She is interested in looking at paraffin sections of the
woody stems (LM). Does anyone have suggestions for a processing schedule? I
have my processor set up for human tissues but I could easily extend the
programmes to accomodate the cellular nature of the material. Having some
suggestions would greatly cut down my trial and error!

Many thanks,

Evelyn Kaplan,
Dept of Pathology,
College of Medicine and Health Sciences,
Sultan Qaboos University,
Oman

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 10 00:57:39 2004

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Dear friends,
the Italian Master on Microscopy at University I Level is starting on
February 2nd, 2004. Only few positions are still available due to a
delayed registration on January 19th, 2004.
Details can be found at "Master Universitario di I livello in
Microscopie ed Analisi Microscopiche in Biologia"
http://www.studenti.unige.it/corsi/master.html and at www.lambs.it.
All my best
Alby

p.s. for further information, please e-mail to diaspro-at-fisica.unige.it
using "microscopy master 2004" as subject.

.......................................................................
...................................
.. non basta, resistere, resistere...resistere
^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
Alberto Diaspro
Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genoa, Italy
voice: +39-0103536426/480 fax 010314218
diaspro-at-fisica.unige.it, http://www.lambs.it
http://wiley.com/cda/product/0,,0471409200,00.html

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 11 10:11:10 2004

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} }
} } Does anyone have a copy of the book "The Cell", 2nd Edition, by Don
} } Wayne Fawcett, MD that they are willing to cell. This is a classic book
} } full of electron micrographs. I am a graduate student and I will be
} } taking an electron microscopy lab this semester and I am looking for 1
} } or more copies of this book.
} }
} } Please reply to hiswayt-at-earthlink.net
} }
} } Thank you.

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 11 10:33:04 2004

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Evelyn,

We occasionally embed plant samples for LM and make a few changes over
what is customary for animal tissue. First of all plant samples do not get
as brittle if dehydrated in a TBA (tertiary butyl alcohol)/ETOH series
ending with 100% TBA.

Start with 15 min in each of 25 and 50% ETOH.
Dehydrate for ~ 2-4hrs in each of the following percents:
90 ETOH - 10 TBA
80 ETOH - 20 TBA
65 ETOH - 35 TBA
45 ETOH - 55 TBA
25 ETOH -75 TBA
100% TBA - 3 changes for at least 4hrs total time

Infiltration is helped along by the following:
Put samples into an oven set at a sufficiently high temperature to melt your
paraffin. (I put all the cassettes into a beaker large enough to hold them
so they are completely covered by TBA and then add room for the paraffin.
Add solid paraffin (paraplast) to container and allowing it to gradually
melt and mix with TBA. The TBA gradually evaporated. The paraplast is then
changed a total of 3x over a period of a couple of days prior to embedding
tissue in molds.

It is also advisable to use subbed slides or slides coated with poly
L-lysine (100µg/ml in 10mM tris at pH 8.0). Plant cell walls tend to lift
from the slide surface during staining.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 1/10/04 12:55 AM, "Evelyn Kaplan" {ekaplan-at-squ.edu.om} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
}
}
} Good morning,
}
} I am trying to help a plant biology student with some plant histology on
} mango saplings. She is interested in looking at paraffin sections of the
} woody stems (LM). Does anyone have suggestions for a processing schedule? I
} have my processor set up for human tissues but I could easily extend the
} programmes to accomodate the cellular nature of the material. Having some
} suggestions would greatly cut down my trial and error!
}
} Many thanks,
}
} Evelyn Kaplan,
} Dept of Pathology,
} College of Medicine and Health Sciences,
} Sultan Qaboos University,
} Oman
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 11 12:40:08 2004

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} }
} } } Does anyone have a copy of the book "The Cell", 2nd Edition, by Don
} } } Wayne Fawcett, MD that they are willing to cell. This is a classic book
} } } full of electron micrographs. I am a graduate student and I will be
} } } taking an electron microscopy lab this semester and I am looking for 1
} } } or more copies of this book.
} } }
} } } Please reply to hiswayt-at-earthlink.net
} } }
} } } Thank you.

If you look at the used book search site www.abebooks.com you'll find
10 copies at prices from $9-$75.
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 09:54:06 2004

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Evelyn,

I have used these old protocols with success on woody materials. Put
plant material always requires greatly extended times compared to
animal tissue. Also, if you have problems with tearing of the embedded
tissue during sectioning you can soften the embedded material in
Gifford's solution (below). The difficulty is trying to get the harder
tissue soft enough so it doesn't tear the softer tissue during
sectioning.

The details we used are as follows:
Fixation for 12 to 48 hours in FAA (you might also try Navashin's
fixative which contains chromic acid)
Infiltrate through TBA series (Johansen series) for 2 hours each step
3 changes of pure TBA over 24 hours
3 changes of Paraplast over 24 hours
Embed

Soften the blocks by soaking overnight to 7 days in water at up to 38°C
If this doesn't work try 2 days to 2 weeks in Gifford's (room temp in
fume hood):
20 ml glacial acetic acid
80 ml 60% ethanol
5 ml glycerine
You will have to try the softening times with your own tissue. If you
leave it too long the soft tissue will become macerated. Let me know if
you need more detail.

Good luck,

Kim

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 10:00:07 2004

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We have recently acquired a Pelco Biowave and are in the process of
acquainting ourselves with it. Currently, I am trying to fix two species
of insects with it for SEM (Colorado potato beetle larvae and Diamond
back moth larvae). A literature search has not turned up much
information on microwave processing for insects. I have tried
adaptations of the standard protocol (2% glut, rinse, 1% osmium, rinse,
ethanol dehydration, critical point dry) at various microwave wattages,
times, and with vacuum applied. So far, I have not achieved reproducible
results for either insect. While I plan on more trial and error, I was
wondering if anyone has a microwave protocol for insects or any advice
on this.

Shannan Little
Research Technician/Technicien de recherche
Electron Microscopy and Image Analysis /
Microscopie électronique et Analyse d'images
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 403-317-3446
Facsimile/Télécopieur: 403-382-3156
P.O. Box 3000 / CP 3000
Lethbridge, Alberta T1J 4B1
littlesm-at-em.agr.ca
http://res2.agr.ca/lethbridge/emia/index_e.htm

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 10:00:47 2004

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Dear all,
We would be interested in users comments about EBSD systems. In
particular, we are looking at the systems offered by HKL and by TSL/EDAX.
Please comment on some of the following points:

* Ease of use

* Robustness/reliability of indexing when dealing with low symmetry
structures

* Calculation of GB misorientations and display of crystallographically
equivalent misorientations

* Possibilities for generating different types of map (e.g. orientation,
GB misorientation, phase)

* Correlation with EDXS data or maps / generation of combined maps

I look forward to hearing from you. Please copy all responses to myself
and to Martin Lee {m.lee-at-earthsci.gla.ac.uk}

Thanks and best wishes

--
Ian MacLaren
Technische Universität Darmstadt
Material- und Geowissenschaften
Petersenstr. 23
64287 Darmstadt
Germany
http://www.tu-darmstadt.de/fb/ms/fg/sf/projekte/maclaren-Dateien/maclaren.html

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 10:32:46 2004

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I have been calibrating my recently installed Philips TEM with a grating
replica and I need some suggestions. At a print magnification of about
80KX I see about a 1% variation in my calculated magnification depending
where I select my stop and start marks.

How much variation should I expect in magnification due to changes in lens
voltage and current?

Thanks!!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 10:46:04 2004

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Frank,
I suspect that these variations are in the grating itself, not your
TEM. They can be a bit variable, depending on stretching and buckling from
the preparation process. We have a record of measurements of semiconductor
standard samples going back 8 years on our Jeol 120CX TEM, and find a
reproducibility better than 1% over this time.
There is a change in magnification from the centre to the edge of the
micrographs on our machine of about 1%, but our microscope is now pretty
ancient and I would hope that newer machines are much better than this.
We are about to embark on a full gauge capability test on the machine,
which should be interesting. I can let you know the results of the study if
you like.

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

-----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
Sent: 12 January 2004 16:18
To: microscopy-at-msa.microscopy.com

I have been calibrating my recently installed Philips TEM with a grating
replica and I need some suggestions. At a print magnification of about
80KX I see about a 1% variation in my calculated magnification depending
where I select my stop and start marks.

How much variation should I expect in magnification due to changes in lens
voltage and current?

Thanks!!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

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From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 11:13:40 2004

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Dear fellow microscopists

In my experience, successful microwave fixation
depends mainly upon the size of the specimen.
How big are these insects? Second, if the larvae
are difficult to penetrate (I have no idea),
longer times may be required. You might also
consider Karnofsky's fixative instead of
Glutaraldehyde (I found that it improved results
in many cases over a wide variety of specimen
types, although I didn't try insects). I would
try lengthening the primary fixation time before
adjusting any of the other processing variables.
Fixation temperatures should never exceed 50°C (I
don't know what this translates to in watts on
your Biowave), or you will get "crispy critters".

best regards,
Steven Slap
Microwave Consultant

At 11:04 AM -0500 1/12/04, Shannan Little wrote:
} We have recently acquired a Pelco Biowave and are in the process of
} acquainting ourselves with it. Currently, I am trying to fix two species
} of insects with it for SEM (Colorado potato beetle larvae and Diamond
} back moth larvae). A literature search has not turned up much
} information on microwave processing for insects. I have tried
} adaptations of the standard protocol (2% glut, rinse, 1% osmium, rinse,
} ethanol dehydration, critical point dry) at various microwave wattages,
} times, and with vacuum applied. So far, I have not achieved reproducible
} results for either insect. While I plan on more trial and error, I was
} wondering if anyone has a microwave protocol for insects or any advice
} on this.

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 11:46:35 2004

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FYI
I just opened a new supply of Kodak Professional Rapid Fixer and
found larger boxes. After the film switch not so very long ago, I
decided to check the ingredients. "Solution A" now has Ammonium
Sulfite, Sodium bisulfite and Sodium acetate added to what was
printed on the old box. The mixing directions are the same 1999
version. "Solution B" and the CAT # 146 4106 appear to be the same.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 11:53:21 2004

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We are trying to install two cameras on a Windows XP computer.

We cannot get XP to recognize both the Sensicam PCI card and the Roper PCI
card. It's completely an exclsuive or installation. We've poked around
the Device driver menu and downloaded the most recent drivers.

Has anybody figured out how to install both these camera simultaneously?

____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 12:01:24 2004

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I would recommend the Mag-I-Cal sample for calibrating your TEM. You can do a much larger range of Magnification settings than using a replica. I think that the error is 1 to 2%. In addition, you can do rotation and camera constant calibrations with the same sample.

One thing to minimize the variation in the microscope is to always changed the lenses in the same direction to avoid hysterisis and to make sure that you are at the eucentric point so that the obj lens is the same. Again, you should bring the focus from the same direction.

If the goniometer has not bee removed or the column split, the values that you get from time to time should be very close. We had to run calibration twice a year on the TEM. I can't remember the range specifically, but I think that the variation in mag was less than 0.5% and may have been better than 0.1% when the above criteria was met.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
Sent: Monday, January 12, 2004 11:18 AM
To: microscopy-at-msa.microscopy.com

I have been calibrating my recently installed Philips TEM with a grating
replica and I need some suggestions. At a print magnification of about
80KX I see about a 1% variation in my calculated magnification depending
where I select my stop and start marks.

How much variation should I expect in magnification due to changes in lens
voltage and current?

Thanks!!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 12:53:50 2004

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When we manufacture TEM or SEM gratings we make them from a replica of a
master grating. When you dissolve away the replication material there is
some shrinkage, but it should be very limited. The shrinkage is inherent in
the manufacturing, but we cull any which show problematic shrinkage.
It is very similar to our carbon substrate manufacturing.

John Arnott

Disclaimer: Ladd Research manufactures and sells the gratings, replicating
materials and substrates mentioned in this email.

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com

----- Original Message -----
} From: {Frank.Karl-at-degussa.com}
To: {microscopy-at-msa.microscopy.com}
Sent: Monday, January 12, 2004 11:17 AM

Frank,
If you are using film, a second variation in measurement may come
from the enlarger when you print the picture. If the negative is not
supported on glass, it can bow in the center and distort the
measurement a bit.

It was a surprise to me to find that if I had set my "MAG. ZERO"
early in the morning and then checked it later in the day, there was
frequently a slight change. It was explained to me that in an old
building, when there was a greater draw of electricity, a change
could be expected and for really important work, I should
re-calibrate. Am I just gullable?

My favorite goof has been the result of not adjusting my tilting
specimen holder to read 0 degrees!

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
}
} When we manufacture TEM or SEM gratings we make them from a replica of a
} master grating. When you dissolve away the replication material there is
} some shrinkage, but it should be very limited. The shrinkage is inherent in
} the manufacturing, but we cull any which show problematic shrinkage.
} It is very similar to our carbon substrate manufacturing.
}
} John Arnott
}
} Disclaimer: Ladd Research manufactures and sells the gratings, replicating
} materials and substrates mentioned in this email.
}
} Ladd Research
} 83 Holly Court
} Williston, VT 05495
} On-line Catalog: http://www.laddresearch.com
} tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
} fax: 1-802-660-8859
} e-mail: sales-at-laddresearch.com
}
} ----- Original Message -----
} } From: {Frank.Karl-at-degussa.com}
} To: {microscopy-at-msa.microscopy.com}
} Sent: Monday, January 12, 2004 11:17 AM
} Subject: [Microscopy] TEM mag question
} -----------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
}
} } I have been calibrating my recently installed Philips TEM with a grating
} } replica and I need some suggestions. At a print magnification of about
} } 80KX I see about a 1% variation in my calculated magnification depending
} } where I select my stop and start marks.
} }
} } How much variation should I expect in magnification due to changes in lens
} } voltage and current?
}
} } Frank Karl

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 15:39:11 2004

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Dear friends,

I wanted to know the vapor pressure of alumina (Al2O3) at 1200 C.
I know that it will be very low, but an estimate would also
be helpful. I looked at various places (such as CRC handbook of
Physics and Chemistry, Handbook of thermophysical properties of solid
materials, ASM handbook, Vol. 5), but got values above 1950C (e.g.
10^-3 torr at 1950 C).

I want to know the answer to this question since I work at vacuum
levels of 10^-6 to 10^-8 torr and at 1200C. I am interested in knowing
if the aluminum oxide layer on my samples evaporates under these
conditions. One company representative said that it wont, but he did not
have vapor pressure values to support the assertion.

thanks in advance

Rahul Panat
Univ of Illinois
Urbana, IL

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 17:23:47 2004

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Email: hadden-at-wingate.edu
Name: Lee Hadden

Organization: Wingate University

Title-Subject: [Microscopy] [Filtered] Kodak 4489 EM film

Question: Can anyone use some left-over Kodak 4489 electron
microscopy film? I was about to throw out 5 boxes [2 x 10 in. 100
strips per box] during "housecleaning" the other day, but thought
there might be someone who could use it. It has been refrigerated
and unopened for about 12 years. [I used to use it in our old RCA EMU
3G TEM.]
If someone wants it send me your mailing address and I'll ship it out
to you. Otherwise, it will be recycled or trashed.

Lee Hadden
Department of Biology
Wingate University
Wingate, NC 28174

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 17:24:33 2004

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Email: ryan.davis-at-hydro.com
Name: Ryan Davis

Organization: Metallurgical Engineer

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am interested in getting quantitative analysis training
for analyzing aluminum alloys and oxides. In our lab, we have an
Hitachi S-3500N equipped with an Oxford EDS Spectrometer (model#
7021)that has the INCA and ISIS software packages installed on the
computer. I would like to visit an independent laboratory or
university for a week or two for training. If someone could assist me
I would appreciate it.

Regards,

Ryan Davis

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 18:21:33 2004

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} } Hello Shannan.
}
} I have some experience with microwave fixation of Drosophila larval
} salivary glands for TEM. First, I run my cold spot -at- 15-18 degrees (this
} removes the heating effect) I fix them in Karnovsky's fix power level
} 1(100 watts on my MW) for 1 minute on-1minute off-1 minute on). Then I
} turn the power up to 450 watts (power level 4 on my machine) and pulse for
} 30 seconds on-30 seconds off-30 seconds on 3 times.They should not get
} hot! I let sit on the bench in fixative for 5 minutes. I have also tried
} this protocol on zebrafish larvae (with vacuum) and they are well fixed.
} The insect probably has a cuticle which may hinder the penetration of the
} fixative. If you can find a way to partially remove this, or inject the
} fix then MW, you might have better results.
} For osmium fix, I repeat the above timetable. I dehydrate under vacuum 45
} seconds -at- power level 3(350 watts) 50, 70,95% once each. I do 100%
} ethanol 3 times followed by 100% acetone before infiltration in resin.
} Hope this helps, JoAnn Buchanan
}
}
} } We have recently acquired a Pelco Biowave and are in the process of
} } acquainting ourselves with it. Currently, I am trying to fix two species
} } of insects with it for SEM (Colorado potato beetle larvae and Diamond
} } back moth larvae). A literature search has not turned up much
} } information on microwave processing for insects. I have tried
} } adaptations of the standard protocol (2% glut, rinse, 1% osmium, rinse,
} } ethanol dehydration, critical point dry) at various microwave wattages,
} } times, and with vacuum applied. So far, I have not achieved reproducible
} } results for either insect. While I plan on more trial and error, I was
} } wondering if anyone has a microwave protocol for insects or any advice
} } on this.

Department of Molecular and Cellular Physiology
Stanford University School of Medicine
Stanford, CA 94305
650-723-5856

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 19:07:09 2004

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Michael,
Have you tried rearranging the cards on the Mobo? I had the same adventure
when installing a Pixera camera and Scion system on an XP system. I did not
get the New Hardware Found announcement for the Pixera card until I did some
card swapping.

Let me know how you get on.

Greg

Dr. G. F. Barclay
Plant Science Unit, Dept of Life Sciences
University of the West Indies
St. Augustine, Trinidad and Tobago
West Indies
Phone: 868 645 3232 ext 3112/2045
Fax: 868 645 7132

} From: Michael Cammer {cammer-at-aecom.yu.edu}
} To: microscopy-at-MSA.microscopy.com
} Subject: [Microscopy] Sensicam QE & Roper HQ
} Date: Mon, 12 Jan 2004 12:58:55 -0500
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_________________________________________________________________
Help STOP SPAM with the new MSN 8 and get 2 months FREE*
http://join.msn.com/?page=features/junkmail

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 20:02:39 2004

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Dear Shannan,
Below is a method we have used for a few different insect types, for TEM
not SEM, but the fixing steps we use might provide a useful comparison at
least.

With SEM I assume you won't want to dissect your samples prior to
processing (as we did) so penetration of the solutions may be more of a
problem, but then the requirements for fixation for SEM are also less
stringent. The microwave conditions may be useful guidelines but of course
you'll have to determine the conditions for your own microwave and samples.
If you haven't already got them, I strongly recommend Gary Login's text
(Login, G. R., & Dvorak, A. M. (1994) " The Microwave Toolbook A Practical
Guide for Microscopist" Boston: Beth Israel Hospital) and Kok and Boon's
book "The Microwave Cookbook for Microscopists", Boon and Kok, Coulomb
Press Leiden, 1992.

Method:
Primary fix: 3% glutaraldehyde in 0.1M Na cacodylate, pH 7.4.
Samples dissected out and placed into the primary fix solution (in a small
plastic petri dish).

They were then put into fresh fixative (specimen containers for a Leica AFS
were
used inside the petri dish) and microwave irradiated as follows:

EMS lab microwave oven setup:
-a dummy load of 100ml dw at 20degC in a 250 glass beaker was used (always
in the same place - right rear corner for us)
-temperature limiting off
-100% 'power' (ie magnetron on continuously)
-sample volume for all the fixing steps was 4.0ml
-magnetron was pre-warmed for 2 minutes with a load of 500-600ml water
before each step (unless the oven was used less than 2 minutes earlier).

1) Microwave Primary Fixation:

The sample in 4 ml of primary fix is irradiated for (7s) to give a final
temperature of about 50degC - check the temperature after irradiation (and
obviously before you use your actual samples if you're doing this for the
first time) and alter subsequent run times if necessary. (We use the spot
in the oven we deem to be receiving a steady, high level of radiation).

Allow sample to sit in fume cupboard in fix container for 3 minutes to cool
it to room temp before removing fix.
Replace fix with fresh and repeat the irradiation process twice.
A cool dummy load must used with each run.

Leave samples in fume cupboard for 30 minutes at room temperature.

2) Rinse the samples:

Three X 10 minutes in 0.1M cacodylate buffer.

3) Secondary fixation:

Place 2% OsO4 in 0.1M cacodylate buffer into fix dish with specimens.
Irradiate for 7s
Leave for 40 minutes in the OsO4.

4) Rinse with 0.1M cacodylate buffer

Three X 10 minutes

The remainder of my method is for TEM preparation so you could do your
usual pre-drying and drying steps then.

Regards,

Richard

}
} We have recently acquired a Pelco Biowave and are in the process of
} acquainting ourselves with it. Currently, I am trying to fix two species
} of insects with it for SEM (Colorado potato beetle larvae and Diamond
} back moth larvae). A literature search has not turned up much
} information on microwave processing for insects. I have tried
} adaptations of the standard protocol (2% glut, rinse, 1% osmium, rinse,
} ethanol dehydration, critical point dry) at various microwave wattages,
} times, and with vacuum applied. So far, I have not achieved reproducible
} results for either insect. While I plan on more trial and error, I was
} wondering if anyone has a microwave protocol for insects or any advice
} on this.
}
} Shannan Little

Richard Easingwood
Otago Centre for Electron Microscopy
Department of Anatomy and Structural Biology
School of Medical Sciences, University of Otago
PO Box 913, Dunedin, NEW ZEALAND
Telephone: 0064 3 479 7301
Facsimile: 0064 3 479 7254
GSM: 0064 21 222 4759
mailto:richard.easingwood-at-stonebow.otago.ac.nz
Web site: http://ocem.otago.ac.nz/

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 21:28:45 2004

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We swapped cards all over the place. The one in the lowest slot gets
recognized, but not the other. Also, the Roper card doesn't seem to
work in the highest slot, even alone. We could get either card to work
with a firewire camera in another slot, but the Retiga we have isn't low
noise enough for this application.
I think we'll have to temporarily get a second computer in the room.
Thanks.

On Tue, 13 Jan 2004, gregor barclay wrote:

} Michael,
} Have you tried rearranging the cards on the Mobo? I had the same adventure
} when installing a Pixera camera and Scion system on an XP system. I did not
} get the New Hardware Found announcement for the Pixera card until I did some
} card swapping.
}
} Let me know how you get on.
}
} Greg
}
}
}
} Dr. G. F. Barclay
} Plant Science Unit, Dept of Life Sciences
} University of the West Indies
} St. Augustine, Trinidad and Tobago
} West Indies
} Phone: 868 645 3232 ext 3112/2045
} Fax: 868 645 7132
}
}
}
}
}
} } From: Michael Cammer {cammer-at-aecom.yu.edu}
} } To: microscopy-at-MSA.microscopy.com
} } Subject: [Microscopy] Sensicam QE & Roper HQ
} } Date: Mon, 12 Jan 2004 12:58:55 -0500
} }
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } We are trying to install two cameras on a Windows XP computer.
} }
} } We cannot get XP to recognize both the Sensicam PCI card and the Roper PCI
} } card. It's completely an exclsuive or installation. We've poked around
} } the Device driver menu and downloaded the most recent drivers.
} }
} } Has anybody figured out how to install both these camera simultaneously?
} }
} }
} }
} }
} } ____________________________________________________________________________
} } Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of
} } Med.
} } Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
} } (718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/
} }
} }
}
} _________________________________________________________________
} Help STOP SPAM with the new MSN 8 and get 2 months FREE*
} http://join.msn.com/?page=features/junkmail
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 12 22:57:10 2004

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Dear all,

We have an old Wild M8 dissecting microscope with a 1.0x objective that can
be converted to 0.4x or 1.6x by clipping adapter lenses onto the bottom of
the 1.0x objective. We'd like to get a second set for another M8 because
they get used so much now that they are sometimes needed by both
microscopes. Unfortunately, these are no longer available from Leica,
instead you have to get an adapter and rather more expensive 0.4x and 1.6x
objectives. These new objectives are better quality than the old adapters,
but for our work, the ease of switching with the adapters and low cost
outweighs the marginal increase in quality at the magnifications we're
using.

Anyone willing to part with their adapters, or know of a source? I've
tried ebay and several other used equipment sites with no luck so far.

0.4x adapter lens part no. 367898
1.6x adapter lens part no. 367916

Thanks much,
Rosemary White

Dr Rosemary White rosemary.white-at-csiro.au
Microscopy Centre fax 61- 2 6246 5000
CSIRO Plant Industry ph. 61- 2 6246 5475 or
GPO Box 1600 mob. 61- 0402 835 973
Canberra, ACT 2601, Australia

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 07:23:25 2004

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Dear fellow microscopists

Richard makes some good points here. I second
his reading recommendations, and want to let
everyone know that there is a brand new edition
of Kok and Boon, Microwaves for the Art of
Microscopy, Coulomb Press, Leiden, 2003, which
has some very useful new information.

I believe that the use of a dummy load is not
needed in the Biowave, which has a recirculating
water cooler. In any event, the end temperature
of 50°C is the key, and Richard's 3 x 7 minutes
should give Shannon a good starting point for
time in the fixative. I would be a little
concerned about using such a small volume of
fixative as Richard did (4.0 ml), both because of
a fear of exceeding the temperature set point and
because a greater volume of fixative to specimen
ratio seems prudent based upon my experience with
light microscopy specimens. I generally work
with about 11.0 ml of fixative.

best regards,
Steven Slap
Microwave Consultant

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 07:44:35 2004

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O.k., folks following the various recommendations from the list for flatbed
scanners we got an Microtek AtrixScan 2500f.

So now, anyone out there with a Microtek 2500f what is the part number
and where do you get the bulbs from?

Microtek offical position is "There are no user servicable parts. You have
to ship it back - at your cost - to Microtek in California for repair". Now, I am
not shipping a 100lb scanner back to California for a $20 bulb replacment - let
alone doing it every 6-8 months. Surely someone else out there has already
come across this (especially since the bulbs never power down).

Thank you in advance for any help.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 08:21:32 2004

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Ryan, Lehigh U. has some excellent courses in this field but they are in
usually in June.

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.
(203) 575-5750

ryan.davis-at-hydro.com (by way of MicroscopyListserver)
01/12/04 06:30 PM

To
microscopy-at-ns.microscopy.com
cc

Subject
viaWWW: quantitative analysis training

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Email: ryan.davis-at-hydro.com
Name: Ryan Davis

Organization: Metallurgical Engineer

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am interested in getting quantitative analysis training
for analyzing aluminum alloys and oxides. In our lab, we have an
Hitachi S-3500N equipped with an Oxford EDS Spectrometer (model#
7021)that has the INCA and ISIS software packages installed on the
computer. I would like to visit an independent laboratory or
university for a week or two for training. If someone could assist me
I would appreciate it.

Regards,

Ryan Davis

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 08:26:02 2004

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Rahul,

My tables* go down to 10^-6, and Al2O3 reaches that vapor pressure at
1637C. I expect that the vapor pressure would be well below your vacuum
level at 1200C.

*The Characterization of High Temperature Vapors, J. L. Margrave, Ed.
John Wiley, 1967.

John Friel

--
---------------------------
John J. Friel
Princeton Gamma-Tech
1026 Rte. 518
Rocky Hill, NJ 08553
(609) 924-7310 x232 phone
(609) 924-1729 fax
E-mail: jjf-at-pgt.com
Web page: www.pgt.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 09:51:03 2004

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Michael,

I can't give you definite answer, but a couple of hints that may help you:

1) Some PCs sense the existence of cards in the slots and turn off the slots
if no card is present. Perhaps the higher slots get turned off. Check in the
BIOS if the computer is in some kind of power saving mode.

2) Take it one at a time. Install one card and get it to work. then take
that card out and install the other card in another slot. If you get that to
work, put the first back in and install again.

3) If one card is not recorgnized, check if there are any conflicts in the
device manager.

4) If one card does not work at all, contact the manufacturer and get their
help.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Michael Cammer [mailto:cammer-at-aecom.yu.edu]
Sent: Monday, January 12, 2004 20:34
To: gregor barclay
Cc: microscopy-at-MSA.microscopy.com

We swapped cards all over the place. The one in the lowest slot gets
recognized, but not the other. Also, the Roper card doesn't seem to
work in the highest slot, even alone. We could get either card to work
with a firewire camera in another slot, but the Retiga we have isn't low
noise enough for this application.
I think we'll have to temporarily get a second computer in the room.
Thanks.

On Tue, 13 Jan 2004, gregor barclay wrote:

} Michael,
} Have you tried rearranging the cards on the Mobo? I had the same adventure

} when installing a Pixera camera and Scion system on an XP system. I did
not
} get the New Hardware Found announcement for the Pixera card until I did
some
} card swapping.
}
} Let me know how you get on.
}
} Greg
}
}
}
} Dr. G. F. Barclay
} Plant Science Unit, Dept of Life Sciences
} University of the West Indies
} St. Augustine, Trinidad and Tobago
} West Indies
} Phone: 868 645 3232 ext 3112/2045
} Fax: 868 645 7132
}
}
}
}
}
} } From: Michael Cammer {cammer-at-aecom.yu.edu}
} } To: microscopy-at-MSA.microscopy.com
} } Subject: [Microscopy] Sensicam QE & Roper HQ
} } Date: Mon, 12 Jan 2004 12:58:55 -0500
} }
} }
} }
}
} ---------------------------------------------------------------------------
---
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
} ---------------------------------------------------------------------------
----
} }
} } We are trying to install two cameras on a Windows XP computer.
} }
} } We cannot get XP to recognize both the Sensicam PCI card and the Roper
PCI
} } card. It's completely an exclsuive or installation. We've poked around
} } the Device driver menu and downloaded the most recent drivers.
} }
} } Has anybody figured out how to install both these camera simultaneously?
} }
} }
} }
} }
}
} ___________________________________________________________________________
_
} } Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of
} } Med.
} } Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY
10461
} } (718) 430-2890 Fax: 430-8996 URL:
http://www.aecom.yu.edu/aif/
} }
} }
}
} _________________________________________________________________
} Help STOP SPAM with the new MSN 8 and get 2 months FREE*
} http://join.msn.com/?page=features/junkmail
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 10:55:59 2004

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Mike Bode writes ...

} 3) If one card is not recorgnized, check if there are
} any conflicts in the device manager.

It's difficult for me to add anything to Mike's response, but to note that
many motherboards inherantly share resources amongst pairs of PCI slots.
For example, many mobos share the resources of AGP slot with the next PCI
slot. Another observation of note is that the Windows OS is designed for
sharing resources amongst slots such there should be no conflicts, but my
own experience is how well this works is highly dependent on the
manufacturer's software driver for the card.

Therefore, I'd suggest you may not yet have found the right combination of
slots, or that you beg the manufacturer(s) for their help.

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

} -----Original Message-----
} } From: Michael Cammer [mailto:cammer-at-aecom.yu.edu]
} Sent: Monday, January 12, 2004 20:34
} To: gregor barclay
} Cc: microscopy-at-MSA.microscopy.com
} Subject: [Microscopy] RE: Sensicam QE & Roper HQ
}
}
}
}
} ------------------------------------------------------------------
} ----------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ------------------------------------------------------------------
} ----------
} ---
}
} We swapped cards all over the place. The one in the lowest slot gets
} recognized, but not the other. Also, the Roper card doesn't seem to
} work in the highest slot, even alone. We could get either card to work
} with a firewire camera in another slot, but the Retiga we have isn't low
} noise enough for this application.
} I think we'll have to temporarily get a second computer in the room.
} Thanks.
}
} On Tue, 13 Jan 2004, gregor barclay wrote:
}
} } Michael,
} } Have you tried rearranging the cards on the Mobo? I had the
} same adventure
}
} } when installing a Pixera camera and Scion system on an XP system. I did
} not
} } get the New Hardware Found announcement for the Pixera card until I did
} some
} } card swapping.
} }
} } Let me know how you get on.
} }
} } Greg
} }
} }
} }
} } Dr. G. F. Barclay
} } Plant Science Unit, Dept of Life Sciences
} } University of the West Indies
} } St. Augustine, Trinidad and Tobago
} } West Indies
} } Phone: 868 645 3232 ext 3112/2045
} } Fax: 868 645 7132
} }
} }
} }
} }
} }
} } } From: Michael Cammer {cammer-at-aecom.yu.edu}
} } } To: microscopy-at-MSA.microscopy.com
} } } Subject: [Microscopy] Sensicam QE & Roper HQ
} } } Date: Mon, 12 Jan 2004 12:58:55 -0500
} } }
} } }
} } }
} }
} } -----------------------------------------------------------------
} ----------
} ---
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} } -----------------------------------------------------------------
} ----------
} ----
} } }
} } } We are trying to install two cameras on a Windows XP computer.
} } }
} } } We cannot get XP to recognize both the Sensicam PCI card and the Roper
} PCI
} } } card. It's completely an exclsuive or installation. We've
} poked around
} } } the Device driver menu and downloaded the most recent drivers.
} } }
} } } Has anybody figured out how to install both these camera
} simultaneously?
} } }
} } }
} } }
} } }
} }
} } _________________________________________________________________
__________
} _
} } } Michael Cammer Analytical Imaging Facility Albert Einstein
} Coll. of
} } } Med.
} } } Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY
} 10461
} } } (718) 430-2890 Fax: 430-8996 URL:
} http://www.aecom.yu.edu/aif/
} } }
} } }
} }
} } _________________________________________________________________
} } Help STOP SPAM with the new MSN 8 and get 2 months FREE*
} } http://join.msn.com/?page=features/junkmail
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 12:17:42 2004

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Dear Microscopists,

This discussion on fixation is interesting from a number of aspects. The
reliance on answers based on almost 10 year old literature and technology,
without consideration of current literature, technique and technology (PELCO
BioWave) is curious. In the last three years at the Microscopy and
Microanalysis meetings whole and half day sessions have been devoted to
microwave processing techniques using new and emerging technology. Current
experimental findings do not support the old literature especially when it
comes to fixation and microwave heating. If one chose to stay reasonably
current with both the new technology and techniques they would not propose
50C as an end point temperature for the fixative. I would direct those
curious to a recent paper in Ultrastructural Pathology (2003) 27:187-196,
Microwave and Digital Imaging Technology Reduce Turnaround Times for
Diagnostic Electron Microscopy and as well as Microwave Techniques and
Protocols (2001) from Humana Press, Totowa, NJ and chapter 16 in particular.
I have been around the microwave scene for over 10 years and have worked
diligently to improve the technology (the dreaded vendor) as well as the
science (proof side of the equation). I have difficulty with advice that is
10 years old and ignores recent developments.

Richard T. Giberson
Manager Research and Development
Ted Pella, Inc.

-----Original Message-----
} From: Steven E. Slap [mailto:siksik03-at-comcast.net]
Sent: Tuesday, January 13, 2004 5:28 AM
To: Richard Easingwood
Cc: microscopy-at-msa.microscopy.com

Dear fellow microscopists

Richard makes some good points here. I second
his reading recommendations, and want to let
everyone know that there is a brand new edition
of Kok and Boon, Microwaves for the Art of
Microscopy, Coulomb Press, Leiden, 2003, which
has some very useful new information.

I believe that the use of a dummy load is not
needed in the Biowave, which has a recirculating
water cooler. In any event, the end temperature
of 50°C is the key, and Richard's 3 x 7 minutes
should give Shannon a good starting point for
time in the fixative. I would be a little
concerned about using such a small volume of
fixative as Richard did (4.0 ml), both because of
a fear of exceeding the temperature set point and
because a greater volume of fixative to specimen
ratio seems prudent based upon my experience with
light microscopy specimens. I generally work
with about 11.0 ml of fixative.

best regards,
Steven Slap
Microwave Consultant

} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 18:13:26 2004

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Email: fremingt-at-fhcrc.org
Name: F.Remington

Organization: Fred Hutchinson Cancer Research Center

Title-Subject: [Microscopy] [Filtered] immuno scanning electron microscopy

Question:
We would appreciate some help if anyone has knowledge of or has used
a method for labelling tissue of cell walls-stomach or intestine-with
ICam-1 for immuno scanning E.M.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 13 18:14:05 2004

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Email: Leanne.Armand-at-csiro.au
Name: Leanne Armand

Organization: CSIRO-Marine

Title-Subject: [Microscopy] [Filtered] MListserver: Seeking Opinions- Image
Analysis Software

Question: Dear M-Listers,

We are interested in using image analysis software for several purposes:
1. to speed the process of counting and measuring of cells in unialgal cultures
2. to assist in counting cells in simple two species competition
experiments where they are relatively easy to separate by shape.
3. to develop the capacity to identify and count the dominant species
from natural samples

To this end we have been offered some software packages with an
epifluorescent inverted microscope. We would like to know if anyone
has any experience with these software packages trying to achieve
similar goals.

1. Image Pro Discovery (by Media Cybernetics)
2. Softimaging System (SIS) Auto version 3.2
4. Leica QWin Standard software
5. Axiovision 4 (Zeiss)
6. Digital Optics V++ Image analysis software

Comments on your experiences would be most welcome.

Many Thanks and All the best for the coming New Year
Leanne Armand and Peter Thompson

___________________________________________
*Contact Days - Tues., Wed., Fri.*
___________________________________________
Dr Leanne Armand
Joint Personal Assistant to Dr Peter Thompson
Sustainable Marine Ecosystems in the South East
CSIRO Marine Research
GPO Box 1538
Hobart, 7001
Tas. Australia

Ph (03) 6232 5085
Fax (03) 6232 5000

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 16:51:22 2004

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-------------------------------------------------------------------------

Email: cavinm-at-vsl.cua.edu
Name: Cavin Mooers

Organization: Vitreous State Lab

Title-Subject: [Microscopy] [Filtered] SEM: Minimum Vacuum for Tungsten Filament

Question: We are currently experiencing vacuum
issues which are causing tungsten oxide growth
and premature failure of the filament while
operating our JEOL 5900. One of the JEOL
technicians has suggested that 5x10-4 torr is
acceptable, but I find this hard to believe. The
issue we are dealing with is extraordinarily slow
pumping times -- 1 hour to obtain 3x10-5 torr and
a max vacuum of 5x10-6 torr after 3-4 hours. We
are a high volume lab, and so I wish to know what
the minimum vacuum I need without seriously
diminishing filament life, in order to maximize
the workload.

Sincerely,

Cavin T. F. Mooers
EM Facility Manager
Vitreous State Laboratory
The Catholic University of America
Hannan Hall ń Rm 433
Washington, D.C. 20064
(202) 319-6237 (Office)
(202) 319-5346 (Lab)
(202) 319-4469 (Fax)

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 16:52:13 2004

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Email: ann-at-northwestern.edu
Name: Ann Chiaramonti

Organization: Northwestern University

Title-Subject: [Microscopy] [Filtered] MListserver: Teaching samples for TEM

Question: Hi,
I am teaching a TEM lab class this quarter and am looking for a
material useful for teaching basic imaging and diffraction in the
TEM. We would like a material with lots of dislocations, stacking
faults, grain boundaries, etc. so that it is interesting for the
students. I would like to use stainless steel but do not have any
non-magnetic readily available.
I would like to avoid using perchloric acid if possible in the
preparation. Any suggestions/comments?
Thank you in advance,

Ann Chiaramonti
Northwestern University
ann-at-northwestern.edu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 17:06:26 2004

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Greetings:

What's the latest word on glow discharge for grids?

We have an old VE that will glow discharge, but have hardly ever used it.
A new faculty person wants to do more glow discharging and is looking for
info.

Somewhere I have a paper describing a home made glow discharge device,
anybody know about this and if it works?

Also have heard that keeping grids in the refrigerator helps too. What's up
with that?

Her application is carbon films for negatively stained macromolecules.

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 18:24:33 2004

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Dear Cavin,
It sounds like the problem is not just that you have a leak, but where the leak
is. The vacuum is usually tested at the top of the diffusion pump, but what
matters for the filament is the vacuum at the gun. If you have a small leak at
the gun, the vacuum near the filament may be quite a bit worse than you are
seeing. I routinely turn on the tungsten filament when the vacuum reads 1X10-4
torr, but I am sure that that vacuum is consistent in the column and that it
will rapidly improve.
I suggest you assume that the leak is near the gun and do some detective work.
You will be much happier, the filament will last longer and your throughput will
better.
Good luck,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "by way of MicroscopyListserver" {cavinm-at-vsl.cua.edu}
To: {microscopy-at-ns.microscopy.com}
Sent: Wednesday, January 14, 2004 2:56 PM

-------------------------------------------------------------------------

Email: cavinm-at-vsl.cua.edu
Name: Cavin Mooers

Organization: Vitreous State Lab

Title-Subject: [Microscopy] [Filtered] SEM: Minimum Vacuum for Tungsten Filament

Question: We are currently experiencing vacuum
issues which are causing tungsten oxide growth
and premature failure of the filament while
operating our JEOL 5900. One of the JEOL
technicians has suggested that 5x10-4 torr is
acceptable, but I find this hard to believe. The
issue we are dealing with is extraordinarily slow
pumping times -- 1 hour to obtain 3x10-5 torr and
a max vacuum of 5x10-6 torr after 3-4 hours. We
are a high volume lab, and so I wish to know what
the minimum vacuum I need without seriously
diminishing filament life, in order to maximize
the workload.

Sincerely,

Cavin T. F. Mooers
EM Facility Manager
Vitreous State Laboratory
The Catholic University of America
Hannan Hall ń Rm 433
Washington, D.C. 20064
(202) 319-6237 (Office)
(202) 319-5346 (Lab)
(202) 319-4469 (Fax)

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 18:26:16 2004

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Thanks to Richard Giberson for his comments. As Pelco is not represented in
this part of the world, I was unaware of this advance in microwave
technology and the new Pelco BioWave.

We have a national microscopy conference in February next year (see
http://ocem.otago.ac.nz/Conference_2005/Microscopy_NZ_2005.html) It would
be fantastic if Pelco would bring this technology out to demonstrate it to
us here during the conference!

Regards,

Richard

} Dear Microscopists,
}
} This discussion on fixation is interesting from a number of aspects. The
} reliance on answers based on almost 10 year old literature and technology,
} without consideration of current literature, technique and technology (PELCO
} BioWave) is curious. In the last three years at the Microscopy and
} Microanalysis meetings whole and half day sessions have been devoted to
} microwave processing techniques using new and emerging technology. Current
} experimental findings do not support the old literature especially when it
} comes to fixation and microwave heating. If one chose to stay reasonably
} current with both the new technology and techniques they would not propose
} 50C as an end point temperature for the fixative. I would direct those
} curious to a recent paper in Ultrastructural Pathology (2003) 27:187-196,
} Microwave and Digital Imaging Technology Reduce Turnaround Times for
} Diagnostic Electron Microscopy and as well as Microwave Techniques and
} Protocols (2001) from Humana Press, Totowa, NJ and chapter 16 in particular.
} I have been around the microwave scene for over 10 years and have worked
} diligently to improve the technology (the dreaded vendor) as well as the
} science (proof side of the equation). I have difficulty with advice that is
} 10 years old and ignores recent developments.
}
} Richard T. Giberson
} Manager Research and Development
} Ted Pella, Inc.
}
} -----Original Message-----
} } From: Steven E. Slap [mailto:siksik03-at-comcast.net]
} Sent: Tuesday, January 13, 2004 5:28 AM
} To: Richard Easingwood
} Cc: microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Re: microwave fixation procedure for insects
}
}
}

Richard Easingwood
Otago Centre for Electron Microscopy
Department of Anatomy and Structural Biology
School of Medical Sciences, University of Otago
PO Box 913, Dunedin, NEW ZEALAND
Telephone: 0064 3 479 7301
Facsimile: 0064 3 479 7254
GSM: 0064 21 222 4759
mailto:richard.easingwood-at-stonebow.otago.ac.nz
Web site: http://ocem.otago.ac.nz/

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 18:28:58 2004

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Dear Ann,
Brass, annealed or slightly deformed, is easy to thin in a high concentration
nitric acid in methanol electropolishing bath (see Van der Voort). It is
non-magnetic, has lots of twins, dislocations and an easy diffraction pattern.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "by way of MicroscopyListserver" {ann-at-northwestern.edu}
To: {microscopy-at-ns.microscopy.com}
Sent: Wednesday, January 14, 2004 2:57 PM

On Jan 13, 2004, at 5:49 AM, Richard Edelmann wrote:

} So now, anyone out there with a Microtek 2500f what is the part number
} and where do you get the bulbs from?
}
Dear Richard,
We have a different model and have yet to need a bulb replaced;
however, we purchased the unit from Calumet photo, and I recommend
talking to Chris Benes, (323)466-1238 x108,
chris.benes-at-calumetphoto.com. (This is in the Pacific Time Zone, so
plan accordingly.) Good luck, and please pass along what you learn.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 14 21:28:06 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Jonathan Krupp wrote:
====================================================
What's the latest word on glow discharge for grids?

We have an old VE that will glow discharge, but have hardly ever used it. A
new faculty person wants to do more glow discharging and is looking for info

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 08:04:18 2004

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Dear fellow microscopists

The Pelco BioWave is not the only new advance in microwave
technology. For something else really new, check out Milestone's REM
microwave for EM processing (http://www.milestonesrl.com). It has a
non-contact infra-red temperature sensor, full computer control by
touch screen and no need for a water load at all. This is another
microwave that you need to have at your conference. Maybe you can
get someone from Milestone (JIm Milius?) to present it.

best regards,
Steven Slap
Microwave Consultant

}
} Thanks to Richard Giberson for his comments. As Pelco is not represented in
} this part of the world, I was unaware of this advance in microwave
} technology and the new Pelco BioWave.
}
} We have a national microscopy conference in February next year (see
} http://ocem.otago.ac.nz/Conference_2005/Microscopy_NZ_2005.html) It would
} be fantastic if Pelco would bring this technology out to demonstrate it to
} us here during the conference!
}
} Regards,
}
}
} Richard
}
}
}
} } Dear Microscopists,
} }
} } This discussion on fixation is interesting from a number of aspects. The
} } reliance on answers based on almost 10 year old literature and technology,
} } without consideration of current literature, technique and technology (PELCO
} } BioWave) is curious. In the last three years at the Microscopy and
} } Microanalysis meetings whole and half day sessions have been devoted to
} } microwave processing techniques using new and emerging technology. Current
} } experimental findings do not support the old literature especially when it
} } comes to fixation and microwave heating. If one chose to stay reasonably
} } current with both the new technology and techniques they would not propose
} } 50C as an end point temperature for the fixative. I would direct those
} } curious to a recent paper in Ultrastructural Pathology (2003) 27:187-196,
} } Microwave and Digital Imaging Technology Reduce Turnaround Times for
} } Diagnostic Electron Microscopy and as well as Microwave Techniques and
} } Protocols (2001) from Humana Press, Totowa, NJ and chapter 16 in particular.
} } I have been around the microwave scene for over 10 years and have worked
} } diligently to improve the technology (the dreaded vendor) as well as the
} } science (proof side of the equation). I have difficulty with advice that is
} } 10 years old and ignores recent developments.
} }
} } Richard T. Giberson
} } Manager Research and Development
} } Ted Pella, Inc.
} }
} } -----Original Message-----
} } } From: Steven E. Slap [mailto:siksik03-at-comcast.net]
} } Sent: Tuesday, January 13, 2004 5:28 AM
} } To: Richard Easingwood
} } Cc: microscopy-at-msa.microscopy.com
} } Subject: [Microscopy] Re: microwave fixation procedure for insects
} }
} }
} }
}
} Richard Easingwood
} Otago Centre for Electron Microscopy
} Department of Anatomy and Structural Biology
} School of Medical Sciences, University of Otago
} PO Box 913, Dunedin, NEW ZEALAND
} Telephone: 0064 3 479 7301
} Facsimile: 0064 3 479 7254
} GSM: 0064 21 222 4759
} mailto:richard.easingwood-at-stonebow.otago.ac.nz
} Web site: http://ocem.otago.ac.nz/

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 08:54:58 2004

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Calvin:

Yes, 5x10-4 is a useable vacuum, but it will shorten fialment life. As
previously suggested you may have a vacuum leak in the gun (check the gun
chamber o-ring). But since you are getting down to 5x10-6 it doesn't sound
like a leak is the main problem. Becasue it takes so long to pump down,
sounds more like a pumping problem. Not exactly sure where your starting
from when you say it takes 1 hour to get 3 x10-5. I just vented my JEOL 840
gun and it took ~ 9 mins to get the same with a warmed and running pumping
system.

-- dirty or cracked DP oil or RP oil (Change oils)

-- poor DP backing (clean RP and replace RP exhaust filter).

-- low RP oil level or DP oil level.

-- check cooling temp on DP. (Too high *or* too low)

Good luck.

} Email: cavinm-at-vsl.cua.edu
} Name: Cavin Mooers
}
} Organization: Vitreous State Lab
}
} Title-Subject: [Microscopy] [Filtered] SEM: Minimum Vacuum for Tungsten Filament
}
} Question: We are currently experiencing vacuum
} issues which are causing tungsten oxide growth
} and premature failure of the filament while
} operating our JEOL 5900. One of the JEOL
} technicians has suggested that 5x10-4 torr is
} acceptable, but I find this hard to believe. The
} issue we are dealing with is extraordinarily slow
} pumping times -- 1 hour to obtain 3x10-5 torr and
} a max vacuum of 5x10-6 torr after 3-4 hours. We
} are a high volume lab, and so I wish to know what
} the minimum vacuum I need without seriously
} diminishing filament life, in order to maximize
} the workload.
}
} Sincerely,
}
} Cavin T. F. Mooers
} EM Facility Manager
} Vitreous State Laboratory
} The Catholic University of America
} Hannan Hall ń Rm 433
} Washington, D.C. 20064
} (202) 319-6237 (Office)
} (202) 319-5346 (Lab)
} (202) 319-4469 (Fax)
}
}
} ---------------------------------------------------------------------------
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 09:06:37 2004

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Cavin Mooers wrote:
}
} Question: We are currently experiencing vacuum
} issues which are causing tungsten oxide growth
} and premature failure of the filament while
} operating our JEOL 5900. One of the JEOL
} technicians has suggested that 5x10-4 torr is
} acceptable, but I find this hard to believe...

We have a JEOL JXA-8900 electron microprobe, and we never expose a hot
filament to pressures above 1x10-4 torr -- and that is only for a minute or
so during a sample change. When, on occasion, a user has exceeded this
pressure for a few seconds, our filament tends to break within a day or
two. I would consider a pressure of 1x10-5 torr to be minimally
acceptable, and we normally operate at about 2x10-6 torr. Once or twice
we've had vacuum problems, and it has been the fault of degraded rubber
gaskets causing leaks.

Ellery

---------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
Department of Geology & Geophysics
University of Minnesota - Twin Cities
Lab Website: http://probelab.geo.umn.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 11:05:01 2004

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I used to use a home-made glow-discharge device for grids and a lot more
besides. I can't find the paper so I'm afraid I can't give you the
reference, but I can tell you that the device is cheap and easy to make if
you have access to a workshop, and it does work very well. That's assuming
that you have the same paper that we used, of course. I never tried keeping
grids in the fridge, but before we had the GD thing I used to use an
anti-static pen from Ladd (I think - one of the usual suppliers, anyway) and
that certainly helped. Sorry to be so vague, but I'm at home.

Lesley Weston.

on 14/01/2004 3:06 PM, Jon Krupp at jmkrupp-at-cats.ucsc.edu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Greetings:
}
} What's the latest word on glow discharge for grids?
}
} We have an old VE that will glow discharge, but have hardly ever used it.
} A new faculty person wants to do more glow discharging and is looking for
} info.
}
} Somewhere I have a paper describing a home made glow discharge device,
} anybody know about this and if it works?
}
} Also have heard that keeping grids in the refrigerator helps too. What's up
} with that?
}
} Her application is carbon films for negatively stained macromolecules.
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 11:30:39 2004

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Hi Shannan
I have followed this theme with interest as we have used a Pelco
Microwave for about four years now. Protocols and equipment have
changed over that time and we have kept up with the changes. They
have certainly improved the timing it takes to either fluoresenctly
label cells for confocal (half an hour instead of 3 hours), or for EM
processing (two hours instead of three days). If it works
conventionally it is likely to work in the microwave. If it doesn't
work conventionally then it is unlikely to work in the microwave.
The results are certainly comparable and for confocal work, the cells
are fresher and there is generally less background.
Researchers can walk in the door at 9 am and go down to the confocal
at 9.30 with labelled cells.

Our protocols have changed somewhat over this time and we are
constantly finding better ways of doing things. Three things are
important in your microwave: 1: a cool spot. This cuts out the
standing waves and the need for load coolers and controls the
temperature together with the temperature probe. 2. a vacuum chamber,
especially for plant material or specimens with a cuticle such as C.
elegans and beetle larvae. 3. Power controller - keep the power below
200 watts and live specimens stay alive.

The present protocol below has been used successfully with a wide
variety of specimens (we are a multiuser facility for the faculty of
medicine and the faculty of science). You may need to tweak the
timings depending on how thick your samples are. You can easily check
the penetration by sacrificing one of the larvae after the osmium
step, though this is probably not a problem for SEM. Our TEM protocol
starts the same way but we use a Spurr-Epon mix for the resin. The
blocks cut better than using either Spurr's or Epon alone. You can of
course use your buffer of choice. Cacodylate buffer is our choice as
we get less chance of precipitates with UA and it is a lot cheaper
than PIPES or HEPES though they have their places too.

Microwave SEM processing for animal tissue

1. Fixation
Fix tissue in 2.5% Glutaraldhyde in 0.1M cacodylate buffer pH 7.3-7.4 at 22 C
Perform under Vacuum
Power level 1 (about 100W)
2 min on, 2 min off, 2 min on
Repeat without changing

2. Cacodylate buffer rinse at 22 C
Do not perform under Vacuum
Power level 2 (about 200W)
40 sec
Repeat three times
If using tannic acid with buffer, rinse in butter once without tannic
before continuing to osmium step.

3. Osmium Tetroxide Fixation at 22 C
1% osmium tetroxide in 0.1M cacodylate buffer
Perform under Vacuum
Power level 1 (about 100W)
2 min on, 2 min off, 2 min on
Repeat without changing

4. Distilled water rinse
Rinse sample in distilled water and change to new water
Do not perform under Vacuum
Power level 2 (about 200W)
40 sec

5. Dehydrate in ethanol at 22 C
50% ETOH
70% ETOH
90% or 95% ETOH
100% ETOH
100% ETOH
100% ETOH
Do not perform under Vacuum
Power level 2 (about 200W)
40 sec

6. Critical Point Dry step
either conventionally in a CPD or in the microwave with
Hexamethyldisilizane (HMDS) at 22 C

Do not perform under Vacuum
Power level 2 (about 200W)
40 sec
Replace with new HMDS
Repeat two more times

Place in 60C oven for 5 mins
Remove excess HMDS
Place back in 60C oven until HMDS has evaporated

No two specimens types are the same. You might have to double the
timings for the larvae depending on how difficult it is to penetrate
the cuticle and how big they are.

A great souce of what is new in the processing of specimens is Rick
Giberson of Pelco. He is working with a number of labs on improving
the technique. I have no doubt that the above is already out of
date, but it usually works for us, so if it ain't broke, don't fix it
eh!

We have been investigating the use of formaldehyde in the microwave.
I had a coop student look at the effect of the microwave on fixation
over 30 mins, 2 hours and 72 hours. The first results have given us
more questions. Hopefully we will be able to present a paper on this
in the future.

Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 11:34:21 2004

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HI.
I would like to know how to measure the size of lattice of very local places
in the HRTEM image (not real lattice dimensions, just the size between any
lattice planes).
The images are two two dimensional (nearly structural images), and the
structure is relative simple, composed of two or three different atoms.
Probably slightly tilting affects the measurement, but I want to know the
size of each one or several lattice layers from the interface. I also want
to know the lattice size of very local places (~10 x ~10 lattices). I think
that some programs may find the lowest or highest contrast (1 pixel) on
digital images, although I am not sure if the idea is correct. Please advise
about some papers or programs. I prefer a free software.

Thank you,

Hiromi Konishi
The University of New Mexico

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 11:53:57 2004

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Ellery Frahm wrote:

} ... we never expose a hot filament to
} pressures above 1x10-4 torr -- and that is
} only for a minute or so during a sample change.

Michael O'Keefe wrote:

} Never = "only for a minute or so"........
} Is that a new definition of "never"?
}
} Mike

Hi Mike,

Let me clarify:

We never deliberately expose a hot filament to pressures above 1x10-4 torr.
We normally operate at about 2x10-6 torr. Only during a sample change
will we reach pressures that *approach* 1x10-4 torr for a minute or so,
often less. I tell our users never to exceed 1x10-4 torr, but sometimes a
user is careless or distracted and will reach higher pressures for a few
seconds, greatly reducing our filament life -- it usually "dies" in a day
or two.

Sorry for the confusion -- I wasn't trying to re-define "never" :)

Ellery

---------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
Department of Geology & Geophysics
University of Minnesota - Twin Cities
Lab Website: http://probelab.geo.umn.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 11:57:40 2004

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The paper describing a home made glow-discharge device is
authored by Aebi and Pollard, J Electron Microsc Tech. 1987 Sep; 7(1): 29-33.
We made a similar one (a bit simpler) which we routinely
use to charge grids prior to picking up sections and
also prior to negative staining. It can probably be
made for less than $150.00. I'd be happy to send a .jpg
image of the device to anyone who wants it.

Doug

On Wed, 14 Jan 2004 15:06:29 -0800 Jon Krupp
{jmkrupp-at-cats.ucsc.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver On-Line
} Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Greetings:
}
} What's the latest word on glow discharge for grids?
}
} We have an old VE that will glow discharge, but have hardly
} ever used it. A new faculty person wants to do more glow
} discharging and is looking for info.
}
} Somewhere I have a paper describing a home made glow
} discharge device, anybody know about this and if it works?
}
} Also have heard that keeping grids in the refrigerator
} helps too. What's up with that?
}
} Her application is carbon films for negatively stained
} macromolecules.
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu
}
}
}

----------------------
Douglas R. Keene
Associate Investigator
Micro-Imaging Center
Shriners Hospital for Children
3101 S.W. Sam Jackson Park Road
Portland, Oregon 97239-3009
phone: 503-221-3434
FAX: 503-412-6894

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 12:23:05 2004

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On Jan 15, 2004, at 9:39 AM, Hiromi Konishi wrote:

} I would like to know how to measure the size of lattice of very local
} places
} in the HRTEM image (not real lattice dimensions, just the size between
} any
} lattice planes).
} The images are two two dimensional (nearly structural images), and the
} structure is relative simple, composed of two or three different atoms.
} Probably slightly tilting affects the measurement, but I want to know
} the
} size of each one or several lattice layers from the interface. I also
} want
} to know the lattice size of very local places (~10 x ~10 lattices). I
} think
} that some programs may find the lowest or highest contrast (1 pixel)
} on
} digital images, although I am not sure if the idea is correct. Please
} advise
} about some papers or programs. I prefer a free software.
}
Dear Hiromi,
I would first calibrate the microscope magnification using a
Mag*I*Cal--no affiliation except satisfied user--then record the images
on film, print enlargements, scan, and measure the areas of interest.
This avoids at least some of the aliasing that can come from digital
imaging. If you take digital images, you have to be sure that Nyquist
frequency, equal to twice the pixel dimension, is larger than the
spacing you are trying to determine; i.e., the lattice layers must span
several pixels. If you know that all the layers have the same spacing,
you can measure the spacing between layer 1 and layer N, but your post
indicates that you are trying to measure the difference in spacing of
layers near an interface--a much more difficult problem. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 14:33:28 2004

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Our venerable JEOL 840A valves over to the diffusion pump about 3 minutes
after we start pumping the chamber. 45 seconds later, the high voltage was
re-enabled at a vacuum of 5x10-5 torr measured at the gun. At 30 minutes,
vacuum had reached 1x10-5 torr. At 60 minutes, the vacuum was about 2x10-6.
I think we get down into the high 10-7 range if we leave the scope
overnight. (FYI, it takes less than 60 seconds for us to pump down just the
gun chamber when we vent it and leave the sample chamber under vacuum. I
don't know your model of JEOL. It may not have a valve to isolate the gun
from the sample chamber.)

It definitely sounds like a leak or a pumping problem. I would defer to the
other posters and their suggestions on those subjects.

You did not say what kind of samples you are examining, or whether samples
are loaded when you are having trouble reaching vacuum. I know that can be
a problem. We tried to examine concrete in our 840A and it took forever to
pump down. We did a bit better by limiting sample volume, but it was still
slow. Oily samples can be a problem depending on the vapor pressure of the
liquid.

You were not clear whether your scope is under service contract or not. If
it is, I would suggest you take advantage of the contract. Something is not
right. If you can't find the problem quickly, I would let the boys earn
their keep. I might assume this is a scope you purchased directly from
JEOL, but that might not be the case. Did the scope used to work right in
your lab and this is a new problem, or is this a matter of trying to get a
scope up and running right for the first time?

Good luck and keep the questions coming.
Warren

At 09:00 AM 1/15/2004, Richard Edelmann wrote:

} Calvin:
}
} Yes, 5x10-4 is a useable vacuum, but it will shorten fialment
} life. As
} previously suggested you may have a vacuum leak in the gun (check the gun
} chamber o-ring). But since you are getting down to 5x10-6 it doesn't sound
} like a leak is the main problem. Becasue it takes so long to pump down,
} sounds more like a pumping problem. Not exactly sure where your starting
} from when you say it takes 1 hour to get 3 x10-5. I just vented my JEOL 840
} gun and it took ~ 9 mins to get the same with a warmed and running pumping
} system.
}
} -- dirty or cracked DP oil or RP oil (Change oils)
}
} -- poor DP backing (clean RP and replace RP exhaust filter).
}
} -- low RP oil level or DP oil level.
}
} -- check cooling temp on DP. (Too high *or* too low)
}
}
} Good luck.
}
} } Email: cavinm-at-vsl.cua.edu
} } Name: Cavin Mooers
} }
} } Organization: Vitreous State Lab
} }
} } Title-Subject: [Microscopy] [Filtered] SEM: Minimum Vacuum for
} Tungsten Filament
} }
} } Question: We are currently experiencing vacuum
} } issues which are causing tungsten oxide growth
} } and premature failure of the filament while
} } operating our JEOL 5900. One of the JEOL
} } technicians has suggested that 5x10-4 torr is
} } acceptable, but I find this hard to believe. The
} } issue we are dealing with is extraordinarily slow
} } pumping times -- 1 hour to obtain 3x10-5 torr and
} } a max vacuum of 5x10-6 torr after 3-4 hours. We
} } are a high volume lab, and so I wish to know what
} } the minimum vacuum I need without seriously
} } diminishing filament life, in order to maximize
} } the workload.
} }
} } Sincerely,
} }
} } Cavin T. F. Mooers
} } ---------------------------------------------------------------------------
}
} Richard E. Edelmann, Ph.D.
} Electron Microscopy Facility Supervisor
} 350 Pearson Hall
} Miami University, Oxford, OH 45056
} Ph: 513.529.5712 Fax: 513.529.4243
} E-mail: edelmare-at-muohio.edu

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 16:22:31 2004

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Micromavens,

Does anybody know of a current supplier of (preferably small lots) of
Sylguard (Dow-Corning)? I've been searching the web, but don't find
any suppliers.
Sylguard as used for potting electronics, the clear stuff (although
clear isn't required right now). A mold-release compound for this
would be nice, too.
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 17:00:42 2004

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Hiromi,
If you have access to a Macintosh Version of Gatan's DigitalMicrograph,
you can download from the NCEM web site a powerful plug-in written by Roar
Kilaas and Martin Hytch. Using this plug-in, you can measure the local
change in lattice parameter from an image. The program does a lot more and
is very easy to use. See the link below:

http://ncem.lbl.gov/frames/software.htm
*********************
A new set of routines for creating digital Moire patterns, displacement maps
and strain images can be downloaded by clicking on the link below. These
routines use the concept of the geometric phase to calculate deviations in
local lattice parameters from variations in reciprocal space around chosen
spatial frequencies (Bragg reflections). On-line help on the routines is
available from the menu-bar.

Download Phase-Extension routines.

PhaseManual.pdf

Last updated May 1999.

Users of this package are encouraged to email comments (email: roar-at-lbl.gov)
on the software.
********************

Cheers, Ray

Ray D. Twesten, PhD.
Center for Microanalysis of Materials
Seitz Materials Research Laboratory
104 S. Goodwin Ave., Urbana, IL 61801
+1 217 244-6177 (Fax -2278)

-----Original Message-----
} From: Hiromi Konishi [mailto:konishi-at-geofourpeaks.com]
Sent: Thursday, January 15, 2004 11:40 AM
To: microscopy-at-ns.microscopy.com

HI.
I would like to know how to measure the size of lattice of very local places
in the HRTEM image (not real lattice dimensions, just the size between any
lattice planes).
The images are two two dimensional (nearly structural images), and the
structure is relative simple, composed of two or three different atoms.
Probably slightly tilting affects the measurement, but I want to know the
size of each one or several lattice layers from the interface. I also want
to know the lattice size of very local places (~10 x ~10 lattices). I think
that some programs may find the lowest or highest contrast (1 pixel) on
digital images, although I am not sure if the idea is correct. Please advise
about some papers or programs. I prefer a free software.

Thank you,

Hiromi Konishi
The University of New Mexico

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 17:30:30 2004

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Jonathan Krupp wrote:
====================================================
What's the latest word on glow discharge for grids?

We have an old VE that will glow discharge, but have hardly ever used
it. A new faculty person wants to do more glow discharging and is
looking for info.

Somewhere I have a paper describing a home made glow discharge device,
anybody know about this and if it works?

Also have heard that keeping grids in the refrigerator helps too. What's
up with that?

Her application is carbon films for negatively stained macromolecules.
=======================================================
Usually the reason why one would want to glow discharge treat their
(carbon coated) grids is to make them more hydrophilic. The technique
we use is to expose the carbon coated grids to a nitrogen (e.g. air)
plasma for roughly 5-10 seconds in one of our standard configured Plasma
Prep II plasma etcher units. Such a treatment will keep the carbon
coatings hydrophilic for roughly 30 days (or more). More information
can be found on URL
http://www.2spi.com/catalog/instruments/etchers1.shtml

This is a low power unit and I don't know how well it might work for
systems putting out more than 100 watts. I have never heard of
storage under refrigeration to slow down the loss in hydrophilic
character of carbon coated grids.

Disclaimer: SPI Supplies manufactures carbon coated grids for customers
and also manufactures the SPI Plasma Prep™ II plasma etcher.

Chuck
===========================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 19:23:22 2004

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A medium 10-6 torr in one hour sounds reasonable for diffusion pump powered
scope. There are two things to consider:
- it may be a leak (perhaps some O-ring);
- it may be pumps (backing or diffusion).

If there is a leak, you need to isolate somehow (depends from the model)
the suspected compartment and measure the leak speed - JEOL guys would tell
you what is the normal for your particular microscope.

The pumps tend to lost their "power" with time if you don't do a
prophylactic. The oil ether in mechanical or diffusion pump should be
changed from time to time. It's more critical for mechanical pump, because
it has moving parts. It's good idea to change oil in mechanical pump at
least ones in a year. You also should keep in mind the possibility of
backstreaming from mechanical pump, if so, diffusion pump may be
affected. If diffusion pump operates in normal condition (not exposed to
air when hot, not much water pumped down etc) the oil may stay good for
years. Still, you need to maintain the level of oil according to the
specification. If you did not manage to look inside of DP for decade, it's
probably time to do so. Look for dark deposits and oil's color. If your DP
has been operated in good conditions, you, perhaps will not find any dark
deposits and oil will be from yellow to light dark (you lucky guy). So,
because you already opened DP, you may need to replace oil for the next few
years. If your DP is contaminated by deposits and oil is dark - it's time
to do good cleaning. Disassemble everything and clean. Everything inside
the DP should be shiny polished -the warranty, it will thankfully works
good for the next decade! Return everything back and check leak speed
again. Personally, I prefer to use Santovac-5 DP oil. It's expensive but
it delivers wonderful results and it's very stable. In my DV502A vacuum
evaporator, it stays for 10 years and I only adjust level from time to
time. It delivers good 10-6 in about 1-2 hours and goes into 10-7
overnight. It's on the "dirty" system. Sergey

At 12:38 PM 1/15/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 20:39:22 2004

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Jonathan Krupp wrote:

What's the latest word on glow discharge for grids?

Another way to make coated grids more hydrophilic is to expose them to UV
light. I know of one lab that stored Formvar-coated grids on racks under a
UV light (did not specify wavelength), and used the oldest ones first. I
personally just make grids on a dry day and let them age naturally -
probably enough UV here to do the job.

But more specifically, a student here at UH tried a lot of different
methods of treating her grids, and found that if she put them in their
Stratolinker UV Crosslinker (for crosslinking DNA), set it for 30 sec, and
pushed the Auto button, it worked great! I looked it up - it uses 254
nm. I have not yet tried any of our UV sources around here, but it would
be worth trying everything from a party blacklight to a zap with the
confocal. Or even a turn on the front porch (weather permitting).

Aloha,
Tina

Yesterday - rainy, gale force winds
Today - 78F, sunny, surf's up

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 23:50:24 2004

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Email: m.kral-at-mech.canterbury.ac.nz
Name: Milo Kral

Organization: University of Canterbury

Title-Subject: [Microscopy] [Filtered] Desktop Microscopist

Question: I am trying to reach Jim Stanley so I can ask him how to
use DM on Mac OS10.

Could Jim, or someone who knows him, tell me how to get in touch?

Regards
Milo

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 15 23:49:51 2004

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Email: gt5185d-at-prism.gatech.edu
Name: Jonathan B.

Organization: Georgia Tech

Title-Subject: [Microscopy] [Filtered] MListserver: SEM analysis of skin tissue...

Question: Hello Microscopy group,

I was hoping to garnish some advice about SEM sample preparation for
my PhD research. I'm investigating a technology to microporate human
skin for transdermal drug delivery, and I want to image the pores
with a SEM. My current plan is to purchase an automated critical
point dryer; currently I'm considering Emitech's 850 and Polaron's
7501. I hope I'm on the right track.

Any comments? Thanks,
Jonathan B.

My biological samples are engineered living tissue 22mm in diameter
and 1mm thick. I'll be using a Hitachi 3500H, with a CVC Products DC
Sputterer at the Georgia Tech MiRC cleanroom.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 08:22:01 2004

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I don't bother with neutralization or anything; I just collect it in a
jug and hand it over to Rutgers Environmental Health & Safety when they
come to pick up hazardous waste.

Kathleen Roberts
Principal Lab Technician
Neurotoxicology Labs
Dept of Pharmacology and Toxicology
Ernest Mario School of Pharmacy
Rutgers University

Barbara Murray wrote:

} Greetings,
} We have been using a solidifier for our formalin, putting it into biohazard boxes for pickup by the housekeeping dept. We were told by our Safety Officer that we can now pour it down the drain with lots of running water.
} For the ones of you who are using formalin, how are you disposing of it?
} Thanks for your replies. Have a great day and weekend!
}
} Barbara A. Murray,HT.(ASCP)
} The Alaska Native Medical Center
} Anchorage, Alaska
}
}
} _______________________________________________
} Histonet mailing list
} Histonet-at-lists.utsouthwestern.edu
} http://lists.utsouthwestern.edu/mailman/listinfo/histonet
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 09:00:59 2004

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Picking up on the thread on disposal of formalin, I have a comment plus a
question. My comment is that many Environmental Health & Safety
departments pick up "hazardous waste" and then pour it down the drain with
lots of water. This includes low level radioisotopes. At my university,
we (lab personnel) can not call anything hazardous waste. We can only have
"unwanted used materials". We can not use the word waste on any label. We
had a box labeled "glass waste" on our microtome bench for our old glass
knives and slides and were cited!

Recently we were told they were going to a policy of users disposing uranyl
acetate ( {1%) by pouring it down the drain with lots of water. I was a
little surprised by this. Do other universities follow this policy?

Thanks, Tom

At 09:33 AM 1/16/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 10:17:29 2004

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We are not allowed to throw anything down the sink--including water wash
from stains and alcohol! The MWRA (Massachusetts Water Resource Assoc.) has
very strict guidelines re: mercury, etc. entering Boston Harbor. As we are
a pathology lab for a research group, we do a lot of staining, so all washes
must be collected in a large container and it is then picked up by an
outside waste management company on a weekely basis. This waste is analyzed
for mercury levels. You would be surprised the number of chemicals that
contain mercury. All our other waste (i.e. formalin, EM fixes, etc.) are
collected in containers and picked up weekly as well. I'm surprised that,
being in Alaska, where there have been problems with major spills in the
waters, that they allow formalin to go down the drain. Are you allowed to
throw other chemicals down as well?

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
Sent: Friday, January 16, 2004 9:34 AM
To: Barbara Murray; Microscopy-at-sparc5.microscopy.com

I don't bother with neutralization or anything; I just collect it in a
jug and hand it over to Rutgers Environmental Health & Safety when they
come to pick up hazardous waste.

Kathleen Roberts
Principal Lab Technician
Neurotoxicology Labs
Dept of Pharmacology and Toxicology
Ernest Mario School of Pharmacy
Rutgers University

Barbara Murray wrote:

} Greetings,
} We have been using a solidifier for our formalin, putting it into
biohazard boxes for pickup by the housekeeping dept. We were told by our
Safety Officer that we can now pour it down the drain with lots of running
water.
} For the ones of you who are using formalin, how are you disposing of it?
} Thanks for your replies. Have a great day and weekend!
}
} Barbara A. Murray,HT.(ASCP)
} The Alaska Native Medical Center
} Anchorage, Alaska
}
}
} _______________________________________________
} Histonet mailing list
} Histonet-at-lists.utsouthwestern.edu
} http://lists.utsouthwestern.edu/mailman/listinfo/histonet
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 10:27:19 2004

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Tom,

I refer you to my general email that I just sent to the group--we cannot
throw anything down the sink. But, especially, uranly acetate, which has a
low level of radioactivity. This is picked up by the radiation safety dept.
I believe they are just storing it until decisions are made as to what waste
site it can be shipped.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Tom Phillips [mailto:phillipst-at-missouri.edu]
Sent: Friday, January 16, 2004 10:06 AM
To: Microscopy-at-msa.microscopy.com

Picking up on the thread on disposal of formalin, I have a comment plus a
question. My comment is that many Environmental Health & Safety
departments pick up "hazardous waste" and then pour it down the drain with
lots of water. This includes low level radioisotopes. At my university,
we (lab personnel) can not call anything hazardous waste. We can only have
"unwanted used materials". We can not use the word waste on any label. We
had a box labeled "glass waste" on our microtome bench for our old glass
knives and slides and were cited!

Recently we were told they were going to a policy of users disposing uranyl
acetate ( {1%) by pouring it down the drain with lots of water. I was a
little surprised by this. Do other universities follow this policy?

Thanks, Tom

At 09:33 AM 1/16/2004 -0500, you wrote:

} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 10:40:33 2004

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We would like to prepare sperm for examination under EM of cross sections of
the tail to investigate integrity of the cilia, and I have never done this
before. Does anyone have a good simple method that would give a good
result?

Garry Burgess
Charge Technologist
Health Sciences Centre
Winnipeg, Canada

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 12:22:01 2004

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Gary,
I just finished doing a sperm prep. I had the investigator pellet
them (very gently to minimize head-tail separation) and fix the
resultant pellet in my "standard" EM fix (2.5% glut, 4% pfa, 0.02%
picric acid [good for membranes] in 0.1M Na-cacodylate). I processed
the pellet as usual with an osmium postifx, ethanol dehydrations and
i embedded in Spurr's. Very straight forward and we got some lovely
images. You do need to hunt around for good cross sections, but
there are usually so many sperm in the pellet its not too hard.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 12:59:24 2004

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} We would like to prepare sperm for examination under EM of cross sections of
} the tail to investigate integrity of the cilia, and I have never done this
} before. Does anyone have a good simple method that would give a good
} result?
}
} Garry Burgess
} Charge Technologist
} Health Sciences Centre
} Winnipeg, Canada
Garry,
I have worked with marine animal sperm in the past. An important
piece of information was that we used artificial sea water as the
carrier for the glutaraldehyde instead of a buffer and as the wash
after that. The best pelleted samples were obtained if the tubes were
centrifuged as soon as possible after the primary fixative was added
to the tube.
If the pellet falls apart, centrifuge during each change of solution.
At the time, the top speed of a table top centrifuge was used but a
microfuge should work better. Care should be taken that the pellet is
not thick.
Acetone (Mallinckrodt #2440) was chosen over ethanol because we were
interested in the cytoskeletin and membranes, and wanted to remove a
lot of background substances.

Procedure:
1% glutaraldehyde in sea water [1 part 8% glut from Electron
Microscopy Sciences + 7 parts sea water], room temp. 30 min.
sea water rinse
1% osmium tetroxide in 0.1 M phosphate buffer, on ice + dark, 30 min.
Cold Water rinse X3, 5 min. each
1% UA in water, refrigerator, overnight
Acetone dehydration - 50% to 100% X2, 15 min. each
Propylene Oxide X2, 15 min. each
1:1::Prop.Ox.:Epon 30 min.
Epon 30 min.
Embed in Epon and polymerize.

All times may be extended except the osmium fixation, especially if
actin is of importance.

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 13:27:34 2004

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On Fri, 16 Jan 2004, Garber, Charles A. wrote:

} Any idea how long the effect lasts? For us it seemed like the effect did
} not last very long at all. But then again, maybe we did not study the
} phenomenon to the extent you did.

A very good question. I know they are using their grids immediately. The
people who kept their grids on racks under a UV light left the light on
all the time, and used the grids soon after taking them out.

Another client of ours has used bacitracin and protein A (not together) to
help his viruses stick and to increase wettability of Formvar coated grids
with great success. He is no longer here, so I don't have his protocols.

When in desparation (a chronic state around here) I have tried a number of
techniques for making coated grids more hydrophilic. The more successful
ones include dipping a grid in 70-80% ethanol, shaking off the excess, and
then using the grid just as the fluid appears to dry, and I have used a
very dilute solution of PhotoFlo, which worked surprisingly well for the
application at hand and did not leave a visible residue. I have not yet
been desparate enough to try spit!

Caroline Schooley, when at Berkeley, used to have a homemade (I
think) Tesla coil kind of thing that she applied to the outside (I
think) of the bell jar of a vacuum evaporator. I don't remember well
because I was terrified of the thing and usually ran out of the room. I
was very young.

In general, however, I coat a lot of grids on our rare dry day, then keep
them in covered Petri dishes. For Formvar-coated grids, I like them best
at about 2 years old, and for carbon films at 6 months or more. I don't
know why the become more hydrophilic as they age, and I'm guessing it's
some kind of contamination, but I haven't seen anything weird, and they
work well for me.

This is all to keep from having to repair my vacuum evaporator, of
course, but glow discharge is probably the most reliable. My new sputter
coater works, however. Chuck, how about plasma mode? What does that do?

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 14:56:43 2004

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Nope, uranyl acetate is treated as radioactive waste here. I don't know
what they do with it after it leaves here, however.

Kathleen Roberts
Rutgers University

Tom Phillips wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Picking up on the thread on disposal of formalin, I have a comment
} plus a question. My comment is that many Environmental Health &
} Safety departments pick up "hazardous waste" and then pour it down the
} drain with lots of water. This includes low level radioisotopes. At
} my university, we (lab personnel) can not call anything hazardous
} waste. We can only have "unwanted used materials". We can not use
} the word waste on any label. We had a box labeled "glass waste" on
} our microtome bench for our old glass knives and slides and were cited!
}
} Recently we were told they were going to a policy of users disposing
} uranyl acetate ( {1%) by pouring it down the drain with lots of water.
} I was a little surprised by this. Do other universities follow this
} policy?
}
} Thanks, Tom
}
}
}
}
} At 09:33 AM 1/16/2004 -0500, you wrote:
}
}
}
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } I don't bother with neutralization or anything; I just collect it in
} } a jug and hand it over to Rutgers Environmental Health & Safety when
} } they come to pick up hazardous waste.
} }
} } Kathleen Roberts
} } Principal Lab Technician
} } Neurotoxicology Labs
} } Dept of Pharmacology and Toxicology
} } Ernest Mario School of Pharmacy
} } Rutgers University
} }
} } Barbara Murray wrote:
} }
} } } Greetings,
} } } We have been using a solidifier for our formalin, putting it into
} } } biohazard boxes for pickup by the housekeeping dept. We were told
} } } by our Safety Officer that we can now pour it down the drain with
} } } lots of running water. For the ones of you who are using formalin,
} } } how are you disposing of it?
} } } Thanks for your replies. Have a great day and weekend!
} } }
} } } Barbara A. Murray,HT.(ASCP)
} } } The Alaska Native Medical Center
} } } Anchorage, Alaska
} } }
} } }
} } } _______________________________________________
} } } Histonet mailing list
} } } Histonet-at-lists.utsouthwestern.edu
} } } http://lists.utsouthwestern.edu/mailman/listinfo/histonet
} } }
} }
} }
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 16:01:28 2004

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Tina Carvalho wrote about glow discharge:
}
} Caroline Schooley, when at Berkeley, used to have a homemade (I
} think) Tesla coil kind of thing that she applied to the outside (I
} think) of the bell jar of a vacuum evaporator. I don't remember well
} because I was terrified of the thing and usually ran out of the room. I
} was very young.

Before someone yells at me, let me correct Tina's memory. I used a
physics demonstration-type Tesla coil in firm contact (to avoid ozone
production in the room) with a current feedthrough that led from
below the baseplate into the bell jar. Ran the discharge during the
rough pump part of the automatic pumpdown cycle, about a minute,
until the purple glow inside the bell jar faded. Worked fine; I used
it for years.

Young and terrified? By then you could completely rebuild a
Volkswagen, Tina....!
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 16:33:57 2004

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The regulations here have changed many times for UA disposal. It
went to sink, then to Chemical waste, then it was too hot for them,
so it was to go to Radiation safety, but it was not hot enough...
Right now I have given up and have an old, covered, tri-pour beaker
in the corner of my hood with a combination of evaporated UA and
uranyl phosphate (UA+PO4 Buffer)!
Maybe I'll have them put it into my coffin when my time comes!

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

} Nope, uranyl acetate is treated as radioactive waste here. I don't
} know what they do with it after it leaves here, however.
}
} Kathleen Roberts
} Rutgers University
}
} } Picking up on the thread on disposal of formalin, I have a comment
} } plus a question. My comment is that many Environmental Health &
} } Safety departments pick up "hazardous waste" and then pour it down
} } the drain with lots of water. This includes low level
} } radioisotopes. At my university, we (lab personnel) can not call
} } anything hazardous waste. We can only have "unwanted used
} } materials". We can not use the word waste on any label. We had a
} } box labeled "glass waste" on our microtome bench for our old glass
} } knives and slides and were cited!
} }
} } Recently we were told they were going to a policy of users
} } disposing uranyl acetate ( {1%) by pouring it down the drain with
} } lots of water. I was a little surprised by this. Do other
} } universities follow this policy?
} }
} } Thomas E. Phillips, PhD
} } Professor of Biological Sciences
} } Director, Molecular Cytology Core
} } 3 Tucker Hall
} } University of Missouri
} } Columbia, MO 65211-7400
} } 573-882-4712 (office)
} } 573-882-0123 (fax)
PhillipsT-at-missouri.edu

} } } I don't bother with neutralization or anything; I just collect it
} } } in a jug and hand it over to Rutgers Environmental Health & Safety
} } } when they come to pick up hazardous waste.
} } }
} } } Kathleen Roberts
} } } Principal Lab Technician
} } } Neurotoxicology Labs
} } } Dept of Pharmacology and Toxicology
} } } Ernest Mario School of Pharmacy
} } } Rutgers University
} } }
} } } Barbara Murray wrote:
} } }
} } } } Greetings,
} } } } We have been using a solidifier for our formalin, putting it into
} } } } biohazard boxes for pickup by the housekeeping dept. We were
} } } } told by our Safety Officer that we can now pour it down the drain
} } } } with lots of running water. For the ones of you who are using
} } } } formalin, how are you disposing of it?
} } } } Thanks for your replies. Have a great day and weekend!
} } } }
} } } } Barbara A. Murray,HT.(ASCP)
} } } } The Alaska Native Medical Center
} } } } Anchorage, Alaska
} } } } _______________________________________________
} } } } Histonet mailing list
} } } } Histonet-at-lists.utsouthwestern.edu
} } http://lists.utsouthwestern.edu/mailman/listinfo/histonet

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 18:31:28 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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Email: echeung-at-eyetk.com
Name: Eunice Cheung

Organization: Eyetech

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Has anyone had success with using nanogold labeling in
whole-mount preparations? What did you use to improve contrast of
cellular structure without using osium tetraoxide?

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 16 18:37:42 2004

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On Jan 16, 2004, at 7:06 AM, Tom Phillips wrote:

} Recently we were told they were going to a policy of users disposing
} uranyl acetate ( {1%) by pouring it down the drain with lots of water.
} I was a little surprised by this. Do other universities follow this
} policy?
}
Dear Tom,
There are different laws in different states, so where you live
determines what is possible. Within those limits, your safety office
may impose more stringent conditions. Disposal of low-level
radioactive waste--oops, spent materials--is expensive, so many
institutions allow only the least costly option.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 17 19:01:42 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday,
January 17, 2004 at 11:26:01
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Email: gbarclay-at-fans.uwi.tt
Name: Greg Barclay

Organization: University of the West Indies

Education: Graduate College

Location: St. Augustine, Trinidad, West Indies

Question: Permount is what we have been using forever and we are now
looking for a slide mountant that dries faster. I would appreciate
any suggestions.

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From MicroscopyL-request-at-ns.microscopy.com Sun Jan 18 19:49:07 2004

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Hello all:

I am considering trying to budget for an
Osmium-based specimen coater to augment (not replace)
my Denton Desk II Au/Pd and Pt coater. There
are some specimens that are going to be taken
at high mag (250KX-450KX) and should not show
coating artifacts (major or minor). The Os
coater looks like a good option. Cr is out
due to short life span based on rapid oxidation.
Is the same true for Os?

I would appreciate feedback from Os coater users
and suppliers. Off-list of course.

tnx,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 18 23:03:46 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Gary Gaugler wrote:
=======================================================
I am considering trying to budget for an Osmium-based specimen coater to
augment (not replace) my Denton Desk II Au/Pd and Pt coater. There are some
specimens that are going to be taken at high mag (250KX-450KX) and should
not show coating artifacts (major or minor). The Os coater looks like a
good option. Cr is out due to short life span based on rapid oxidation. Is
the same true for Os?

I would appreciate feedback from Os coater users and suppliers. Off-list of
course.
=========================================================
Osmium is a precious group metal and therefore it has essentially the
intertness of gold, platinum, etc. It is a pretty permanent coating, and
could be expected to have a life time comparable to what one would expect
for gold.

We are often times asked if there is any danger that it could convert to the
tetroxide (and then sublime and disappear). From a practical standpoint,
absolutely not. Of course, if you exposed the coating to a strong oxidizer,
perhaps sodium iodide, the metallic osmium could be oxidized back up to the
dioxide and then the tetroxide and then there would be a dangerous condition
but most of us don't expose our coated SEM samples to strong oxidizers......

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 18 23:26:04 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Gary Gaugler wrote:
=======================================================
I am considering trying to budget for an Osmium-based specimen coater to
augment (not replace) my Denton Desk II Au/Pd and Pt coater. There are some
specimens that are going to be taken at high mag (250KX-450KX) and should
not show coating artifacts (major or minor). The Os coater looks like a
good option. Cr is out due to short life span based on rapid oxidation. Is
the same true for Os?

I would appreciate feedback from Os coater users and suppliers. Off-list of
course.
=========================================================
Osmium is a precious group metal and therefore it has essentially the
intertness of gold, platinum, etc. It is a pretty permanent coating, and
could be expected to have a life time comparable to what one would expect
for gold.

We are often times asked if there is any danger that it could convert to the
tetroxide (and then sublime and disappear). From a practical standpoint,
absolutely not. Of course, if you exposed the coating to a strong oxidizer,
perhaps sodium iodide, the metallic osmium could be oxidized back up to the
dioxide and then the tetroxide and then there would be a dangerous condition
but most of us don't expose our coated SEM samples to strong oxidizers!

Chuck

============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Sun Jan 18 23:54:39 2004

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Hello all,
We are currently working with a student who is interested in corals and
possible virus associations within them. Fo course, problems arise when
trying to process and section the samples, which contain both normal
soft biological tissue and the hard calcified material. Could anyone
please suggest a method to decalcify them without doing too much damage
to the ultrastructure? Should a decalcification step be done on fresh or
fixed tissue? The samples we have to work with now are fixed. Any
suggestions would be appreciated.
Thanks.

Lyn Waterhouse
Adelaide Microscopy
University of Adelaide
Adelaide SA 5005
Ph: (08) 8303 4074 or 8303 5855
Fax: (08) 8303 4356
http://www.adelaide.edu.au/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 01:22:17 2004

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hello,

The best decalcifier to use on biological samples is actually a chelating
agent; EDTA ethylene-diaminetetracetic acid. It does not act like a normal
acid but binds metallic ions, especially calcium and magnesium. It works
better at at pH 7-8 and can be used as an aqueous solution or mixed with
formaldehyde.It takes longer than the usual decalcifiers such as acids but
the results are very good. Dense cortical bone takes about 6-8 weeks to
decalcify. If you have x-ray facilities you can monitor the process well.
Decalcification must be done on well fixed material otherwise the
decalcifier will macerate the biological matter, particularly the nucleic
acids.

Regards,
Evelyn Kaplan,
Dept of Pathology,
College of Medicine and Health Sciences,
Sultan Qaboos University,
Oman

-----Original Message-----
} From: Lyn Waterhouse [mailto:lyn.waterhouse-at-adelaide.edu.au]
Sent: Monday, January 19, 2004 10:03 AM
To: Microscopy-at-MSA.Microscopy.Com

Hello all,
We are currently working with a student who is interested in corals and
possible virus associations within them. Fo course, problems arise when
trying to process and section the samples, which contain both normal
soft biological tissue and the hard calcified material. Could anyone
please suggest a method to decalcify them without doing too much damage
to the ultrastructure? Should a decalcification step be done on fresh or
fixed tissue? The samples we have to work with now are fixed. Any
suggestions would be appreciated.
Thanks.

Lyn Waterhouse
Adelaide Microscopy
University of Adelaide
Adelaide SA 5005
Ph: (08) 8303 4074 or 8303 5855
Fax: (08) 8303 4356
http://www.adelaide.edu.au/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 02:21:36 2004

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Eunice,

Marc Moeremans, who recently joined us, was one of the scientists
involved in the development of the Nanovid microscopy technique at
Janssen Pharmaceutics (Beerse, Belgium), which involved immunogold staining.

I forward your question to him, maybe he can help ?

Best regards,

Peter Van Osta

Union Biometrica N.V./S.A.
European Scientific Operations (ESO)
Cipalstraat 3
B-2440 Geel
Belgium
Tel.: +32 (0)14 570 620
Fax.: +32 (0)14 570 621

http://www.unionbio-eu.com/

http://ourworld.compuserve.com/homepages/pvosta/cvwww.htm

===========================================
by way of Nestor J. Zaluzec wrote:

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} submitted by (echeung-at-eyetk.com) from
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} Friday, January 16, 2004 at 13:40:06
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} Email: echeung-at-eyetk.com
} Name: Eunice Cheung
}
} Organization: Eyetech
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: Has anyone had success with using nanogold labeling in
} whole-mount preparations? What did you use to improve contrast of
} cellular structure without using osium tetraoxide?
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 05:15:26 2004

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Dear Eunice,

Wonderful results on pre-embedding labeling vibratome sections of brain
tissue have been described by Yi et al., (2001) J. Histochem. Cytochem.
49(3), 279-283. F(ab')2 and single Fab fragments coupled to ultra-small
gold particles were used to immunolabel different intra cellular
antigens. The detection of MGP-160, a golgi marker localized within the
lumen demonstrates the potential of these ultra-small gold conjugates.
Hong Yi uses osmium tetroxide to reveal morphological detail. She uses
osmium after silver enhancing the ultra-small gold particles.

Similar protocols are used for whole mount preparations. A few examples:
Briane et al; (2002) J. Histochem. Cytochem. 50(7), 983-991
Verbeek et al; (2002) J. Histochem. Cytochem. 50(5), 681-690.

More pre-embedding labeling protocols you can find in Aurion newsletter
nr.5
Please contact me in case you need additional technical information.

Kind regards,

Peter

On Saturday, January 17, 2004, at 01:36 AM, by way of Nestor J. Zaluzec
wrote:

}
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} America
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} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (echeung-at-eyetk.com) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Friday, January 16, 2004 at 13:40:06
} -----------------------------------------------------------------------
} ----
}
} Email: echeung-at-eyetk.com
} Name: Eunice Cheung
}
} Organization: Eyetech
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: Has anyone had success with using nanogold labeling in
} whole-mount preparations? What did you use to improve contrast of
} cellular structure without using osium tetraoxide?
}
} -----------------------------------------------------------------------
} ----
}
}
}
-----------
Peter van de Plas
Aurion
Costerweg 5
6702 AA Wageningen
The Netherlands
Phone: +31 317 497676
Fax: +31 317 415955

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 07:01:46 2004

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One and all,

I have been given two samples and asked to determine if they are concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

-----------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 07:27:39 2004

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It seems to me.....
Sandstone is an agglomeration of chiefly quartz in a matrix of carbonates
and iron oxides. Concrete can have sand and small rocks or pebbles, but
the assuming the concrete has reacted or set, it should be loaded with a
variety of high refractive index (greater than 1.660 - which tells you
where I got my training) particles. It the material is not cured or set
up, you should be able to find high refractive index particles of calcium
oxide which isn't found in sandstone.

Best wishes..............

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 08:05:00 2004

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Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

To
Microscopy-at-msa.microscopy.com
cc

Subject
SEM/LM of concrete vs. sandstone

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One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

-----------------------------------------
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reader of this message is not the intended recipient or an agent
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review, dissemination, distribution, or copying of this message is
strictly prohibited. If you have received this communication in error,
please notify us immediately, and delete the original message.

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 09:10:26 2004

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You raise questions on some of the perplexing results from this job. While
I am well aware of the heterogeneous nature of the samples, a summary of
the "bulk" analysis results yielded (approx.):
Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also present.
Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also present.

A small piece from each sample was sanded through 320 grit paper to get a
fresh, flat surface for the EDS analyses.

Now, neither sample is known to be concrete nor sandstone. Neither sample
contains any aggregate material. The discrete particles present in the
light gray sample are more populous and twice the size of the particles in
the red material. There is no color banding in either sample, which could
be indicative of the stratified layers in a sandstone.

I may be making this harder than it has to be, but I am suspecting that
neither sample is sandstone.

ekomarnicki-at-MacDe
rmid.com To: holpc-at-firstenergycorp.com
cc: Microscopy-at-msa.microscopy.com
01/19/2004 09:13 Subject: [Microscopy] Re: SEM/LM of concrete vs.
AM sandstone

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Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

To
Microscopy-at-msa.microscopy.com
cc

Subject
SEM/LM of concrete vs. sandstone

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

-----------------------------------------
The information contained in this message is intended only for the
personal and confidential use of the recipient(s) named above. If the
reader of this message is not the intended recipient or an agent
responsible for delivering it to the intended recipient, you are hereby
notified that you have received this document in error and that any
review, dissemination, distribution, or copying of this message is
strictly prohibited. If you have received this communication in error,
please notify us immediately, and delete the original message.

-----------------------------------------
The information contained in this message is intended only for the personal and confidential use of the recipient(s) named above. If the reader of this message is not the intended recipient or an agent responsible for delivering it to the intended recipient, you are hereby notified that you have received this document in error and that any review, dissemination, distribution, or copying of this message is strictly prohibited. If you have received this communication in error, please notify us immediately, and delete the original message.

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 09:33:16 2004

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Ed and Chris,

The difference between sandstones and concretes is usually fairly
obvious in a polished thin section viewed under plain and crossed
polars. The Atlas of sedimentary rocks under the microscope (Adams,
MacKenzie and Guilford, 1984, Longmans) gives examples of the commonest
types of sedimentary rock.
A sandstone is composed of two components the clasts (sand/rock) and the
cement (sorry that is the term the geologists use). Either of these
components may contain calcium bearing minerals, so the simple presence
of a signficiant calcium peak in an EDX spectra may not necessarily
prove that the material is a concrete. However, the cement of concrete
will not normally show visible crystallinity in the optical microscope
whereas many sandstones will. It also allows you to identify the clasts
and their size so distinguish between mortar and concrete (if samples is
large enough to include representative clasts).

ekomarnicki-at-MacDermid.com wrote:

}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Chris, I'm not a geologist or a cement expert, but concrete and mortar
} have cement as part of their make-up (ingredient). So you probably should
} start out comparing sandstone and cement. Commonly, concrete is cement
} with crushed stones (aggregates) in it. You don't mention having EDS at
} your disposal. Having EDS spectra obtained on your sample, I would expect
} higher Si concentration in the sandstone. and higher Ca conc. in the
} cement. Drop/spots tests may not reveal conc. differences. You may also
} want to run standards (i. e. Portland Cement, etc.) with your samples for
} positive confimation. Or even call a cement company and find out how they
} analyze their products. Hope this helps.
}
} The Materials Handbook, 13th ed. has some basic (starting) info on all
} three materials. ED
}
} Ed Komarnicki
} Sr. Analytical Chemist
} MacDermid Inc.
}
}
}
}
}
} holpc-at-firstenergycorp.com
} 01/19/04 08:09 AM
}
} To
} Microscopy-at-msa.microscopy.com
} cc
}
} Subject
} SEM/LM of concrete vs. sandstone
}
}
}
}
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
} One and all,
}
} I have been given two samples and asked to determine if they are
} concrete,
} sandstone, or some mix. One sample is light gray, and I suspect may be
} mortar rather than concrete. The other sample has a slight rust/red hue
} and
} contains appreciably more calcium. Both samples contain silica, and both
} test positive for calcium carbonate by the acid drop test, with the light
} gray sample showing a yellow residue from this test.
}
} Hours of reading test procedures for Portland cement and concrete, coupled
} with internet searches have left me wondering if I can draw a conclusion
} based on a few grams of sample. I would appreciate any suggestions about
} what to read or how to make this kind of determination.
}
} Thanks,
}
} Chris Holp
} FirstEnergy Corp.
} Beta Labs
} HolpC-at-firstenergycorp.com
}
}
}
} -----------------------------------------
} The information contained in this message is intended only for the
} personal and confidential use of the recipient(s) named above. If the
} reader of this message is not the intended recipient or an agent
} responsible for delivering it to the intended recipient, you are hereby
} notified that you have received this document in error and that any
} review, dissemination, distribution, or copying of this message is
} strictly prohibited. If you have received this communication in error,
} please notify us immediately, and delete the original message.
}
}
}
}
}
}

--
Chris Salter,
Oxford Materials Characterisation Service,
Oxford University Begbroke Science Park,
Sandy Lane, Yarnton, Oxford, OX5 1PF
Tel 01865 283722, EPMA 283741, Mobile 07776031608

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 10:05:44 2004

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"Now, neither sample is known to be concrete nor sandstone. ..." Well
that doesn't narrow it down any. According to my limited resource; cement
would have } 3x more Ca than Si; and in sandstone the ratio of Si to Ca is
expected to be much greater than double (what you have). I would guess
that neither sample is sandstone.

Perhaps a geologist could guide you further. ED

holpc-at-firstenergycorp.com
01/19/04 10:18 AM

To
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cc
Microscopy-at-msa.microscopy.com
Subject
Re: Re: SEM/LM of concrete vs. sandstone

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You raise questions on some of the perplexing results from this job. While
I am well aware of the heterogeneous nature of the samples, a summary of
the "bulk" analysis results yielded (approx.):
Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also present.
Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also
present.

A small piece from each sample was sanded through 320 grit paper to get a
fresh, flat surface for the EDS analyses.

Now, neither sample is known to be concrete nor sandstone. Neither sample
contains any aggregate material. The discrete particles present in the
light gray sample are more populous and twice the size of the particles
in
the red material. There is no color banding in either sample, which could
be indicative of the stratified layers in a sandstone.

I may be making this harder than it has to be, but I am suspecting that
neither sample is sandstone.

ekomarnicki-at-MacDe
rmid.com To: holpc-at-firstenergycorp.com
cc: Microscopy-at-msa.microscopy.com
01/19/2004 09:13 Subject: [Microscopy] Re: SEM/LM of concrete
vs.
AM sandstone

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Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

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Subject
SEM/LM of concrete vs. sandstone

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One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

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From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 12:21:16 2004

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you are all probably getting a virus from me. it is spreading through
scripps. don't open it. delete it.

have a nice day!

gary

Gary S. Laevsky, Ph.D.
Research Associate
The Scripps Research Institute
10550 N. Torrey Pines Road/IMM-24
La Jolla, CA 92037
(858) 784-9372

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Dear Microscopists

EDTA decalcification can be carried out on well-fixed specimens,
including corals, in a laboratory (tempreature-controlled) microwave
in a fraction of the time needed on the bench at room temperature.
Stirring during the process is important to keep fresh decalcifying
agent at the specimen at all times.

best regards,
Steven Slap

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 15:23:41 2004

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Two questions:
1. I was looking up the density of glycerol on the web and several sites gave it as 1.26 and several as 1.476. I had presumed the higher number but what is the other referring to?
2. In making a Mowiol mounting media as described in previous posts, I noted that the final glycerol concentration is only about 20% which is much lower than I am used to doing and seems a poor match in refractive index for oil. Does the Mowiol raise the refractive index to nearer the desired level? Thanks-Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 19 15:49:51 2004

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JEOL vacuum systems are normally set to allow the filament to be turned
on at 5X10-4 torr but, I personally don't recommend turning the gun on
at this point, unless you are in a real hurry to get something done.
Waiting 10-15 minutes after achieving a vacuum ready condition should
get you in the high 10-5 torr range which would be more acceptable and
extend filament life. Running at poor vacuum will also contaminate your
column and apertures sooner which may contribute to your down time.

Taking several hours to get to 5X10-6 torr is pretty normal. Using a
nitrogen back fill and a LN trap on the DP might help speed things up.

Good Luck,
Bill

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Email: cavinm-at-vsl.cua.edu
Name: Cavin Mooers

Organization: Vitreous State Lab

Title-Subject: [Microscopy] [Filtered] SEM: Minimum Vacuum for Tungsten
Filament

Question: We are currently experiencing vacuum
issues which are causing tungsten oxide growth
and premature failure of the filament while
operating our JEOL 5900. One of the JEOL
technicians has suggested that 5x10-4 torr is
acceptable, but I find this hard to believe. The
issue we are dealing with is extraordinarily slow
pumping times -- 1 hour to obtain 3x10-5 torr and
a max vacuum of 5x10-6 torr after 3-4 hours. We
are a high volume lab, and so I wish to know what
the minimum vacuum I need without seriously
diminishing filament life, in order to maximize
the workload.

Sincerely,

Cavin T. F. Mooers
EM Facility Manager
Vitreous State Laboratory
The Catholic University of America
Hannan Hall ń Rm 433
Washington, D.C. 20064
(202) 319-6237 (Office)
(202) 319-5346 (Lab)
(202) 319-4469 (Fax)

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Thanks for the reply.

No, I had not considered Ir. My basic problem is
that I am getting more specimens that have Pt, W,
Ta, Si, O, N, Mo, and C (not necessarily all of these
elements at the same time!). A typical problem is
a Au/Pd coated specimen that has large or small amounts
of Pt. Sputter coating with Pt would not be smart,
so I use Au/Pd. However, the Pt, when trace or thin,
is right next to Au Z-wise. And my 50-70A Au/Pd coating
shows up about the height in EDS as does the Pt.

The EDAX Genesis "knows" that it is there via the HPD
sanity check. I was thinking of using Os to get further
Z distance from the Pt and also from W. The pile up
convolution is at the M alpha series for Pt and Au.
This can be overcome by increasing KV to 20KV rather
than the 10-15KV I usually use. But the specimens
sometimes don't like the higher KV and volumetric
interaction also can be an issue. So I figured that
if I could keep in the M alpha region and put more
Z distance between elements, that would be a good move.

I looked at the Emitech you suggested. It is a monster
unit! All I need is a small desktop unit for pin stubs.
That drew me to the Os unit. But, are you indicating that
Os coated specimens will oxidize similar to Cr coating?
Not good. perhaps there is no one good answer.

gary g.

At 12:31 PM 1/19/2004, you wrote:
} Gary: have you considered Iridium coating? Ir is a noble metal so no
} oxidation
} will happen. It's also less worrisome than Os tetroxide if you're not used to
} using it. One of my labs uses it and has found no noticeable artifacts at
} 500KX
} SEM. They use Ir foil in an ion-beam sputtering unit and also have an Ir
} target in
} an Emitech sputter coater (http://www.empdirect.com/k675.html). I think
} Ted Pella
} also has an Ir option.
}
} Gary Gaugler wrote:
}
} } --
} }
} } Hello all:
} }
} } I am considering trying to budget for an
} } Osmium-based specimen coater to augment (not replace)
} } my Denton Desk II Au/Pd and Pt coater. There
} } are some specimens that are going to be taken
} } at high mag (250KX-450KX) and should not show
} } coating artifacts (major or minor). The Os
} } coater looks like a good option. Cr is out
} } due to short life span based on rapid oxidation.
} } Is the same true for Os?
} }
} } I would appreciate feedback from Os coater users
} } and suppliers. Off-list of course.
} }
} } tnx,
} } gary g.
}
} --
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} Becky Holdford (r-holdford-at-ti.com)
} 972-995-2360
} 972-648-8743 (pager)
} SC Packaging FA Development
} Texas Instruments, Inc.
} Dallas, TX
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

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Hi,
I would like to stain Biofilm polysaccharide on human
specimens with Ruthenium red. How should I get my
specimens ready for SEM? dehydration process before or
after the stain? 0.05% Ruthenium red in gluteraldehyde
or Formalin? what should I expect to look for under
SEM? any interferences or false positives with human
substances? Appreciate any input. Thanks, Jose

__________________________________
Do you Yahoo!?
Yahoo! Hotjobs: Enter the "Signing Bonus" Sweepstakes
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Dear Colleague,

Formatex, a Spanish Research Center, in association with Kluwer Academic
Publishers, is now preparing the Second number of the Formatex Microscopy
book series, with the preliminary title of "Current Issues in
Multidisciplinary Microscopy Research and Education". You can see the
contents of the first number published in 2003 in
http://www.formatex.org/micro2002/callforpaper.htm

Website of the 2004 edition is
http://www.formatex.org/micro2003/callforpaper2.htm

This second number of the series is committed to giving an overview of the
state of the art as well as upcoming trends, and to promoting discussion
about scientific, technological and educational aspects of Microscopy in
both the biological/biomedical and physical/chemical sciences. Although all
types of papers are a priori accepted (research articles, reviews, case
studies, etc.), priority will be given to those which clearly emphasize the
scientific/technological/pedagogical results, as well as those making
comparative discussions of two or more microscopy techniques or showing the
complementarity of microscopy techniques with other techniques. For this
second number, "educationally-oriented" and mini-review papers are
specially welcome, although also "regular" research papers are accepted.

If you are interested in participating in this edition submitting a
(technical, scientific, educational, introductory...) chapter related to
microscopy, please see the website for details.

As you may see from the Call for Papers' website, the deadline for chapter
submission is MARCH 15TH. Early submission of a short abstract of your
chapter proposal is appreciated in order to allow potencial authors to know
what other authors will write about for the book and avoid contents
duplications.

We hope that you find this new approach to microscopy issues interesting
and we hope to hear from you/your team for this and/or future editions.

If you any enquiry or suggestion about this volume, please contact us.

Best wishes from Spain.

José Antonio Mesa Gonzalez
Editorial Assistant
Formatex Research Center
C / Encarnacion, 3 1şE
06001 Badajoz
SPAIN
Phone/Fax: +34 924258615
Email: micro-at-formatex.org

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 02:10:27 2004

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Hello:

Many month ago I have asked for advise regarding a problem with
LaB6 filament. Well, finally we decided to switch for W filament.
So, the W filament is working in vacuum proper for LaB6 one (ion
pump). Now is almost one year (maybe 10 month) and still is working.

Talking about LaB6 problem, during this time we have been observing
behaviour of our microscope and it seems that the problem with LaB6
was caused be emergancy shut down of high voltage which was caused
probably by wrong signal from dirty Penning gauge. This shut
down caused a deposition of a layer (prabably LaB6) on the outside
surface of Whenelt cup and this was our problem.

Best regards,

Witold Zielinski

* Date sent: Mon, 19 Jan 2004 16:58:11 -0500
*From: William J Mushock {wim5-at-lehigh.edu}
*Organization: Lehigh University
*To: microscopy-at-ns.microscopy.com
*Subject: [Microscopy] viaWWW: SEM: Minimum Vacuum for Tungsten Filament

*
*
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Witold Zielinski, Ph.D.
Warsaw University of Technology
Department of Materials Science and Engineering
02-507 Warszawa, Woloska 141
POLAND

phone #: /48 22/ 660 87 07
660 87 36
fax #: /48 22/ 848 48 75

email: wiziel-at-inmat.pw.edu.pl

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 05:09:59 2004

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Chris Holp write ...

} I have been given two samples and asked to determine
} if they are concrete, sandstone, or some mix.
} One sample is light gray, and I suspect may be
} mortar rather than concrete. The other sample has a slight
} rust/red hue and contains appreciably more calcium.
} ...

Natural and sedimentary sandstone is likely to run a gamut in composition of
clasts and cement (the glue between the grains). One the other hand, I
should think concrete would be predominantly calcium sulphate (Portland
Cement), but containing clasts from a natural source.

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 08:05:49 2004

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Dear all,

I not been working with TEM diffraction or image simulations programs for a
few years now and am wondering what programs are now available and widely
used. I do not know which operating system I will be using for the
analysis, so any advice will be appreciated.

Thank you for your help.
Amy

Amy R. Ross
Los Alamos National Laboratory

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 09:44:12 2004

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I stand corrected! ... {g} ...

} -----Original Message-----
} From: Chris Salter
} Sent: Tuesday, January 20, 2004 11:11 AM
} To: michael shaffer
}
} No. The mechanism the setting of hydraulic cements (those based on
} Portland cement) have nothing to do with Calicum Sulphate. They work on
} the hydration of CaAlSilicates - fine tubules grow out from each cement
} grain and mesh with those from surrounding grains to give the initial
} set, thereafter various other chemical changes occur strengthen the
} bonds. The aluminium is essential for thise mechanism to work.
} Plasters work by the mechanism you are thinking of, but
} plaster is far
} weaker than cement or lime mortarand plaster is water soluble.
}
} } Thanx for the clarification ... but isn't the primary process for the
} } hardening of cement the cystallization of CaSO4, i.e.:
} }
} } CaSO4 (powder) + water =} CaSO4(H2O)n (??)
} }
} } cheerios ... shAf :o)
} } Avalon Peninsula, Newfoundland
} } www.micro-investigations.com
} }
} }
} }
} }
}
}
} --
} Chris Salter,
} Oxford Materials Characterisation Service,
} Oxford University Begbroke Science Park,
} Sandy Lane, Yarnton, Oxford, OX5 1PF
} Tel 01865 283722, EPMA 283741, Mobile 07776031608
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 10:28:34 2004

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Hi all,

We are just in the process of buying a FEG-SEM and have been tempted
by the vendors to add a STEM-detector to use for TEM imaging of normal
tissue sections up to around 40 - 50 kX. This would mean that we could
skip our old (17 years) TEM, which would save us money and trouble.
I would be very happy for some input from the list on a few issues
around this.
Is it a good idea to replace a 'proper' TEM with a STEM-detector? What
are the limitations with such a setup?
The FEG-SEM will run at max 30kV, which will obviously put a limitation
to the resolution, but the images we have seen (of our own samples) do
not seem to suffer as much as we had expected. Indeed, one of the
companies even did the test images at 10 kV, saying that it was the
'best' setting for that kind of images. How is the imaging actually
done?

thanks for any views,
Stefan
+++++++++++++++++++++++++++++++++++++++++++++++++++++++
Dr Stefan Gunnarsson
Evolutionsbiologiskt Centrum Evolutionary Biology Centre
Enheten för biologisk strukturanalys Microscopy and Imaging Unit
Norbyvägen 18A
SE75236 Uppsala, Sweden Tel & Fax: +46 - 18471 2638
+++++++++++++++++++++++++++++++++++++++++++++++++++++++

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 11:31:14 2004

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Stefan,

I am also very interested in the development of this area and seeking to
broaden my knowledge. I believe there are some interesting opportunities
for SEM-Based STEM in biological applications. However, the utility is yet
to be proven (at least I am not aware of a large number of results). So, I
would strongly suggest you obtain results on your samples. I don't believe
you can say the 30kV SEM-based STEM will replace a quality cryo TEM. But I
believe there are some interesting possibilities that need to be explored.

Currently, biological EM imaging does not present challenges in terms of
resolution, but rather in terms of contrast and beam induced damage. A low
voltage SEM-based STEM image will provide relatively high contrast due to
the low voltage. I am aware of some very promising results on biological
materials that even challenge zero loss imaging in terms of contrast. A
sufficiently high angle STEM will also eliminate diffaction contrast, which
is more ideal for tomographic applications (may not be an issue for your
samples).

STEM mode on a SEM-based STEM also provides the best resolution mode on the
tool. You should be able to achieve subnanometer resolution. The effect of
beam broadening, etc., on your particular sample may degrade that ideal
performance specification.

The question remaining (to me) is what exactly can be achieved with a 30kV
system and what is the beam damage? I assume you'd have a cryo transfer
type system. Again, I believe the best option is to see some results on
your samples.

I'd be very intersted in your final assessment. Good luck.

Regards,
Ed

----- Original Message -----
} From: "Stefan Gunnarsson" {Stefan.Gunnarsson-at-ebc.uu.se}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Tuesday, January 20, 2004 8:38 AM

Chris-

Based on your chemical data neither sample looks like a sandstone to me. A
sandstone typically contains a lot of quartz (SiO2), and also contains
other minerals such as feldspar, calcite, pyrite and clay minerals. I
would expect a lot more aluminum to combine with the Ca and Si to make
feldspar and/or clay minerals. Calcite (CaCO3) is a typical mineral that
binds the particles in a sandstone (we geologists call this a "cement") and
I do not see any Carbon in either analysis. Can you detect carbon with
your instrument or not?

Another method you can use to determine the mineralogy of your samples is
XRD (X-ray Diffraction). Yes, this is what I do but you need to use the
right tool for the job. It does not matter to me if you use me or another
lab. XRD will help you get the answer a lot quicker and with a lot more
certainty.

Contact me off list if you have any questions.

Sincerely,
James Talbot

K/T GeoServices, Inc.
Bulk and Clay Mineralogy by X-ray Diffraction
www.ktgeo.com
(940) 597-9076

At 10:18 AM 1/19/04 -0500, you wrote:

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You can find distributors for Dow Corning products on
their website.
http://www.dowcorning.com

Choose youre product and that page will have an option to
search for local suppliers. We use Sylgard 184 to make
dissecting surfaces for biological samples.

On Thu, 15 Jan 2004 16:27:37 -0600
Philip Oshel {peoshel-at-wisc.edu} wrote:
}
}
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} Society of America

Larry Ackerman
Keck Advanced Microscopy Lab
Dept. of Biochemistry & Biophysics
University of California San Francisco
600-16th Street, Room S101, Box 2140
San Francisco, CA 94158 (for postal mail use 94143)

415-476-4441 FAX 415-514-4142

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 16:18:39 2004

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I agree with James Talbot's opinion that X-ray diffraction would probably
give a definitive answer quite quickly. I think you might be able to get a
pretty good idea by taking spot analyses or an x-ray map of your two
samples. (It is what I do - on concrete.) Concrete or mortar is such a
heterogeneous mess that I would not get much out of an overall analysis.
However, if I can probe the cement paste and find Ca and Si and O, I can
suppose it to be Portland cement. There might also be unreacted cement
grains. You should also find substantial amounts of fine aggregate (i.e.,
sand) used to make the mortar. Those could be of most any composition, and
often are. I see calcite, quartz, feldspars and more. Because cement and
concrete are such hodge-podge mixtures, I often choose to do an x-ray map
rather than to probe every point in the image by hand.

But back to x-ray diffraction, even if you can get chemistry from the SEM,
you may still want to use XRD for a more definitive answer about the phases
present. I use an SEM to solve a lot of problems, but it has its
limitations. There is no substitute for diffraction or thermal analysis or
FTIR if the samples require it.

Warren

At 09:18 AM 1/19/2004, you wrote:

} You raise questions on some of the perplexing results from this job. While
} I am well aware of the heterogeneous nature of the samples, a summary of
} the "bulk" analysis results yielded (approx.):
} Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also present.
} Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also present.
}
} A small piece from each sample was sanded through 320 grit paper to get a
} fresh, flat surface for the EDS analyses.
}
} Now, neither sample is known to be concrete nor sandstone. Neither sample
} contains any aggregate material. The discrete particles present in the
} light gray sample are more populous and twice the size of the particles in
} the red material. There is no color banding in either sample, which could
} be indicative of the stratified layers in a sandstone.
}
} I may be making this harder than it has to be, but I am suspecting that
} neither sample is sandstone.

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

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"Now, neither sample is known to be concrete nor sandstone. ..." Well
that doesn't narrow it down any. According to my limited resource; cement
would have } 3x more Ca than Si; and in sandstone the ratio of Si to Ca is
expected to be much greater than double (what you have). I would guess
that neither sample is sandstone.

Perhaps a geologist could guide you further. ED

holpc-at-firstenergycorp.com
01/19/04 10:18 AM

To
ekomarnicki-at-MacDermid.com
cc
Microscopy-at-msa.microscopy.com
Subject
Re: Re: SEM/LM of concrete vs. sandstone

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You raise questions on some of the perplexing results from this job. While
I am well aware of the heterogeneous nature of the samples, a summary of
the "bulk" analysis results yielded (approx.):
Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also present.
Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also
present.

A small piece from each sample was sanded through 320 grit paper to get a
fresh, flat surface for the EDS analyses.

Now, neither sample is known to be concrete nor sandstone. Neither sample
contains any aggregate material. The discrete particles present in the
light gray sample are more populous and twice the size of the particles
in
the red material. There is no color banding in either sample, which could
be indicative of the stratified layers in a sandstone.

I may be making this harder than it has to be, but I am suspecting that
neither sample is sandstone.

ekomarnicki-at-MacDe
rmid.com To: holpc-at-firstenergycorp.com
cc: Microscopy-at-msa.microscopy.com
01/19/2004 09:13 Subject: [Microscopy] Re: SEM/LM of concrete
vs.
AM sandstone

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Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

To
Microscopy-at-msa.microscopy.com
cc

Subject
SEM/LM of concrete vs. sandstone

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

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From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 19:19:47 2004

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------------------------------------------------------------------------

Email: hitesh.jain-at-brocku.ca
Name: Hitesh Jain

Organization: Brock University

Title-Subject: [Microscopy] [Filtered] Applications for a wide
field of view confocal microscope

Question: Hello All,

We are assessing applications for a new type of
confocal microscope. The microscope is like a
confocal scanning laser microscope, but with ten
times the field of view (at the same resolution).

The instrument can be used to image large
samples, with a field of view of 1cm at submicron
resolution. The instrument can be used in room
light and can be highly automated. One of the
applications for this microscope is to image
tissue samples. In this application, some
advantages include:

Images entire biopsy specimens in a single scan (no tiling)
Fast scanning ń scans 10mmX10mm -at- 2 micron in 2 minutes
Simultaneous acquisition of 2-fluorophores
Scan area is 70mm x 22mm

We are compiling a list of potential applications
for this technology (in any sector). Can you
think of any specific applications for this
technology where the large field of view and
submicron resolution would be of particular use?

Thank you very much for your time and help,
Best wishes

Hitesh Jain, B.Sc., M.F.C
Senior Research Analyst
VISTA - The Canadian Centre for Science and Technology Solutions
Brock University

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You raise questions on some of the perplexing results from this job. While
I am well aware of the heterogeneous nature of the samples, a summary of
the "bulk" analysis results yielded (approx.):
Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also present.
Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also present.

A small piece from each sample was sanded through 320 grit paper to get a
fresh, flat surface for the EDS analyses.

Now, neither sample is known to be concrete nor sandstone. Neither sample
contains any aggregate material. The discrete particles present in the
light gray sample are more populous and twice the size of the particles in
the red material. There is no color banding in either sample, which could
be indicative of the stratified layers in a sandstone.

I may be making this harder than it has to be, but I am suspecting that
neither sample is sandstone.

ekomarnicki-at-MacDe
rmid.com To: holpc-at-firstenergycorp.com
cc: Microscopy-at-msa.microscopy.com
01/19/2004 09:13 Subject: [Microscopy] Re: SEM/LM of concrete vs.
AM sandstone

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

To
Microscopy-at-msa.microscopy.com
cc

Subject
SEM/LM of concrete vs. sandstone

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

-----------------------------------------
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reader of this message is not the intended recipient or an agent
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notified that you have received this document in error and that any
review, dissemination, distribution, or copying of this message is
strictly prohibited. If you have received this communication in error,
please notify us immediately, and delete the original message.

-----------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Tue Jan 20 21:17:50 2004

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I am intrigued by the similarity between your problem and a similar
problem confronting the Mars Rover scientists.
They are hoping that the landing site is a lake bed and are looking for
textures indicative of a sedimentary rock type, such as sandstone. All
they have is an optical microscope, an alpha-particle x-ray
spectrometer and an extraterrestrial grinder to make a flat surface
similar to your tools but significantly more expensive.

Sandstone is defined by texture: grain size, shape and sorting, not
chemistry.
Probably the last instrument a sedimentary petrologist would use is EDS
to define the rock type.
Look for rounded grains of quartz in a size range from 0.06 mm to 2.0
mm comprising most of the sample.
Larger than that is gravel, smaller is mud.

If you can't see the grains in a hand lens or binocular microscope you
may have a sediment with smaller grain size
such as a siltstone or mudstone or perhaps cement but not sandstone.

Your best bet is examining the texture in a petrographic thin section -
are these still made or am I too old.

Dr. Gordon Nord
Senior Scientist
Center for Applied Studies of the Environment
The Graduate School and University Center
City University of New York
365 Fifth Avenue
NY NY 10016-4309

On Monday, January 19, 2004, at 10:18 AM, holpc-at-firstenergycorp.com
wrote:

}
}
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}
}
} You raise questions on some of the perplexing results from this job.
} While
} I am well aware of the heterogeneous nature of the samples, a summary
} of
} the "bulk" analysis results yielded (approx.):
} Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also
} present.
} Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also
} present.
}
} A small piece from each sample was sanded through 320 grit paper to
} get a
} fresh, flat surface for the EDS analyses.
}
} Now, neither sample is known to be concrete nor sandstone. Neither
} sample
} contains any aggregate material. The discrete particles present in the
} light gray sample are more populous and twice the size of the
} particles in
} the red material. There is no color banding in either sample, which
} could
} be indicative of the stratified layers in a sandstone.
}
} I may be making this harder than it has to be, but I am suspecting that
} neither sample is sandstone.
}
}
}
}
}
} ekomarnicki-at-MacDe
} rmid.com To:
} holpc-at-firstenergycorp.com
} cc:
} Microscopy-at-msa.microscopy.com
} 01/19/2004 09:13 Subject: [Microscopy]
} Re: SEM/LM of concrete vs.
} AM sandstone
}
}
}
}
}
}
}
}
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} -------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
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} -----------------------------------------------------------------------
} --------
}
}
} Chris, I'm not a geologist or a cement expert, but concrete and mortar
} have cement as part of their make-up (ingredient). So you probably
} should
} start out comparing sandstone and cement. Commonly, concrete is cement
} with crushed stones (aggregates) in it. You don't mention having
} EDS at
} your disposal. Having EDS spectra obtained on your sample, I would
} expect
} higher Si concentration in the sandstone. and higher Ca conc. in the
} cement. Drop/spots tests may not reveal conc. differences. You may
} also
} want to run standards (i. e. Portland Cement, etc.) with your samples
} for
} positive confimation. Or even call a cement company and find out how
} they
} analyze their products. Hope this helps.
}
} The Materials Handbook, 13th ed. has some basic (starting) info on all
} three materials. ED
}
} Ed Komarnicki
} Sr. Analytical Chemist
} MacDermid Inc.
}
}
}
}
}
} holpc-at-firstenergycorp.com
} 01/19/04 08:09 AM
}
} To
} Microscopy-at-msa.microscopy.com
} cc
}
} Subject
} SEM/LM of concrete vs. sandstone
}
}
}
}
}
}
}
}
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} -------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
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} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
}
} One and all,
}
} I have been given two samples and asked to determine if they are
} concrete,
} sandstone, or some mix. One sample is light gray, and I suspect may be
} mortar rather than concrete. The other sample has a slight rust/red hue
} and
} contains appreciably more calcium. Both samples contain silica, and
} both
} test positive for calcium carbonate by the acid drop test, with the
} light
} gray sample showing a yellow residue from this test.
}
} Hours of reading test procedures for Portland cement and concrete,
} coupled
} with internet searches have left me wondering if I can draw a
} conclusion
} based on a few grams of sample. I would appreciate any suggestions
} about
} what to read or how to make this kind of determination.
}
} Thanks,
}
} Chris Holp
} FirstEnergy Corp.
} Beta Labs
} HolpC-at-firstenergycorp.com
}
}
}
} -----------------------------------------
} The information contained in this message is intended only for the
} personal and confidential use of the recipient(s) named above. If the
} reader of this message is not the intended recipient or an agent
} responsible for delivering it to the intended recipient, you are hereby
} notified that you have received this document in error and that any
} review, dissemination, distribution, or copying of this message is
} strictly prohibited. If you have received this communication in error,
} please notify us immediately, and delete the original message.
}
}
}
}
}
}
}
}
}
}
} -----------------------------------------
} The information contained in this message is intended only for the
} personal and confidential use of the recipient(s) named above. If the
} reader of this message is not the intended recipient or an agent
} responsible for delivering it to the intended recipient, you are
} hereby notified that you have received this document in error and that
} any review, dissemination, distribution, or copying of this message is
} strictly prohibited. If you have received this communication in error,
} please notify us immediately, and delete the original message.
}
}
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}

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 04:53:33 2004

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Stefan

I think you would really need to compare pictures from the same or similar samples. Ideally you would also need to see the process of producing images on the STEM because I suspect time and convenience for routine specimens would also be important.

I use a fairly old (} 10 years) Hitachi H7000 TEM with STEM and SEM facilities and it always takes longer to achieve a good STEM image than a TEM image. The STEM is useful for thick, low contrast specimens or x-ray analysis but for routine specimens the TEM will always be quicker and more convenient. Other issues may include whether it will take longer to train other users or more supervision would be needed with the STEM than with a TEM.

It may well be that modern SEM/STEM combinations are much improved (certainly resolution for a FEG should be much better) but it's worth considering how practical the STEM will be for routine TEM specimens. This will be greatly affected by the number and type of routine TEM specimens you handle.

I hope this helps.

Malcolm

Malcolm Haswell
e.m. unit
Chemispec
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: principe {eprincipe01-at-hotmail.com}

INVITATION

(1st Announcement)

College of Medicine & Health Sciences

Pathology Department

Electron Microscopy Unit

In collaboration with

Center for Community Service & Continuing Education

Invites you to attend

“OMAN FIRST ELECTRON MICROSCOPY WORKSHOP”

March 6 – 9, 2004

Venue: Lecture Theater 1, Sultan Qaboos University

Opening Ceremony: Saturday March 6 2004 at 9:00 a.m.

Tentative Program Schedule:

Day (1) Saturday, 6 March 2004

8:00-9:00 Registration, Coffee

9:00-9:45 Opening Ceremony

9:45-10:00 Break

10:00-11:00 Lecture

11:00-12:00 Lecture

12:00-12:30 Tour around EM Lab

12:30-14:00 Lunch

13:00-17:30 Sample preparation for TEM

Day (2) Sunday, 7 March 2004

8:30-9:30 Lecture

9:30-10:30 Lecture

10:30-11:00 Break / Exhibition

11:00-12:00 Lecture

12:00-13:00 Lunch

13:00-17:00 Sample preparation for SEM

19:00- 21:00 Workshop Dinner

Day (3) Monday, 8 March 2004

8:30-9:30 Lecture

9:30-10:30 Lecture

10:30-11:00 Break / Exhibition

11:00-12:00 Lecture

12:00-13:00 Lunch

13:00-17:00 Operation & Maintenance of Electron Microscopes

Day (4) Tuesday, 9 March 2004

8:30-9:30 Lecture

9:30-10:30 Lecture

10:30-11:00 Break / Exhibition

11:00-14:00 Operation & Maintenance of Electron Microscopes

14:00-15:00 Lunch

17:00-21:00 Tour - Muscat area

For registration and full details about the workshop please visit our web
site address:

http://www.squ.edu.om/med/NEWS/med/index.htm

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 08:03:34 2004

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Dear Microscopists

EDTA decalcification can be carried out on well-fixed specimens,
including corals, in a laboratory (tempreature-controlled) microwave
in a fraction of the time needed on the bench at room temperature.
Stirring during the process is important to keep fresh decalcifying
agent at the specimen at all times.

best regards,
Steven Slap

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 08:03:22 2004

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Dear Microscopists

EDTA decalcification can be carried out on well-fixed specimens,
including corals, in a laboratory (tempreature-controlled) microwave
in a fraction of the time needed on the bench at room temperature.
Stirring during the process is important to keep fresh decalcifying
agent at the specimen at all times.

best regards,
Steven Slap

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 08:39:48 2004

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The simplest technique is to have petrographic thin sections made
(there are several labs that specialize in this service at very reasonable
rates and turn-around times) and to use polarized light microscopy
(PLM). There
are several texts available for both sedimentary petrography (107 listed at
Amazon) or cement petrography (101 listed at Amazon). My background is in
geology, but I haven't looked at any rocks for a couple of years now, and I
have never compared a sandstone to a cement. However, if a client
brought a similar problem to my facility, PLM is the technique I would use.

Not to discredit any of the previous techniques (XRD, SEM/EDS, etc.) but
PLM
is the best way to go with this problem (in my opinion). Especially if you
aren't sure if you are looking at sandstone or cement or a third type of
rock/cement-like material, a few minutes with a PLM, and a couple of good
references one can provide a definite answer.

Bryan Bandli

----- Original Message -----
} From: "Warren E Straszheim" {wesaia-at-iastate.edu}
To: {Microscopy-at-msa.microscopy.com}
Sent: Tuesday, January 20, 2004 5:26 PM
Subject: [Microscopy] Re: SEM/LM of concrete vs. sandstone

}
}
}
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} To Subscribe/Unsubscribe --
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}
} I agree with James Talbot's opinion that X-ray diffraction would
probably
} give a definitive answer quite quickly. I think you might be able to
get a
} pretty good idea by taking spot analyses or an x-ray map of your two
} samples. (It is what I do - on concrete.) Concrete or mortar is such a
} heterogeneous mess that I would not get much out of an overall analysis.
} However, if I can probe the cement paste and find Ca and Si and O, I can
} suppose it to be Portland cement. There might also be unreacted cement
} grains. You should also find substantial amounts of fine aggregate
(i.e.,
} sand) used to make the mortar. Those could be of most any
composition, and
} often are. I see calcite, quartz, feldspars and more. Because cement and
} concrete are such hodge-podge mixtures, I often choose to do an x-ray
map
} rather than to probe every point in the image by hand.
}
} But back to x-ray diffraction, even if you can get chemistry from the
SEM,
} you may still want to use XRD for a more definitive answer about the
phases
} present. I use an SEM to solve a lot of problems, but it has its
} limitations. There is no substitute for diffraction or thermal
analysis or
} FTIR if the samples require it.
}
} Warren
}
} At 09:18 AM 1/19/2004, you wrote:
}
} } You raise questions on some of the perplexing results from this job.
While
} } I am well aware of the heterogeneous nature of the samples, a
summary of
} } the "bulk" analysis results yielded (approx.):
} } Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also
present.
} } Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also
present.
} }
} } A small piece from each sample was sanded through 320 grit paper to
get a
} } fresh, flat surface for the EDS analyses.
} }
} } Now, neither sample is known to be concrete nor sandstone. Neither
sample
} } contains any aggregate material. The discrete particles present in the
} } light gray sample are more populous and twice the size of the
particles
in
} } the red material. There is no color banding in either sample, which
could
} } be indicative of the stratified layers in a sandstone.
} }
} } I may be making this harder than it has to be, but I am suspecting that
} } neither sample is sandstone.
}
} -------------------------------------------
} No files should be attached to this message
} -------------------------------------------
} Warren E. Straszheim, Ph.D.
} Materials Analysis and Research Lab
} Iowa State University
} 46 Town Engineering
} Ames IA, 50011-3232
}
} Ph: 515-294-8187
} FAX: 515-294-4563
}
} E-Mail: wesaia-at-iastate.edu
} Web: www.marl.iastate.edu
}
} Scanning electron microscopy, x-ray analysis, and image analysis of
materials
} Computer applications and networking
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 09:31:46 2004

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Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

To
Microscopy-at-msa.microscopy.com
cc

Subject
SEM/LM of concrete vs. sandstone

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

-----------------------------------------
The information contained in this message is intended only for the
personal and confidential use of the recipient(s) named above. If the
reader of this message is not the intended recipient or an agent
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From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 13:23:19 2004

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Hi to all:
Attached to our HItachi H600 TEM, we have a Kevex Delta EDX system that has gone out. Specifically, smoke was seen coming out of the monitor shortly before it was last shut off with no image. The system was working fine until this event. We got a replacement monitor that has 5 inputs (RGBHV), but we still get no image. Is there a special type of monitor needed for these old systems, or should we be looking deeper into the system for other problems? The old monitor was an Electrohome ECM 1311U, Model 38-D051MA-UU.
Off-list replies OK.
thx
Mark Floyd
Forensic Analytical
Hayward, CA
msf-at-forensica.com

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Does anyone happen to have the error codes for the Agfa scanners? We
are having problems in scanning negatives, although the scans of
reflective materials are working fine.

We get back an error code saying the "scanner has a problem"
referencing code : F0000400:5

The Duoscan HiD model is hooked up to a Mac, and was working
faithfully for years. Reloading the software from the original CD
has helped us to get the error code rather than a freeze of the
machine, but has not solved the problem.

The Agfa machines are now out of production. I looked online and
found part of the manual available, but it doesn't include the pages
detailing troubleshooting. Thanks for any help in advance.

DHH
--
David H. Hall, Ph.D.
Center for C. elegans Anatomy
Department of Neuroscience
Albert Einstein College of Medicine
1410 Pelham Parkway
Bronx, NY 10461

www.wormatlas.org
www.aecom.yu.edu/wormem

phone 718 430-2195
fax 718 430-8821

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You raise questions on some of the perplexing results from this job. While
I am well aware of the heterogeneous nature of the samples, a summary of
the "bulk" analysis results yielded (approx.):
Lt. gray sample; O 38%, Si 40%, Ca 20%, with Mg, Al, and S also present.
Rust/Red sample; O 48%, Si 4%, Ca 47%, with Mg, Al, S, and Fe also present.

A small piece from each sample was sanded through 320 grit paper to get a
fresh, flat surface for the EDS analyses.

Now, neither sample is known to be concrete nor sandstone. Neither sample
contains any aggregate material. The discrete particles present in the
light gray sample are more populous and twice the size of the particles in
the red material. There is no color banding in either sample, which could
be indicative of the stratified layers in a sandstone.

I may be making this harder than it has to be, but I am suspecting that
neither sample is sandstone.

ekomarnicki-at-MacDe
rmid.com To: holpc-at-firstenergycorp.com
cc: Microscopy-at-msa.microscopy.com
01/19/2004 09:13 Subject: [Microscopy] Re: SEM/LM of concrete vs.
AM sandstone

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Chris, I'm not a geologist or a cement expert, but concrete and mortar
have cement as part of their make-up (ingredient). So you probably should
start out comparing sandstone and cement. Commonly, concrete is cement
with crushed stones (aggregates) in it. You don't mention having EDS at
your disposal. Having EDS spectra obtained on your sample, I would expect
higher Si concentration in the sandstone. and higher Ca conc. in the
cement. Drop/spots tests may not reveal conc. differences. You may also
want to run standards (i. e. Portland Cement, etc.) with your samples for
positive confimation. Or even call a cement company and find out how they
analyze their products. Hope this helps.

The Materials Handbook, 13th ed. has some basic (starting) info on all
three materials. ED

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

holpc-at-firstenergycorp.com
01/19/04 08:09 AM

To
Microscopy-at-msa.microscopy.com
cc

Subject
SEM/LM of concrete vs. sandstone

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One and all,

I have been given two samples and asked to determine if they are
concrete,
sandstone, or some mix. One sample is light gray, and I suspect may be
mortar rather than concrete. The other sample has a slight rust/red hue
and
contains appreciably more calcium. Both samples contain silica, and both
test positive for calcium carbonate by the acid drop test, with the light
gray sample showing a yellow residue from this test.

Hours of reading test procedures for Portland cement and concrete, coupled
with internet searches have left me wondering if I can draw a conclusion
based on a few grams of sample. I would appreciate any suggestions about
what to read or how to make this kind of determination.

Thanks,

Chris Holp
FirstEnergy Corp.
Beta Labs
HolpC-at-firstenergycorp.com

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Ed and Chris,

The difference between sandstones and concretes is usually fairly
obvious in a polished thin section viewed under plain and crossed
polars. The Atlas of sedimentary rocks under the microscope (Adams,
MacKenzie and Guilford, 1984, Longmans) gives examples of the commonest
types of sedimentary rock.
A sandstone is composed of two components the clasts (sand/rock) and the
cement (sorry that is the term the geologists use). Either of these
components may contain calcium bearing minerals, so the simple presence
of a signficiant calcium peak in an EDX spectra may not necessarily
prove that the material is a concrete. However, the cement of concrete
will not normally show visible crystallinity in the optical microscope
whereas many sandstones will. It also allows you to identify the clasts
and their size so distinguish between mortar and concrete (if samples is
large enough to include representative clasts).

ekomarnicki-at-MacDermid.com wrote:

}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Chris, I'm not a geologist or a cement expert, but concrete and mortar
} have cement as part of their make-up (ingredient). So you probably should
} start out comparing sandstone and cement. Commonly, concrete is cement
} with crushed stones (aggregates) in it. You don't mention having EDS at
} your disposal. Having EDS spectra obtained on your sample, I would expect
} higher Si concentration in the sandstone. and higher Ca conc. in the
} cement. Drop/spots tests may not reveal conc. differences. You may also
} want to run standards (i. e. Portland Cement, etc.) with your samples for
} positive confimation. Or even call a cement company and find out how they
} analyze their products. Hope this helps.
}
} The Materials Handbook, 13th ed. has some basic (starting) info on all
} three materials. ED
}
} Ed Komarnicki
} Sr. Analytical Chemist
} MacDermid Inc.
}
}
}
}
}
} holpc-at-firstenergycorp.com
} 01/19/04 08:09 AM
}
} To
} Microscopy-at-msa.microscopy.com
} cc
}
} Subject
} SEM/LM of concrete vs. sandstone
}
}
}
}
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} One and all,
}
} I have been given two samples and asked to determine if they are
} concrete,
} sandstone, or some mix. One sample is light gray, and I suspect may be
} mortar rather than concrete. The other sample has a slight rust/red hue
} and
} contains appreciably more calcium. Both samples contain silica, and both
} test positive for calcium carbonate by the acid drop test, with the light
} gray sample showing a yellow residue from this test.
}
} Hours of reading test procedures for Portland cement and concrete, coupled
} with internet searches have left me wondering if I can draw a conclusion
} based on a few grams of sample. I would appreciate any suggestions about
} what to read or how to make this kind of determination.
}
} Thanks,
}
} Chris Holp
} FirstEnergy Corp.
} Beta Labs
} HolpC-at-firstenergycorp.com
}
}
}
} -----------------------------------------
} The information contained in this message is intended only for the
} personal and confidential use of the recipient(s) named above. If the
} reader of this message is not the intended recipient or an agent
} responsible for delivering it to the intended recipient, you are hereby
} notified that you have received this document in error and that any
} review, dissemination, distribution, or copying of this message is
} strictly prohibited. If you have received this communication in error,
} please notify us immediately, and delete the original message.
}
}
}
}
}
}

--
Chris Salter,
Oxford Materials Characterisation Service,
Oxford University Begbroke Science Park,
Sandy Lane, Yarnton, Oxford, OX5 1PF
Tel 01865 283722, EPMA 283741, Mobile 07776031608

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 15:11:25 2004

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A quick question, does anyone known the thermal
conductivity/properties of carbon adhesive tabs used to mount SEM
samples? The various vendors talk about electrical conductivity but
not thermal.

Thanks
Scott
--
-----------------------------------------------------------------------
Scott D. Davilla Phone: 919 489-1757 ext 13 (tel)
4pi Analysis, Inc. Fax: 919 489-1487 (fax)
3500 Westgate Drive, Suite 403 email: davilla-at-4pi.com
Durham, North Carolina 27707-2534 web: http://www.4pi.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 15:14:28 2004

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Fellow Microscopists,

We are studying cell migration, as a result, I am interested in
opinions/suggestions on various motion tracking software solutions for
the analysis of cell movement. In my limited experience, I found that
following fluorescently labelled cells is easier than brighfield cells -
simpler to find fiducial points - so any suggestions for both types of
studies would be highly appreciated.

Thank you
Judy

Judy Trogadis
Bio-Imaging Coordinator
St. Michael's Hospital, 7Queen
30 Bond St.
Toronto, ON M5B 1W8
Canada
ph: 416-864-6060 x6337
pager: 416-685-9219
fax: 416-864-6043
trogadisj-at-smh.toronto.on.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 21 15:14:27 2004

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Ed and Chris,

The difference between sandstones and concretes is usually fairly
obvious in a polished thin section viewed under plain and crossed
polars. The Atlas of sedimentary rocks under the microscope (Adams,
MacKenzie and Guilford, 1984, Longmans) gives examples of the commonest
types of sedimentary rock.
A sandstone is composed of two components the clasts (sand/rock) and the
cement (sorry that is the term the geologists use). Either of these
components may contain calcium bearing minerals, so the simple presence
of a signficiant calcium peak in an EDX spectra may not necessarily
prove that the material is a concrete. However, the cement of concrete
will not normally show visible crystallinity in the optical microscope
whereas many sandstones will. It also allows you to identify the clasts
and their size so distinguish between mortar and concrete (if samples is
large enough to include representative clasts).

ekomarnicki-at-MacDermid.com wrote:

}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Chris, I'm not a geologist or a cement expert, but concrete and mortar
} have cement as part of their make-up (ingredient). So you probably should
} start out comparing sandstone and cement. Commonly, concrete is cement
} with crushed stones (aggregates) in it. You don't mention having EDS at
} your disposal. Having EDS spectra obtained on your sample, I would expect
} higher Si concentration in the sandstone. and higher Ca conc. in the
} cement. Drop/spots tests may not reveal conc. differences. You may also
} want to run standards (i. e. Portland Cement, etc.) with your samples for
} positive confimation. Or even call a cement company and find out how they
} analyze their products. Hope this helps.
}
} The Materials Handbook, 13th ed. has some basic (starting) info on all
} three materials. ED
}
} Ed Komarnicki
} Sr. Analytical Chemist
} MacDermid Inc.
}
}
}
}
}
} holpc-at-firstenergycorp.com
} 01/19/04 08:09 AM
}
} To
} Microscopy-at-msa.microscopy.com
} cc
}
} Subject
} SEM/LM of concrete vs. sandstone
}
}
}
}
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} One and all,
}
} I have been given two samples and asked to determine if they are
} concrete,
} sandstone, or some mix. One sample is light gray, and I suspect may be
} mortar rather than concrete. The other sample has a slight rust/red hue
} and
} contains appreciably more calcium. Both samples contain silica, and both
} test positive for calcium carbonate by the acid drop test, with the light
} gray sample showing a yellow residue from this test.
}
} Hours of reading test procedures for Portland cement and concrete, coupled
} with internet searches have left me wondering if I can draw a conclusion
} based on a few grams of sample. I would appreciate any suggestions about
} what to read or how to make this kind of determination.
}
} Thanks,
}
} Chris Holp
} FirstEnergy Corp.
} Beta Labs
} HolpC-at-firstenergycorp.com
}
}
}
} -----------------------------------------
} The information contained in this message is intended only for the
} personal and confidential use of the recipient(s) named above. If the
} reader of this message is not the intended recipient or an agent
} responsible for delivering it to the intended recipient, you are hereby
} notified that you have received this document in error and that any
} review, dissemination, distribution, or copying of this message is
} strictly prohibited. If you have received this communication in error,
} please notify us immediately, and delete the original message.
}
}
}
}
}
}

--
Chris Salter,
Oxford Materials Characterisation Service,
Oxford University Begbroke Science Park,
Sandy Lane, Yarnton, Oxford, OX5 1PF
Tel 01865 283722, EPMA 283741, Mobile 07776031608

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 00:45:58 2004

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Hi all,
Thank you to everyone who answered my query about TEM processing of
coral. We now have several methods to try, and the samples won't be
wasted.

Cheers,

Lyn Waterhouse
Adelaide Microscopy
University of Adelaide
Adelaide SA 5005
Ph: (08) 8303 4074 or 8303 5855
Fax: (08) 8303 4356
http://www.adelaide.edu.au/microscopy

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 08:20:29 2004

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Dear all,

I can't find the web site of this society?
SMI (Scientific Manufacturing Industries), 1399 Sixty-fourth Street
EMERYVILLE, CAL. 94608

perhaps it has moved?

I am surching for this product
micro-re/pettor : 1055A type D

Thank you all

Didier Goux -CENTRE DE MICROSCOPIE ELECTRONIQUE
Université de CAEN BASSE NORMANDIE- Campus I - Esplanade de la Paix
14032 CAEN cedex FRANCE
Tel : (33) 02.31.56.58.13 - Fax : (33) 02.31.56.56.00
} e-mail: didier.goux-at-unicaen.fr
visit our Web page : http://www.microscopie.unicaen.fr/microscopie/

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 09:29:48 2004

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Dear all,
I am trying to get a first rough idea of the cost of an above-screen CCD
camera for a TEM, suitable for recording Kikuchi patterns, together with
other diffraction patterns and images. I am looking at an above-screen
solution as my application requires a largish field of view. It would
need to fit in the ports available on a new TEM (yet to be ordered) to be
installed at the University of Glasgow (where I shall move to shortly).

If someone wishes to quote for a complete system including software for
the indexing of Kikuchi patterns, then I would also find that useful.

Also, generally I would be interested in any software for, or recent work
on, the automatic indexing of TEM Kikuchi patterns.

I need this information to help in making suitable estimates for the
equipment costings in a research proposal. Since the equipment is for the
UK, please give all estimates in British Pounds, where possible.

All the best

--
Ian MacLaren
Technische Universität Darmstadt
Material- und Geowissenschaften
Petersenstr. 23
64287 Darmstadt
Germany
http://www.tu-darmstadt.de/fb/ms/fg/sf/projekte/maclaren-Dateien/maclaren.html

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 12:20:49 2004

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Hi all,

We have a rare mouse coming in and don't want to goof on this one so I
wanted some advise.

Does anyone have any recommendations for fixation of neonatal (3 day)
mouse cardiac muscle for immuno? I had planned to use 0.5% glutaraldehyde
+ 3% PAF in 0.1M cacodylate buffer pH 7.4 containing 2mM MgCl, 1mMCaCl2, and
0.25% NaCl (final concentrations).

Do you fix neonatal and adult tissue similarly? If not, what modifications
do you make for the adult?

Many thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 14:51:45 2004

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I have a couple of students who need to look at thin films in cross
section in the TEM. Is there a classic reference for preparing cross
section samples?

Thanks,

Tom

------------------------------------------------------------------------
---------------------------------------------
Thomas M Murray email: murraytm-at-u.washington.edu
Electron Microscopy Center manager Phone: (206)543-2836
Materials Science & Engineering Fax: (206)543-3100
Box 352120 302 Roberts Hall Cell: (425)345-0083
University of Washington Home: (425)742-6819
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From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 15:54:16 2004

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At 01:00 PM 1/22/2004 -0800, you wrote:
} I have a couple of students who need to look at thin films in cross
} section in the TEM. Is there a classic reference for preparing cross
} section samples?

It's probably bad form to reply to a message asking for "classic
references" with a citation to one of my own papers, but I did write
something recently on preparing thin film cross sections by tripod
polishing. The paper is

{http://dx.doi.org/10.1016/S0304-3991(03)00092-5} "Imaging Individual Atoms
Inside Crystals with ADF-STEM" P. M. Voyles, J. L. Grazul, and D. A.
Muller, Ultramicroscopy 96, 251 (2003),

one the web at {http://dx.doi.org/10.1016/S0304-3991(03)00092-5} . It
contains a complete recipe for tripod polishing modified for HRTEM on
blanket thin film samples.

For devices or to achieve very large electron transparent but slightly
thicker areas, the original tripod polishing technique described in:

S. J. Klepeis, J. P. Benedict and R. M. Anderson, in: J. C. Bravman (Ed),
Materials Research Society Vol. 115, Pittsburgh Pa., 1988, p. 179.

J. Benedict, R. Anderson and S. J. Klepeis, in: R. Anderson, B. Tracy and
J. Bravman (Ed), Materials Research Society, Vol. 254, Boston, 1992, p. 121

is better.

Best wishes,
Paul Voyles

Paul Voyles
Assistant Professor
Materials Science and Engineering Department
University of Wisconsin - Madison
1509 University Ave.
Madison, WI 53706-1595
Voice: (608) 265-6740
Fax: (608) 262-8353
voyles-at-engr.wisc.edu
www.engr.wisc.edu/mse/faculty/voyles_paul.html

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 17:41:09 2004

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Tom:

There are several excellent references for doing TEM cross sections
depending on the method you would like to use. I have listed a few of
them below.

Dimpling/Ion Milling
Bravman and Sinclair, "The Preparation of Cross Section Specimens for
Transmission ELectron Microscopy, Journal of Electron Microscopy
Technique 1:53-61 (1984)

McCaffrey and Barna, "Preparation of Cross Sectional TEM Samples for Low
Angle Ion Milling, Microscpoy Reasearch and Technique 36:362-367 (1997)

MicroCleaving
McCaffrey, "TEM Samples of Semiconductors Prepared by a Small-Angle
Cleavage Technique", Materials Research Society Symposium Volume 254 pp
109-120

S.D. Walck, H. Colijn, G. Thompson, "Pre-thinning for FIB TEM Specimen
Preparation Using the Small Angle Cleavage Technique", Microscopy and
Microanalysis, Vol. 7(2001).

Tripod Polishing
J. Benedict, R. Anderson, S. Klepeis, M. Chaker, A Procedure for Cross
Sectioning Specific Semiconductor Devices for both SEM and TEM Analysis,
ed. R. Anderson, Mat. Res. Soc. Proc. vol 199, Pittsburgh, PA USA. Pp.
189, 1990.

We have a very thorough bibliography on our website which you can also
take a look at. If you find anything of interest there, let me know and
I will send you a copy. We also have numerous applcaition notes that
can be downloaded from the site.

There is also an excellent book you may want to look at titled:

"Progress in Transmission Eelctron Microscopy 1 - Concepts and
Techniques". The ISBN number is 3-540-67680-5 and it is available from
Springer (http://www.springer.de). The book is also available from
South Bay Technology, Inc. at a reduced price.

Chapter 10 in the book it titled "Advanced Techniques in TEM Specimen
Preparation". The chapter is edited by Shane Roberts who is the
Director of our Applications Laboratory and includes sections written by
Dr. John McCaffrey, Dr. Lucille Giannuzzi and Dr. Nestor J. Zaluzec.

Also Volumes 254 and 480 Of the Materials Research Society Proceedings
would be a great addition to your library.

I would be pleased to provide other references or advice at any time.
Please feel free to contact me or visit our website at
www.southbaytech.com and navigate to "Applications Support".

Best regards-

David

DISCLAIMER: As one of the world's leading suppliers of sample
preparation equipment and supplies for electron microscopy, South Bay
Technology, Inc. has a vested interest in promoting all of these
techniques as well as their use.

Tom Murray wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
} I have a couple of students who need to look at thin films in cross
} section in the TEM. Is there a classic reference for preparing cross
} section samples?
}
} Thanks,
}
} Tom
}
} ------------------------------------------------------------------------
} ---------------------------------------------
} Thomas M Murray email: murraytm-at-u.washington.edu
} Electron Microscopy Center manager Phone: (206)543-2836
} Materials Science ? Engineering Fax: (206)543-3100
} Box 352120 302 Roberts Hall Cell: (425)345-0083
} University of Washington Home: (425)742-6819
} Seattle, WA 98195

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Vice President

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From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 18:25:12 2004

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I have a couple of students who need to look at thin films in cross
section in the TEM. Is there a classic reference for preparing cross
section samples?

Thanks,

Tom

------------------------------------------------------------------------
---------------------------------------------
Thomas M Murray email: murraytm-at-u.washington.edu
Electron Microscopy Center manager Phone: (206)543-2836
Materials Science & Engineering Fax: (206)543-3100
Box 352120 302 Roberts Hall Cell: (425)345-0083
University of Washington Home: (425)742-6819
Seattle, WA 98195

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 22 19:06:33 2004

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Just to make this interesting thread a little more complete, let me add two
wildly different techniques that produce remarkably similar TEM specimens
(i.e. uniform, controlled thickness):

1. Diamond knife ultramicrotomy - I list some 20 thin film examples in a
slide I use to illustrate the versatility of UM, though some are coatings
rather than thin films. (How about diamond on cubic born nitride on single
crystal silicon!). The main advantage here is that almost every campus will
have ultramicrotomes in various life science departments (Medicine, Biology,
etc). Learning the technique for 'hard' materials is a challenge, however,
so your films better be fairly soft if you wish immediate results from the
life science campus practitioners.

2. Focused ion beam (FIB) - though David noted Lucille Gianuzzi's
contribution to the textbook he mentioned, there is still a fair bit of
unawareness concerning the versatility of FIB for cross-sections. We have a
collaboration with a small FIB company up here in the Great White North, and
if you visit their website (www.fibics.com), you will see interesting images
of cross-sections through Kodak film and a beverage can label, both of which
many might have prejudged to likley have unacceptable levels of ion damage.
That might still hold true for high resolution TEM, but these SED images
suggest that a lot can still be observed in 'soft' films sectioned via FIB.
However, the cost of a FIB is non-trivial, and there are still not that many
on campuses.

Tom

Dr. Tom Malis
Scientist Advisor
Natural Resources Canada
Govt. of Canada
Phone: 613-995-7358
cell: 613-371-4577
FAX: 613-947-6606
malis-at-nrcan.gc.ca

-----Original Message-----
} From: David Henriks
To: Tom Murray
Cc: Microscopy Listerver
Sent: 1/22/2004 5:32 AM

Tom:

There are several excellent references for doing TEM cross sections
depending on the method you would like to use. I have listed a few of
them below.

Dimpling/Ion Milling
Bravman and Sinclair, "The Preparation of Cross Section Specimens for
Transmission ELectron Microscopy, Journal of Electron Microscopy
Technique 1:53-61 (1984)

McCaffrey and Barna, "Preparation of Cross Sectional TEM Samples for Low
Angle Ion Milling, Microscpoy Reasearch and Technique 36:362-367 (1997)

MicroCleaving
McCaffrey, "TEM Samples of Semiconductors Prepared by a Small-Angle
Cleavage Technique", Materials Research Society Symposium Volume 254 pp
109-120

S.D. Walck, H. Colijn, G. Thompson, "Pre-thinning for FIB TEM Specimen
Preparation Using the Small Angle Cleavage Technique", Microscopy and
Microanalysis, Vol. 7(2001).

Tripod Polishing
J. Benedict, R. Anderson, S. Klepeis, M. Chaker, A Procedure for Cross
Sectioning Specific Semiconductor Devices for both SEM and TEM Analysis,
ed. R. Anderson, Mat. Res. Soc. Proc. vol 199, Pittsburgh, PA USA. Pp.
189, 1990.

We have a very thorough bibliography on our website which you can also
take a look at. If you find anything of interest there, let me know and
I will send you a copy. We also have numerous applcaition notes that
can be downloaded from the site.

There is also an excellent book you may want to look at titled:

"Progress in Transmission Eelctron Microscopy 1 - Concepts and
Techniques". The ISBN number is 3-540-67680-5 and it is available from
Springer (http://www.springer.de). The book is also available from
South Bay Technology, Inc. at a reduced price.

Chapter 10 in the book it titled "Advanced Techniques in TEM Specimen
Preparation". The chapter is edited by Shane Roberts who is the
Director of our Applications Laboratory and includes sections written by
Dr. John McCaffrey, Dr. Lucille Giannuzzi and Dr. Nestor J. Zaluzec.

Also Volumes 254 and 480 Of the Materials Research Society Proceedings
would be a great addition to your library.

I would be pleased to provide other references or advice at any time.
Please feel free to contact me or visit our website at
www.southbaytech.com and navigate to "Applications Support".

Best regards-

David

DISCLAIMER: As one of the world's leading suppliers of sample
preparation equipment and supplies for electron microscopy, South Bay
Technology, Inc. has a vested interest in promoting all of these
techniques as well as their use.

Tom Murray wrote:

}
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}
} I have a couple of students who need to look at thin films in cross
} section in the TEM. Is there a classic reference for preparing cross
} section samples?
}
} Thanks,
}
} Tom
}
}
------------------------------------------------------------------------
} ---------------------------------------------
} Thomas M Murray email:
murraytm-at-u.washington.edu
} Electron Microscopy Center manager Phone: (206)543-2836
} Materials Science ? Engineering Fax:
(206)543-3100
} Box 352120 302 Roberts Hall Cell:
(425)345-0083
} University of Washington Home:
(425)742-6819
} Seattle, WA 98195

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
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email: henriks-at-southbaytech.com

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 03:16:51 2004

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----- Forwarded by ahk/RES/RVN/Haldor Topsoe on 23-01-04 10:24 -----

"Anne-Mette Heie
Kjćr" To: Tom Murray {murraytm-at-u.washington.edu}
{ahk-at-topsoe.dk} cc:
bcc:
23-01-04 09:23 Subject: [Microscopy] Re: Reference for TEM cross-section Sample Prep(Document link: ahk)

Hi!

If you have to prepare the cross-section "by hand in the oldfashioned way"
- without ultramicrotome or FIB, I would strongly advise you to buy a Gatan
cross-sectional kit. It saves you a lot of time.

Best regards
Anne-Mette Heie Kjaer

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 05:45:55 2004

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A few openings are still available for the course on Quantitative Image
Analysis that will be taught in Orlando, Florida, March 11 - 12 by John Russ. The
course emphasizes practical solutions to imaging problems and includes 2 days
of intensive training in current techniques, including an evening open
laboratory where participants are encouraged to bring and work with their own images.
The course is taught using the Fovea Pro software
{http://www.reindeergraphics.com/foveapro} , which participants receive as well as a copy of "The Image
Processing Handbook" 4th Edition (CRC Press).

The course syllabus and registration information are available at the
Reindeer Graphics website. {http://www.reindeergraphics.com/courses} Further
information may be obtained from the website or by contacting Reindeer Graphics
directly at courses-at-reindeergraphics.com or by telephone at 828.252.7515. The
deadline for registration is February 1st, so act now.

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 06:51:32 2004

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Hi Ian,

An early paper on automatic indexing of Kikuchi line patterns was

N. C. Krieger Lassen:
"Computerized analysis of Kikuchi patterns"
In: Proceedings of the 16th Risoe International Symposium on Materials Science,
"Microstructural and Crystallographic Aspects of Recrystallization"
Edited by N. Hansen et al.
Risoe National Laboratory, Roskilde, Denmark 1995
ISBN 87-550-2088-7
ISSN o907-0079

Best regards,
Jorgen.
{:::} --- {:::} --- {:::} --- {:::} --- {:::} --- {:::}

Joergen B. Bilde-Soerensen
Senior Research Scientist, Ph. D.
Materials Research Department
Risoe National Laboratory
DK-4000 Roskilde
Denmark

e-mail: j.bilde-at-risoe.dk
phone: +45 4677 5802 (direct)
phone: +45 4677 4677 (switchboard)
fax: +45 4677 5758
website: http://www.risoe.dk/afm/Personal/jqbi/jqbi.htm

-----Original Message-----
} From: Ian MacLaren [mailto:maclaren-at-tu-darmstadt.de]
Sent: 22. januar 2004 16:37
To: Microscopy Listserver

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (petra.rosner-at-ww.uni-erlangen.de) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, January 23, 2004 at 06:31:59
---------------------------------------------------------------------------

Email: petra.rosner-at-ww.uni-erlangen.de
Name: Petra Rosner

Organization: Universit”t Erlangen N¸rnberg

Title-Subject: [Microscopy] [Filtered] MListserver:

Question:
Hi,
has anyone experience in preparing bulkmaterial of bromide specimen for TEM?

Petra

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 08:25:52 2004

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Email: rgrebe-at-jhmi.edu
Name: Rhonda R. Grebe

Organization: The Johns Hopkins University

Title-Subject: [Microscopy] [Filtered] MListserver: auto-fluorescence of melanin in fetal human eye

Question: Will the melanin contained in the retinal pigment epithelium and choroid of the fetal human eye absorb the light and prevent visualization of fluorescently labeled endothelial cells, etc. in the choriodal vessels of unbleached whole mount choroidal tissue? If it is possible to visualize the choroidal vessels, what would be the most efficient excitation wave lenght to use? And finally, would a conventional inverted fluorescent scope with a UV and a super high pressure mercury lamp power supply be sufficient for this purpose or is a confocal required?

Thank you,

Rhonda Grebe

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 08:36:46 2004

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Hi,

We are surplusing a cabinet full of old RCA EMU TEM manuals and parts
(we've announced this before, but it's for real this time), and wanted
to check if anybody has any use for them. We have lots a vacuum tubes,
both new and used, miscellaneous parts, like lead glass, a film holder,
a lot of new and used filaments, and others, as well as a stack of
hardbound manuals. The old kind, with decent binding and illustrations
and glossy paper.

If this interests anyone, we will send them for shipping costs. We need
the cabinet space for our overflowing supply of researchers' grids.

Thanks,

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 08:37:41 2004

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Hi all,

I have also experienced the constantly changing guidelines for UA
disposal brought up by Tom Phillips. We have gone full circle here from
"dilute and pour down the drain", to collecting it with other fixatives
for pickup, to collecting it separately for pickup and disposal by the
radiation people (along with any pipettes, syringes, etc. that have
touched it), and back to dilute and pour. In my experience a major rule
change happens about every six months. The problem seems to be that the
extremely low level of radioactivity apparently doesn't justify the very
high cost of the specialized disposal methods used for "hot" wastes (er,
used materials---sorry), and there doesn't seem to be any consensus
about how dangerous small amounts of the material actually are. The odd
thing to me is that I have heard for many years, rightly or wrongly,
that UA is only dangerous when allowed to accumulate in larger
quantities or when it is in powder form and can be inhaled. It seems
strange then that rules for pickup either seem to require its
accumulation or, more rarely, the evaporation of the solvent liquid to
return UA to powder form and reduce the collection volume (although I
haven't seen that particularly approach required any place where I have
worked---so far).

My favorite UA tale comes from another lab I worked in, when we were
told by the safety people that we could use UA, but we could not pour it
down the sink, we were not allowed to accumulate it, and the safety
folks would no longer pick it up because they didn't know what to do
with it. What did we do? We kept it large bottles out of sight until
the inevitable rule change happened.

Maybe the microscopy community could come up with a consensus
recommendation on how to handle this problematic substance in an effort
to bring some standardization to its handling. The web of federal,
state, and local regulations on hazardous waste probably make this
difficult, but we need to try to seal up the crack that UA appears to
keep falling through.

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 09:28:19 2004

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Greetings,
Two comments on the UA situation.

My favorite story: Where I was in graduate school was a small
research institute, started around 1900. Over the years, a large set
of shelves where chemicals were stored went from communal necessity
to historical relic as labs maintained their own supplies. By the
time I was there, these shelves were fascinating, containing bottles
of colored powder with handwritten labels from Germany or murky
gray-black solids labeld odd things like 'hairy tin'. One day,
someone looking at the more neglected shelves covering last part of
the alphabet, way down near the floor, found a bottle of UA.
Handwritten label, radiation detectable with a Geiger counter
through the bottle (probably not so pure as today's stuff). Ignored,
this stuff for years had led an untroubled existence, but
discovered--something had to be done. But what? The institute was
attached to a University which was right then being hammered by the
NRC for alleged abuses of radiation safety, so they wanted to play by
the rules. But the trouble was that the rules demanded that all
radioactive compounds be inventoried as soon as they arrived on
campus, and fines were levied based on the number of days the
compound was on campus but off inventory. There were a lot of days
between then and say 1907! The solution was simple but not elegant.
It involved some shovels, a bag or two of ready mix, and a big hole
in the back of the compound. You can imagine the rest.

The other comment is to point out why UA causes such a
regulatory problem. Danger from low doses of anything is hard to
study because the sample sizes are too huge. So danger from low doses
is extrapolated from high doses. This is obviously uncertain and
leads to lots of models, and with the uncertainty, a lot of argument.
A useful benchmark for UA is the radiation in the rocks all around
us. Probably the diluted UA we use to stain grids has on that order
of radiation and adding it the drain poses no more risk than posed by
our surroundings. Likewise the small amount of heavy metal in the
solution can probably be reduced to the usual ambient levels in tap
water by modest dilution. But agreeing to this in a regulatory
sense means taking a stand on the low dose end and this is difficult.
Though probably wise.

My few decays,
Tobias
}
}
} Hi all,
}
} I have also experienced the constantly changing guidelines for UA
} disposal brought up by Tom Phillips. We have gone full circle here from
} "dilute and pour down the drain", to collecting it with other fixatives
} for pickup, to collecting it separately for pickup and disposal by the
} radiation people (along with any pipettes, syringes, etc. that have
} touched it), and back to dilute and pour. In my experience a major rule
} change happens about every six months. The problem seems to be that the
} extremely low level of radioactivity apparently doesn't justify the very
} high cost of the specialized disposal methods used for "hot" wastes (er,
} used materials---sorry), and there doesn't seem to be any consensus
} about how dangerous small amounts of the material actually are. The odd
} thing to me is that I have heard for many years, rightly or wrongly,
} that UA is only dangerous when allowed to accumulate in larger
} quantities or when it is in powder form and can be inhaled. It seems
} strange then that rules for pickup either seem to require its
} accumulation or, more rarely, the evaporation of the solvent liquid to
} return UA to powder form and reduce the collection volume (although I
} haven't seen that particularly approach required any place where I have
} worked---so far).
}
} My favorite UA tale comes from another lab I worked in, when we were
} told by the safety people that we could use UA, but we could not pour it
} down the sink, we were not allowed to accumulate it, and the safety
} folks would no longer pick it up because they didn't know what to do
} with it. What did we do? We kept it large bottles out of sight until
} the inevitable rule change happened.
}
} Maybe the microscopy community could come up with a consensus
} recommendation on how to handle this problematic substance in an effort
} to bring some standardization to its handling. The web of federal,
} state, and local regulations on hazardous waste probably make this
} difficult, but we need to try to seal up the crack that UA appears to
} keep falling through.
}
}
} Randy Tindall
} EM Specialist
} Electron Microscopy Core Facility---We Do Small Well!
} W122 Veterinary Medicine
} University of Missouri
} Columbia, MO 65211
} Tel: (573) 882-8304
} Fax: (573) 884-5414
} Email: tindallr-at-missouri.edu
} Web: http://www.biotech.missouri.edu/emc/

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 10:36:14 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Anthony_McCormick-at-brown.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, January 23, 2004 at 09:01:03
---------------------------------------------------------------------------

Email: Anthony_McCormick-at-brown.edu
Name: Anthony McCormick

Organization: Brown University

Title-Subject: [Microscopy] [Filtered] MListserver:HPGe x-ray detector

Question: We have recently had a window failure on a HPGe x-ray detector for the JEOL 2010 TEM. Upon asking the manufacturer of this detector about repairing the window, their reply was "We can only repair the HPGe detector only if it is converted to a SiLi detector...". Are HPGe detectors no longer available? Are there companies that repair/replace windows on x-ray detectors on equipment that they did not manufacture?

Anthony McCormick
Electron Microscope Facility
014 Barus & Holley
Brown University
Providence, RI 02912
(401) 863-3909

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 11:40:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (swwatkins-at-pitt.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, January 23, 2004 at 11:30:40
---------------------------------------------------------------------------

Email: swwatkins-at-pitt.edu
Name: Simon watkins

Organization: University of Pittsburgh

Title-Subject: [Microscopy] [Filtered] QFM 2k04

Question: Folks,

We would like to announce that enrollment for Quantitative Fluorescence Microscopy 2k04 at the Mount Desert Island Marine Laboratory in Maine is now open. The tremendous success of the course over the last several years has encouraged us to run it again next year, and as it is January it is time to start our enrollment. This is an intensive lab/lecture course, focusing on fluorescence microscopy in all its forms, including widefield, Confocal, Multiphoton, Decon, TIRF, FRET etc, though with an emphasis on live cell methods. We also encourage students to provide their own specimens such that the hands on components of the course are as enriching as possible. Enrollment is highly competitive, so if you think that you or your colleagues would benefit from the course please enroll as soon as possible. The url for the course is http://www.cbi.pitt.edu/qfm/index.html

If you have any specific questions about the course feel free to contact me directly I look forward to hearing from interested applicants soon
Thanks
Simon

By the way; I am sorry if this is a repost, but I still have not seen my original mailing to the group. Nestor, could you let me know if this has been posted so I avoid future duplications.

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From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 12:19:12 2004

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Dear List,
I have lost track of Doug Dorset's contact info, and the MSA directory
did not reveal it. Could someone--preferably Doug--please reply
off-list with his email address? TIA.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 13:52:51 2004

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Dear Lists,
We have been experiencing an unusual problem on the F30H. At
intervals of a few weeks the vacuum measured by the IGP at the top of
the FEG (IGP3 for those who know the scope) deteriorates and the FEG is
shut off by the computer. Examination of a record of the vacuum shows
that IGP3 has a vacuum too good to show above baseline for the first
few days--the reading is constant at 10^-12 Pa--then the pressure rises
into the range of ~10^-7 Pa, often will briefly get slightly better,
then will rather quickly get worse and the FEG will shut off. The
boards containing the power supply and the electronics for measuring
the vacuum have been replaced, but that did not solve the problem.
Both the FEG and IGP are pretty simple devices, and it is hard to think
of what could be going wrong. A vacuum leak would not show the
observed time course of vacuum readings, and the SF6 that surrounds the
outside of the FEG apparatus would give different symptoms.
Has anyone seen anything similar? TIA for any help.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 16:04:52 2004

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Hi All,

Thanks for the replies. I now have much reading to do, but I feel I
will have the knowledge at the end to make successful samples.

There were a couple of questions on the system I'm looking at. The
samples are cobalt oxide deposited onto a lanthanum oxide substrate.

Once I get into the actual hands on portion of sample prep I may be
back for some pointers.

Thanks for the swift and copious relies.

Tom

------------------------------------------------------------------------
---------------------------------------------
Thomas M Murray email: murraytm-at-u.washington.edu
Electron Microscopy Center manager Phone: (206)543-2836
Materials Science & Engineering Fax: (206)543-3100
Box 352120 302 Roberts Hall Cell: (425)345-0083
University of Washington Home: (425)742-6819
Seattle, WA 98195

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 23 16:36:41 2004

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Dear Bill,
I have maintained both the Coates and Welter and Zeiss (LEO) DSM982 Gemini
FESEMs in this lab. Although a frequent bake out routine is performed,
after several thousand hours of operation (~2 years), my SEM gun ion pumps
sometimes began to 'burp' intermittently. Without going into all of the
possible reasons I guess that most likely the pumps are growing titanium
whiskers. Some of those whiskers are shorting out the pump power supply for
a fraction of a second until they burn away. Of course the vacuum appears
very bad for a split second during that short circuit and the gun power
supply kicks off (just when I'm about to leave on vacation). For about 24
years the fix that works for me is to whack the ion pump with the palm of
my hand several times before and after a bake (cooled first). (NEVER DO
THIS WITH THE FEG ON OR ION PUMP HOT). This causes the vacuum readout to
jump several orders of magnitude (into the poorer direction) but after
about 30 minutes, the vacuum recovers and remains stable. [I usually whack
until the readout begins to drop toward recovery (~2-3 seconds) and a
second try for good measure). Firm but cautious taps is the best way I can
describe the force of these 'whacks'.]

Caution: If your ion pumps are very used, whacking them may cause titanium
flakes to come loose and short the grids permanently. I have been lucky and
not lost a pump yet. Depending on the tightness of the vacuum system my ion
pumps have worked very well for about 6-10 years each. Before computer
interfaces I use to 'hi pot' an ion pump by sending the output of a high
voltage spark generator into it for a few seconds (FE emitter grounded to
anode, SEM ion pump power supply disconnected and all circuits off and
disconnected from the column). That is another way to get rid of whiskers
but not recommended as it obviously risks damage to the microscope computer
control circuits (and the technician).

Good luck,
Jim

Disclaimer:
I am not responsible for any damage incurred to you or your equipment if
the above methods are used. I am not familiar with an F30H microscope and
the vibrations from this method could damage or loosen the emitter or other
components in the area of the ion pump. Shock hazard is always present when
working with these devices. Refer to qualified personal only.

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

James S. Romanow
The University of Connecticut
Physiology and Neurobiology Department
Electron Microscopy Facility
Unit 3242
91 North Eagleville Road
BSP Building, Room G06
Storrs, CT 06269-3242

860 486-2914 voice
860 486-6369 fax
james.romanow-at-uconn.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 24 10:07:12 2004

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Email: rpowell-at-nanoprobes.com
Name: Rick Powell at Nanoprobes

Organization: Nanoprobes, Incorporated

Title-Subject: [Microscopy] Re: WWW: nanogold labeling

Question: Hello Eunice:

I assume that you are planning to use gold-labeled antibodies for your experiment (our product, Nanogold, can be used tolabel other types of probes of different sizes; if you are planning to Nanogold-label a much smaller or larger protein and use this to stain your preparation, or if you plan to use a Nanogold labeling reagent to mark a specific chemical group in your specimen, it will likely make a difference to your staining procedure)...in any case, labeling procedures similar to those used for pre-embedding labeling should work well. We have an article on our web site that gives some procedures:

http://www.nanoprobes.com/App3.html

References:

(1) Tanner, V. A., Ploug, T., and Tao-Cheng, J.-H. Subcellular localization of SV2 and other secretory vesicle components in PC12 cells by an efficient method of preembedding EM Immunocytochemistry for cell cultures. J. Histochem. Cytochem., 44, 1481-1488 (1996).
(2) Du, J.; Tao-Cheng, J.-H.; Zerfas, P., and McBain, C. J. The K+ channel, Kv2.1, is apposed to astrocytic processes and is associated with inhibitory postsynaptic membranes in hippocampal and cortical principal neurons and inhibitory interneurons. Neuroscience, 84, 37-48 (1998).

If you mean the Nanoprobes product, Nanogold, then we also maintain a comprehensive list of references sorted by application, which includes a section on pre-embedding labeling:

http://www.nanoprobes.com/RefTopNG.html#Npre

Lin et al's paper may also be helpful (Lin, M., Sistina, Y., and Rodger, J. C.: Electron-microscopic localisation of thiol and disulphide groups by direct monomaleimido-Nanogold labeling in the spermatozoa of a marsupial, the tammar wallaby (Macropus eugenii); Cell Tisue Res., 282, 291-296 (1995)).

If negative staining is an option, we offer NanoVan, a negative stain based on vanadium; since vanadium has lower Z than uranium, NanoVan gives a lighter stain that uranyl acetate and allows easier visualization of small gold particles, and can be mixed with our tungsten-based negative stain, Nano-W, to increase density (http://www.nanoprobes.com/Nstain.html). The vast majority of publications by our users describe the use of osmium tetroxide, most frequently after silver enhancement of the gold. A few papers describe the use of uranyl acetate withour osmium tetroxide. Hebert et al used postfixation in 1% osmium tetroxide, 1% potassium ferrocyanide (Hebert, S. S.; Daviau, A.; Grondin, G.; Latreille, M.; Aubin, R. A.; and Blouin, R.: The mixed lineage kinase DLK is oligomerized by tissue transglutaminase during apoptosis. J. Biol. Chem., 275, 32482-90 (2000)).

Hope this helps,

Rick Powell
Nanoprobes, Inc.

*****************************************************************************************
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NANOPROBES, Incorporated
95 Horse Block Road, Yaphank, NY 11980-9710, USA

US Toll-free: (877) 447-6266 * Tel: (919) 845-6324 * Fax: (631) 980-3608

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From MicroscopyL-request-at-ns.microscopy.com Sun Jan 25 12:45:16 2004

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Hello Listers:

I have a question regarding morphometric analysis, specifically how many
individual measurements should be done for a cardiac muscle research
project?

The investigators have 4 groups of muscle tissue. Group one, the control
has 3 specimens, experimental groups contain 5, 6 & 6 specimens
respectively. So that equals 20 specimens total.

I have been asked to measure the width of 20 muscle fibers for each specimen
and the diameter of 20 individual fibers on cross section in each group.
That adds up to 800 measurements! This seems like overkill. Wouldn't ten
do? Does anyone have a reference for how one would measure and what numbers
of samples are necessary to provide a statistically appropriate sampling
when using a transmission electron microscope.?

Thanks for any advice!

Karen Bentley

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 03:16:08 2004

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Dear Petra,

I don't have any experience with bromide material, but I will just make you aware that most halides are very difficult to work with in TEM because the specimens are very rapidly filled with radiation-induced defects unless they are cooled to very low temperatures.

Best regards,
Jorgen.

{:::} --- {:::} --- {:::} --- {:::} --- {:::} --- {:::}

Joergen B. Bilde-Soerensen
Senior Research Scientist, Ph. D.
Materials Research Department
Risoe National Laboratory
DK-4000 Roskilde
Denmark

e-mail: j.bilde-at-risoe.dk
phone: +45 4677 5802 (direct)
phone: +45 4677 4677 (switchboard)
fax: +45 4677 5758
website: http://www.risoe.dk/afm/Personal/jqbi/jqbi.htm

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:petra.rosner-at-ww.uni-erlangen.de]
Sent: 23. januar 2004 15:35
To: microscopy-at-ns.microscopy.com

Dear all in Western/Central Europe,
Are there likely to be any courses/workshops on specimen preparation in
the near future in western or central Europe? In particular it would be
lovely for my colleagues if they are held in German somewhere in one of
the German speaking countries. Alternatively, they could be held in
English in somewhere reasonably easily reached from the western side of
Germany.
I can train people to some extent in specimen prep, but it would be nice
if they could learn further through courses, hands-on training or such
like.

Best wishes

--
Ian MacLaren
Technische Universität Darmstadt
Material- und Geowissenschaften
Petersenstr. 23
64287 Darmstadt
Germany
http://www.tu-darmstadt.de/fb/ms/fg/sf/projekte/maclaren-Dateien/maclaren.html

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 06:32:31 2004

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Hi

Your question is a little like "how long is a piece of string"! The number
of readings you need will depend mostly on the variation within and between
the different samples.

You could try a test within your control group - take the readings and plot
a cumulative mean. Eventually the curve will become 'flat' indicating that
you have reached a point where there is 'no point' in continuing - the
statistical equivalent of empty magnification.

I am a little confused about your use of the words 'width' and 'diameter' -
in a cylindrical object, are they not the same thing?

All the best

Gareth
Med vänliga hälsningar/With best regards

Gareth

***Come to Stockholm in 2004 to the 26th IFBLS congress*** Take a look at
http://www.vardforbundet.se/ifbls2004

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 08:40:58 2004

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Hi Karen,

I don't agree this is overkill.
I have done this type of quantitation before, and ended
up doing close to 100 measurements per sample! Since
these measurements can be done at low magnification,
you should be able to measure several fibers from each
micrograph, therefore greatly reducing the number of
micrographs you need to take. 800 measurements might
seem like a lot, but in fact it wouldn't take that long if you
are using an appropriate sampling and measurement
technique. The fact is you need to sample a lot because
of the huge variations you are going to observe, especially
if you are measuring fiber width from longitudinal sections
as in this case you have no way of knowing if the plane
of section is going through the center of the fiber or not.
Even when measuring diameters from cross-sections,
you expect some variation as sections through the ends
of fibers are likely to be smaller than those through the
center.
Good luck!

Marc

On Sunday, January 25, 2004, at 01:56 PM, Jensen, Karen wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Hello Listers:
}
} I have a question regarding morphometric analysis, specifically how
} many
} individual measurements should be done for a cardiac muscle research
} project?
}
} The investigators have 4 groups of muscle tissue. Group one, the
} control
} has 3 specimens, experimental groups contain 5, 6 & 6 specimens
} respectively. So that equals 20 specimens total.
}
} I have been asked to measure the width of 20 muscle fibers for each
} specimen
} and the diameter of 20 individual fibers on cross section in each
} group.
} That adds up to 800 measurements! This seems like overkill. Wouldn't
} ten
} do? Does anyone have a reference for how one would measure and what
} numbers
} of samples are necessary to provide a statistically appropriate
} sampling
} when using a transmission electron microscope.?
}
} Thanks for any advice!
}
} Karen Bentley
}
} Karen L. Bentley, M.S.(previously Jensen)
} Associate Scientist & Project Manager
} Electron Microscope Research Core
} University of Rochester Medical Center
} Rochester, NY 14642
} 585-275-1954
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 09:26:21 2004

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Hi Karen:

Have a look at "Unbiased Stereology" by C.V Howard and M.G. Reed,
BIOS Scientific Publishers in the UK, Springer in the USA, 1998. In
order to determine if a sample size is "big enough", you will have to do
the trial measuerements suggested by Gareth Morgan. Too large a sample
wastes your time, too small risks having the paper retuned for more data
at a much later time (when details and technique have been forgotten).
In my experience measuring things always sounds like more work than it
turns out to be. Once you get rolling it is not that bad.

Geoff

Jensen, Karen wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 09:59:15 2004

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Your question is fairly basic, and that is good, because if it was much
more than that, it would be beyond me. {G}

Similar to what Gareth wrote, the measured mean value will stabilize with
increased measurements. After multiple measurements, you will be able to
determine a mean and standard variation for the population. Both values
SHOULD be stable no matter how many measurements you take, but of course it
isn't - you have only taken a finite sampling of the entire population. But
for multiple random samplings of a population, you will find that the
standard deviation in the multiple mean values is equal to the standard
deviation of the population divided by the square root of the number of
measurements in each sampling.

So consider this example. You take 16 measurements and calculate a mean of
40 um with a standard deviation of 4 um. That 4 um refers to the deviation
in any one measurement in the population. How good is your average
measurement? It's standard deviation would be 1 um. But suppose you have a
different population for which 16 measurements gives you a mean value of 41
also with a standard deviation of 4 um. Are the two populations
significantly different? The means are only one standard deviation apart;
it is not very certain. But suppose you took 64 measurements per population
and obtained the same means and standard deviations. Now the expected
deviation in the mean is now 0.5 um due to the increased measurements and
the means are now 2 standard deviations apart. That increases the certainty
markedly. I haven't dug out my stat tables to verify the exact numbers, but
I think the chance of the populations having the same mean dropped from
around 37% to around 5% due to the larger sampling. I believe it is the
T-test that is used to determine the certainty of such differences.

In your case, cutting the number of measurements from 20 to 10 will lead to
a 41% increase in the standard deviation of the mean (SD-10 = SD/Sqrt(10)
and SD-20 = SD/Sqrt(20), so SD-10 = Sqrt(2)*SD-20). That may or may not be
allowed for the magnitude of the differences between your groups. Indeed, I
don't believe it is possible to determine the required sample size without
some knowledge of the standard deviations of the populations. Once that is
known, you can theoretically set the number of measurements to achieve the
desired level of precision, no matter how small; however, you will be
constrained by reality. For example, if SD=0.5 units and you wish to detect
differences of 0.02 units, you probably want the standard deviation of the
mean to be 0.01 units. But that means 0.01=0.5/Sqrt(N), so N=2500
measurements. That is probably not practical. You would probably pick a
realistic number of measurements then calculate and report your minimum
detectable difference for those conditions. Since you have to quadruple the
number of measurements to improve the precision by a factor of 2, you
quickly run into practical limits.

It is also probably worth a trip to a statistics book or a stat consultant
at that stage. Even as I write, I am remembering principles such as the
standard deviation in the difference of means of two populations is the
root of the sum of the squares of the deviations of the means of the
populations involved. You are testing to see if |Mean(A)-Mean(B)| } 0. It
may not be possible to explain such issues succinctly and concisely through
e-mail. A book or consultant would probably do better, but I hope this
helps some.

Warren

At 12:56 PM 1/25/2004, you wrote:

} Hello Listers:
}
} I have a question regarding morphometric analysis, specifically how many
} individual measurements should be done for a cardiac muscle research
} project?
}
} The investigators have 4 groups of muscle tissue. Group one, the control
} has 3 specimens, experimental groups contain 5, 6 & 6 specimens
} respectively. So that equals 20 specimens total.
}
} I have been asked to measure the width of 20 muscle fibers for each specimen
} and the diameter of 20 individual fibers on cross section in each group.
} That adds up to 800 measurements! This seems like overkill. Wouldn't ten
} do? Does anyone have a reference for how one would measure and what numbers
} of samples are necessary to provide a statistically appropriate sampling
} when using a transmission electron microscope.?
}
} Thanks for any advice!
}
} Karen Bentley
}
} Karen L. Bentley, M.S.(previously Jensen)
} Associate Scientist & Project Manager
} Electron Microscope Research Core
} University of Rochester Medical Center
} Rochester, NY 14642
} 585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 10:12:40 2004

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I have found a home for the RCA manuals and parts. I'll be responding
individually to everyone who answered my query shortly. Thanks to all.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 10:24:39 2004

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Ian:

South Bay Technology regularly conducts specimen preparation workshops around the
world as well as in our own facility here in San Clemente, CA. We also do
cutomized workshops for customers that we can do at your facility. We cover any
topic in specimen preparation: Tripod Polishing, Dimpling, Low Energy Ion Milling,
Jet Polishing, Plasma Cleaning, Plasma Trimming, Pre-FIB preparation, MicroCLeaving
etc. Please contact me off-line and I will let you know what we have planned and
what we can arrange to meet your needs.

Best regards-

David

Ian MacLaren wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
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} -------------------------------------------------------------------------------
}
} Dear all in Western/Central Europe,
} Are there likely to be any courses/workshops on specimen preparation in
} the near future in western or central Europe? In particular it would be
} lovely for my colleagues if they are held in German somewhere in one of
} the German speaking countries. Alternatively, they could be held in
} English in somewhere reasonably easily reached from the western side of
} Germany.
} I can train people to some extent in specimen prep, but it would be nice
} if they could learn further through courses, hands-on training or such
} like.
}
} Best wishes
}
} --
} Ian MacLaren
} Technische Universit?t Darmstadt
} Material- und Geowissenschaften
} Petersenstr. 23
} 64287 Darmstadt
} Germany
} http://www.tu-darmstadt.de/fb/ms/fg/sf/projekte/maclaren-Dateien/maclaren.html

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy,
Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and
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If you are not the intended recipient, please do not read, copy or disclose this
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From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 13:28:25 2004

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Listers:

Looking for opinions, comments, pros & cons, etc. in comparing a Low
Vacuum-SEM with a tungsten gun vs a Lab6 gun.

Details: One of the primary applications presently is EBSD and XEDS of
geologic samples, of these one of the primary sample types is very fine
(nano) crystals ranging 10-100nm in size. And it is for these types of
samples we are strongly considering LAB6. Our thoughts are smaller spot
size and increased beam current, which will improve our diffraction signal, as
well improving our ability to locate the particles. Secondly, the scope will
primarily be operated by neophyte SEM users, users who are primarily
concerned with generating good EBSD and XEDS data not SEI/BEI imaging
(yeah, yeah but I don’t wish to open that discussion again).

So I am seeking comments: are the advantages of LAB6 real under these
conditions? How do these LAB6 advantages compare to the costs of
purchase and operation? And would a better recommendation be to spend
funds for other items like an “after-market” BSE detector (i.e. Robinson, etc.).

Thank you!

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 14:03:42 2004

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Dear MSA members,

I need some tips on EBSP sample prepration for a Zn alloy with additions on Bi and In that have concentrations of {0.3 wt.%. I wish to characterize these phases, which are {1 micron in size. TEM has not worked for me. The material is in powder form, but I have managed to compact them into disks for handling. I tried electropolishing with phosphoric acid and ethanol, and got good results for the Zn matrix (even got a Kikuchi pattern), but I was unable to get a pattern for the Bi-In phases. I believe that these are tarnishing. Can somebody recommend an EBSP sample prep method using mechanical polishing or ion etch? I have a Buehler Vibromet and a PIP tool that may help me. I am still open to electropolishing if anybody has any ideas. All prepared samples will be placed on an FESEM. All responses are greatly appreciated. Thank you! :o)

Martin Perez
Ph D student
University of Missouri-Rolla

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 14:23:48 2004

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Yes, folks I realize that across the board microscope vendors have moved
to concentrate on both W- or FEG scopes, with LaB6 left by the way side or
in the middle. And yes, FEG is the way to go - but with two caveats: (1) FEG
is $120-190K more than W- for every thing else the same, and (2) service
contracts are $17-20K more per year. So these are two BIG reasons to look
at LaB6.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 15:11:21 2004

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Coming from a physical sciences background, this is something that
has often puzzled me - apologies if I have missed something obvious.

When making measurements on regular biological structures, such as
muscle fibres, why not use diffraction?

The big advantage, it would seem to me, is that a single diffraction
pattern immediately and automatically gives average spacings over a
large number of individual fibres, something that would require
several images and a great deal of tedious measurement (almost
guaranteed to lead to errors).

In this case, couldn't 20 diffraction patterns (one from each sample)
give statistically better data than the 800 measurements from images?

Of course, there are disadvantages - you need a TEM capable of
operating at long camera lengths (although most, as far as I am
aware, can) and you need to calibrate the TEM for operation at such
camera lengths. Even so, I still think you would take less time and
the results would be statistically better.
--
Larry Stoter

NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 18:27:36 2004

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Most of the previous responders have made valid points, but many important
issues have been neglected. First you stated

"I have been asked to measure the width of 20 muscle fibers for each
specimen
and the diameter of 20 individual fibers on cross section in each group."

Do you mean that you need to measure the diameter of individual myofibrils
in addition to the diameter of the myofibers? And how do you intend to
measure the "diameter" or "width"? of these structures? Traditionally,
muscle fibers (in cross section) are measured by their "least diameter",
which can be defined as the distance between the closest parallel lines that
can be drawn around the fiber. This measurement is used because it is less
sensitive to error caused by poor orientation than other values, such as
area, circumference, or maximum diameter.

It will be much quicker and cost effective to measure the myofibers by light
microscopy. If myofibrils must also be measured, TEM will obviously be
required for those measurements. But for both types of measurements,
careful thought must be given to the sampling procedure as well as the total
number of structures measured. Because muscle fibers are more like
irregular polyhedrons than cylinders, even the least diameter statistic is
affected to some extent by orientation. Heart tissue is particularly
problematic because the fibers are not all parallel, and fascicles will be
seen in different orientation in the same section. When a muscle fiber
contracts, it's diameter increases. During fixation of muscle it is common
for some areas to become hyper contracted and other areas to become hyper
extended. Skeletal muscle is "stretched" during fixation with some kind of
clamping device to minimize this, but this is rarely done with heart. The
diameters of the fibers and fibrils will also be affected by the quality of
the fixation and the osmolarity of the fixative. You may well see variation
between areas on the surface of the sample versus those deeper in.

The upshot of this is that even if large numbers of fibers are measured from
each sample, the results will be meaningless unless the sampling procedure
is appropriate. There may well be greater variations between areas within
each sample than between the samples as a whole. You may need to do an
analysis of variance (ANOVA) looking at variation within an area of a
sample, between different areas of a sample, between samples with the same
treatment, and between treatments, in order to determine if there is a real
difference between the treatments. If you are trying to find subtle
differences, 800 measurements may not be nearly enough. Also, your
investigators may be interested in the distribution of fiber diameters (the
results are usually displayed as histograms), not just the means, and that
would require even larger numbers. If the samples are not well prepared and
handled identically, the project may be hopeless.

The good news is that the least diameter measurements are not difficult or
time consuming if you have an appropriate morphometry program. I routinely
measure 400-800 fibers per case for muscle biopsies, and that takes less
than 2 hours. If you do not have a morphometry package, NIH Image (for Mac)
and SCION Image (for Windows) are available as free downloads.

Ralph Common
Electron Microscopist
Michigan State University
Division of Human Pathology
A608 East Fee Hall
East Lansing, MI 48824
517-355-7558; fax 517-432-1053
ralph.common-at-ht.msu.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jan 26 22:49:34 2004

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Hello all:

I have two separate issues regarding 16-bit TIFF
files that I cannot get resolved. Perhaps someone
has run into one or both of these issues.

EDAX: The direct active image capture will go up
to 4096 or in my case, 8192 pixels at 1.33 aspect
ratio. However, the images are 8-bit. Well, the
image capture ADC is 12-bits...4096 shades. There
does not seem a way to capture an image as 16-bit
TIFF. Very frustrating. Is there some way around this?

LEO: The LEO32 GUI will save TIFF files as 16-bit
but the files are not readable on any system other
than the LEO SEM. The 8-bit files are standard TIFF.
The LEO ADC is also 12-bit. So why can't the 16-bit
TIFF be read by some other app? Photoshop will not
read it. ImageJ will not read it. Nothing I have will.

Any ideas?

tnx,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 00:00:13 2004

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If you are compressing the powders in to a pellet, there is a high risk
of plastically deforming phases enough to blur any pattern. In that
case, no prep technique will yield patterns.

John Mardinly
408-765-2346
877-277-1182

-----Original Message-----
} From: Perez, Martin Gerardo (UMR-Student) [mailto:mperez-at-umr.edu]
Sent: Monday, January 26, 2004 12:15 PM
To: Microscopy-at-MSA.Microscopy.Com

Dear MSA members,

I need some tips on EBSP sample prepration for a Zn alloy with additions
on Bi and In that have concentrations of {0.3 wt.%. I wish to
characterize these phases, which are {1 micron in size. TEM has not
worked for me. The material is in powder form, but I have managed to
compact them into disks for handling. I tried electropolishing with
phosphoric acid and ethanol, and got good results for the Zn matrix
(even got a Kikuchi pattern), but I was unable to get a pattern for the
Bi-In phases. I believe that these are tarnishing. Can somebody
recommend an EBSP sample prep method using mechanical polishing or ion
etch? I have a Buehler Vibromet and a PIP tool that may help me. I am
still open to electropolishing if anybody has any ideas. All prepared
samples will be placed on an FESEM. All responses are greatly
appreciated. Thank you! :o)

Martin Perez
Ph D student
University of Missouri-Rolla

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 02:18:25 2004

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*Subject: [Microscopy] Need help: EBSP sample prep
*Date sent: Mon, 26 Jan 2004 14:14:40 -0600
*From: "Perez, Martin Gerardo (UMR-Student)" {mperez-at-umr.edu}
*To: {Microscopy-at-MSA.Microscopy.Com}

*
*
*------------------------------------------------------------------------------
*The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hello:

Maybe it would be goog idea to check www.hkltechnology.com page.
There is a lot of useful information and papers too.

Good luck.

Best regards,

Witold Zielinski

*Dear MSA members,
*
*I need some tips on EBSP sample prepration for a Zn alloy with additions on Bi and In that have concentrations of {0.3 wt.%. I wish to characterize these phases, which are {1 micron in size. TEM ha

* not worked for me. The material is in powder form, but I have managed to compact them into disks for handling. I tried electropolishing with phosphoric acid and ethanol, and got good results for

*he Zn matrix (even got a Kikuchi pattern), but I was unable to get a pattern for the Bi-In phases. I believe that these are tarnishing. Can somebody recommend an EBSP sample prep method using mech

*nical polishing or ion etch? I have a Buehler Vibromet and a PIP tool that may help me. I am still open to electropolishing if anybody has any ideas. All prepared samples will be placed on an FESE

*. All responses are greatly appreciated. Thank you! :o)
*
*Martin Perez
*Ph D student
*University of Missouri-Rolla
*
*
*
:) :) :) :) :) :) :) :) :) :) :) :) :) :) :) :) ;)

Witold Zielinski, Ph.D.
Warsaw University of Technology
Department of Materials Science and Engineering
02-507 Warszawa, Woloska 141
POLAND

phone #: /48 22/ 660 87 07
660 87 36
fax #: /48 22/ 848 48 75

email: wiziel-at-inmat.pw.edu.pl

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 04:02:39 2004

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Hi

Back in sand free civilisation again after my trip to Egypt I note that not
one person took up my challenge to take a look at their laboratories
performance by way of www.iaaem.com/mppa1 .

We all seem to agree that the standards of EM output that we see in journals
have dropped. You may not agree with what the quality people have
developed, but you do
have to admit that we do not have, anywhere in the world, a standard by
which
EM units may be judged. Country by country the ISO/Quality procedures are
moving in. In time everyone will have to conform to some form of quality
standard, why not get ahead of the game?

In Australia the Quality movement is being spread country wide fast and
furious. Building on their theme of inter laboratory co-operation on
instrumentation they seem to be tackling the future of electron microscopy
with a very positive attitude Not all will survive, so they are making sure
everything is being done working together to set a very firm foundation for
their future.

On my travels it frightens me when I see how good some laboratories are and
how poor are some others. It is not the actual standard that really
concerns me, it is the perceived position of these laboratories within a
specific region. Are the perceived top laboratories really putting out the
best work, or do they just rely upon their reputation?

I hope this is worth a thought?

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob 07711 606967
www.emcourses.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 04:56:45 2004

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Hello Listers:

We got used Zeiss CEM902. After installation and initial switch on a
resistor in the Lens Current Unit(?) and a wired connection between resistor
and condenser in the Power Supply were burned out. To find out the reason(s)
we need Circuit Diagrams. I would be very pleased if anyone could send
theses about appropriate units.

Dr.Raivo Raid, PhD

Institute of Zoology&Hydrobiology
University of Tartu
Vanemuise 46
51014 Tartu
Estonia
Tel. +372 7 375840
Fax +372 7 375830

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 07:55:46 2004

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Martin,

It might be worthwhile to take a look at the following papers from a group
at the University in Saarbrucken in Germany. Both papers provide extensive
information on the optimal polishing of a wide range of materials.

1.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part I: Metals
Prakt. Metallogr. 38, 10, pp.547-565

2.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part II:
Ceramics Prakt. Metallogr. 39, 12, pp.644-662

Rene de Kloe
EDAX-TSL

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, 27 January, 2004 07:11
To: Perez, Martin Gerardo (UMR-Student); Microscopy-at-MSA.Microscopy.Com

Email: ecd10-at-psu.edu
Name: Prof. Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver: TEM Facility Manager Opening

Question: The Materials Research Institute at the Pennsylvania State University invites applications for a Transmission Electron Microscopist to oversee its TEM facilities. The facility supports a wide variety of materials research programs at Penn State. The Facility Manager will have primary responsibility for management and operation of the JEOL 2010F, JEOL 2010 LaB6 and Philips CM20 TEMs and auxiliary equipment, which reside in the facility. The Facility Manager will oversee training of PSU students, faculty and staff on TEM-related equipment and software and assist users with performing advanced microscopy techniques.

A MS is required with a PhD preferred in Materials, Physical Sciences or Engineering. The prospective candidate must have a strong background in the theory and practice of TEM microcharacterizaton with a minimum of 5 years post-graduate experience. The candidate should also have experience with vacuum technology, electronics, and computers. Strong interpersonal and communications skills are essential.

Interested candidates should send a resume and cover letter to Prof. Elizabeth Dickey, The Pennsylvania State University, 223 MRL Building, University Park, PA 16802. In addition, candidates should arrange to have three letters of recommendation sent to the above address.

Penn State is committed to affirmative action, equal opportunity and the diversity of its workforce.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 09:07:35 2004

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Gary;

Does the TIFF images that are saved in 16 bit format have a "TIF" extension or are they similar to a "composite" image as would be saved by PCI Quartz for example? I ask because PCI Quartz saves both the TIF image and the data that has annotations on it and can only be opened in that form by the PCI application.

Peter Tomic
Agere Systems

Peter
-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Tuesday, January 27, 2004 12:01 AM
To: MSA listserver

Hello all:

I have two separate issues regarding 16-bit TIFF
files that I cannot get resolved. Perhaps someone
has run into one or both of these issues.

EDAX: The direct active image capture will go up
to 4096 or in my case, 8192 pixels at 1.33 aspect
ratio. However, the images are 8-bit. Well, the
image capture ADC is 12-bits...4096 shades. There
does not seem a way to capture an image as 16-bit
TIFF. Very frustrating. Is there some way around this?

LEO: The LEO32 GUI will save TIFF files as 16-bit
but the files are not readable on any system other
than the LEO SEM. The 8-bit files are standard TIFF.
The LEO ADC is also 12-bit. So why can't the 16-bit
TIFF be read by some other app? Photoshop will not
read it. ImageJ will not read it. Nothing I have will.

Any ideas?

tnx,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 09:42:11 2004

Contents Retrieved from Microscopy Listserver Archives
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Steve Chapman wrote:

} Country by country the ISO/Quality procedures are
} moving in. In time everyone will have to conform to some form of quality
} standard ...

Yes, but my problem with ISO9000 and its ilk is that it is
much more concerned with documentation and reproducibility
than with what you and I would call quality. Reproducible
mediocrity, generated by a well-defined procedure, is just fine.
In fact, I might argue that your perceived decline in average
quality is CAUSED by the assumption that as long as it's ISO
compliant, it's good enough, so there's no point in investing
additional time to optimize. Cut-and-dried canned procedures
allow managers to use lower-level personnel.

Additionally, IMO, the documentation burden inhibits innovation
by encasing whatever you do now in concrete. That is certainly
true for small US manufacturers in conforming to CE requirements.
The cost of change is insignificant for a large consumer electronics
firm, but quite large for the smaller companies that largely serve
the microscopy field.

And who's to say that's not what the majority of the customer
base actually wants? Predictability over excellence or innovation?

Rick Mott

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 09:45:44 2004

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Hi All,

I have a Durst Enlarger with all accessories and a Ilford light source now.
I have a interested party, but have no idea as to what or how to price the
instrument?

Any suggestions would be helpful..

Eric
UCLA Medical Center
Electron Microscopy Lab

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 11:01:39 2004

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I put the same image as 8-bit and 16-bit
here:

www.microtechnics.com/leo_td_08.tif

www.microtechnics.com/leo_td_16.tif

These are as they came off of a Supra 55.
They are named tif by the system. Windows
TIFF reader does not like the 8-bit files
but Photoshop does. The 16-bit files come
out as grey snow--all garbaged bits. ImageJ
correctly reads the image frame size (1024x768)
and has a offset but it too can't read the image
file.

For 16-bit analySIS files, save as 16-bits and
do Image/Auto Level in Photoshop.

gary g.

At 07:18 AM 1/27/2004, you wrote:
} Gary;
}
} Does the TIFF images that are saved in 16 bit format have a "TIF"
} extension or are they similar to a "composite" image as would be saved by
} PCI Quartz for example? I ask because PCI Quartz saves both the TIF image
} and the data that has annotations on it and can only be opened in that
} form by the PCI application.
}
} Peter Tomic
} Agere Systems
}
} Peter
} -----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Tuesday, January 27, 2004 12:01 AM
} To: MSA listserver
} Subject: [Microscopy] EDAX and LEO 16-bit files
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 13:07:28 2004

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------------------------------------------------------------------------------
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Martin,

It might be worthwhile to take a look at the following papers from a group
at the University in Saarbrucken in Germany. Both papers provide extensive
information on the optimal polishing of a wide range of materials.

1.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part I: Metals
Prakt. Metallogr. 38, 10, pp.547-565

2.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part II:
Ceramics Prakt. Metallogr. 39, 12, pp.644-662

Rene de Kloe
EDAX-TSL

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, 27 January, 2004 07:11
To: Perez, Martin Gerardo (UMR-Student); Microscopy-at-MSA.Microscopy.Com

Gary:

The 16 bit image you posted does open correctly in Graphics Converter if you
tell it to swap the order of the bytes. When opened in Photoshop, what you are
apparently seeing is the low byte (essentially random values) first. That
suggests that the Leo folks set one of the (many) flags in the tif format wrong.
Tif is really a collection of possibilities rather than a well defined format.
There are so many combinations that not even Adobe, who is the caretaker of
the standard, opens all of the legal variants in programs like Photoshop. I've
seen someone's estimate that there are at least 160 combinations of legal
settings. If in addition to that, someone gets one of the flags wrong, there is no
limit to the confusion that can result. this time it looks like the fault is
Leo's but in general many companies use and abuse the tif format. Still, it's
better than something that is purely proprietary and undocumented.

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 13:18:15 2004

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------------------------------------------------------------------------------
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Email: ecd10-at-psu.edu
Name: Prof. Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver: TEM Facility Manager Opening

Question: The Materials Research Institute at the Pennsylvania State University invites applications for a Transmission Electron Microscopist to oversee its TEM facilities. The facility supports a wide variety of materials research programs at Penn State. The Facility Manager will have primary responsibility for management and operation of the JEOL 2010F, JEOL 2010 LaB6 and Philips CM20 TEMs and auxiliary equipment, which reside in the facility. The Facility Manager will oversee training of PSU students, faculty and staff on TEM-related equipment and software and assist users with performing advanced microscopy techniques.

A MS is required with a PhD preferred in Materials, Physical Sciences or Engineering. The prospective candidate must have a strong background in the theory and practice of TEM microcharacterizaton with a minimum of 5 years post-graduate experience. The candidate should also have experience with vacuum technology, electronics, and computers. Strong interpersonal and communications skills are essential.

Interested candidates should send a resume and cover letter to Prof. Elizabeth Dickey, The Pennsylvania State University, 223 MRL Building, University Park, PA 16802. In addition, candidates should arrange to have three letters of recommendation sent to the above address.

Penn State is committed to affirmative action, equal opportunity and the diversity of its workforce.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 13:34:56 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Email: ecd10-at-psu.edu
Name: Prof. Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver: TEM Facility Manager Opening

Question: The Materials Research Institute at the Pennsylvania State University invites applications for a Transmission Electron Microscopist to oversee its TEM facilities. The facility supports a wide variety of materials research programs at Penn State. The Facility Manager will have primary responsibility for management and operation of the JEOL 2010F, JEOL 2010 LaB6 and Philips CM20 TEMs and auxiliary equipment, which reside in the facility. The Facility Manager will oversee training of PSU students, faculty and staff on TEM-related equipment and software and assist users with performing advanced microscopy techniques.

A MS is required with a PhD preferred in Materials, Physical Sciences or Engineering. The prospective candidate must have a strong background in the theory and practice of TEM microcharacterizaton with a minimum of 5 years post-graduate experience. The candidate should also have experience with vacuum technology, electronics, and computers. Strong interpersonal and communications skills are essential.

Interested candidates should send a resume and cover letter to Prof. Elizabeth Dickey, The Pennsylvania State University, 223 MRL Building, University Park, PA 16802. In addition, candidates should arrange to have three letters of recommendation sent to the above address.

Penn State is committed to affirmative action, equal opportunity and the diversity of its workforce.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 13:42:30 2004

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Gary;

Does the TIFF images that are saved in 16 bit format have a "TIF" extension or are they similar to a "composite" image as would be saved by PCI Quartz for example? I ask because PCI Quartz saves both the TIF image and the data that has annotations on it and can only be opened in that form by the PCI application.

Peter Tomic
Agere Systems

Peter
-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Tuesday, January 27, 2004 12:01 AM
To: MSA listserver

Hello all:

I have two separate issues regarding 16-bit TIFF
files that I cannot get resolved. Perhaps someone
has run into one or both of these issues.

EDAX: The direct active image capture will go up
to 4096 or in my case, 8192 pixels at 1.33 aspect
ratio. However, the images are 8-bit. Well, the
image capture ADC is 12-bits...4096 shades. There
does not seem a way to capture an image as 16-bit
TIFF. Very frustrating. Is there some way around this?

LEO: The LEO32 GUI will save TIFF files as 16-bit
but the files are not readable on any system other
than the LEO SEM. The 8-bit files are standard TIFF.
The LEO ADC is also 12-bit. So why can't the 16-bit
TIFF be read by some other app? Photoshop will not
read it. ImageJ will not read it. Nothing I have will.

Any ideas?

tnx,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 15:09:10 2004

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Email: marc.walton-at-lacma.org
Name: Marc Walton

Organization: Los Angeles County Museum

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for a firm to service the Los Angeles County Museum's Cambridge Stereoscan 200 SEM. We are looking for a someone to assess the health of the instrument, to provide recommendations for upgrades, and then to possibly provide ongoing emergency service. Could anyone recommend such a company?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 15:39:10 2004

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Hello Listers:

We got used Zeiss CEM902. After installation and initial switch on a
resistor in the Lens Current Unit(?) and a wired connection between resistor
and condenser in the Power Supply were burned out. To find out the reason(s)
we need Circuit Diagrams. I would be very pleased if anyone could send
theses about appropriate units.

Dr.Raivo Raid, PhD

Institute of Zoology&Hydrobiology
University of Tartu
Vanemuise 46
51014 Tartu
Estonia
Tel. +372 7 375840
Fax +372 7 375830

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 15:59:17 2004

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Steve Chapman wrote:

} Country by country the ISO/Quality procedures are
} moving in. In time everyone will have to conform to some form of quality
} standard ...

Yes, but my problem with ISO9000 and its ilk is that it is
much more concerned with documentation and reproducibility
than with what you and I would call quality. Reproducible
mediocrity, generated by a well-defined procedure, is just fine.
In fact, I might argue that your perceived decline in average
quality is CAUSED by the assumption that as long as it's ISO
compliant, it's good enough, so there's no point in investing
additional time to optimize. Cut-and-dried canned procedures
allow managers to use lower-level personnel.

Additionally, IMO, the documentation burden inhibits innovation
by encasing whatever you do now in concrete. That is certainly
true for small US manufacturers in conforming to CE requirements.
The cost of change is insignificant for a large consumer electronics
firm, but quite large for the smaller companies that largely serve
the microscopy field.

And who's to say that's not what the majority of the customer
base actually wants? Predictability over excellence or innovation?

Rick Mott

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 16:32:58 2004

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I have used horseradish peroxidase as a tracer in vivo in the past and am
aware that it can damage cells and cross membranes with prolonged
exposure. I am now trying to find a reference that demonstrates this
fact. A literature search using Medline is difficult on this topic since
it is hard to come up with a good Boolean logic search of keywords (this is
one of two problems that I am posting that I am having a difficult time
searching the literature for). Any citations would be greatly
appreciated. TIA, tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 16:35:05 2004

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I know this is a longshot but has anyone ever seen a paper where someone
looked at a sample by SEM and then embedded the sample and looked at the
exact same cells by TEM? A literature search using Medline is difficult
on this topic since it is hard to come up with a good Boolean logic search
of keywords that doesn't pull up 1000's of non-relevant TEM & SEM
papers. (this is one of two problems that I am posting that I am having a
difficult time searching the literature for). Any citations would be
greatly appreciated. TIA, tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jan 27 20:04:06 2004

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Hi Thomas

I did quite a bit of this sort of work many years ago. Works quite
well although the organelle ultrastructure does suffer a little.
Don't expect the same clarity of membranes as a specimen processed
directly for TEM.

The text 'Principles and Techniques of Scanning Electron Microscopy'
by Hayat, has a chapter outlining the method. Chapter 5 written by
M.Gary Wickham and David M. Worthen.

Also Chaptr 11 written by Willis K. Paul.

In our library this text had the code QH 212.53. If you wish I could
check whether our library still has this book for an ISBN number. We
are talking 1974 edition.

Other references at the time,

Anat Rec (1973) Vol 176, pp 245-252. Samuel M. Meller, et al.
Transmission electron microscopy of critical point dried tissue after
observation in the scanning electron microscope.

Cell Tissue Research Vol 162 pp 61-73 (1975) D.E. Scott, et al. The
Primate Median Eminence. Correlative scanning transmission electron
microscopy.

Cell Tissue Research Vol 190 pp 317-336 (1978) D.E. Scott, et al.
Coorelative Scanning-Transmission EM Examination of the Perinatal rat
brain.

Human Reproduction (1991), Vol 6 pp 645-660, and Human Reproduction
(1992), Vol 7, pp 446 - 452. W.R. Gillet et al, Both to do with
human ovary, examined in SEM then same sample examined in TEM.

At the time we played around with doing SEM on blocks that had
ultrathins cut from them. Worked really well also.

Hope this gets you started

Allan

}
} I know this is a longshot but has anyone ever seen a paper where
} someone looked at a sample by SEM and then embedded the sample and
} looked at the exact same cells by TEM? A literature search using
} Medline is difficult on this topic since it is hard to come up with
} a good Boolean logic search of keywords that doesn't pull up 1000's
} of non-relevant TEM & SEM papers. (this is one of two problems that
} I am posting that I am having a difficult time searching the
} literature for). Any citations would be greatly appreciated. TIA,
} tom
}
} Thomas E. Phillips, PhD
--
-------------------------------------------------
Allan Mitchell
Technical Manager
Otago Centre for Electron Microscopy
C/-Department of Anatomy and Structural Biology
School of Medical Sciences
P.O. Box 913
Dunedin
New Zealand

-----------------------------------------------------------------
2005 Microscopy Conference in Dunedin:
http://ocem.otago.ac.nz/Conference_2005/Microscopy_NZ_2005.html

-----------------------------------------------------------------

Phone (03) 479 5642 or 479 7301
Fax (03) 479 7254

EM Centre: http://ocem.otago.ac.nz/
Confocal Centre: http://occm.otago.ac.nz/
Department: http://anatomy.otago.ac.nz/

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 00:39:45 2004

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Martin,

It might be worthwhile to take a look at the following papers from a group
at the University in Saarbrucken in Germany. Both papers provide extensive
information on the optimal polishing of a wide range of materials.

1.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part I: Metals
Prakt. Metallogr. 38, 10, pp.547-565

2.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part II:
Ceramics Prakt. Metallogr. 39, 12, pp.644-662

Rene de Kloe
EDAX-TSL

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, 27 January, 2004 07:11
To: Perez, Martin Gerardo (UMR-Student); Microscopy-at-MSA.Microscopy.Com

Search for Gareth Griffiths, he has done a lot of HRP experiments as I know
Good luck
daničle

--------------------------------------------
Daničle Spehner, INSERM EPI 99-08 - EFS-Alsace
10 rue Spielmann - 67065 STRASBOURG
tel : 03 88 21 25 25 - fax : 03 88 21 25 44
e-mail : daniele.spehner-at-efs-alsace.fr
------------------------------------

-----Message d'origine-----
De : Tom Phillips [mailto:phillipst-at-missouri.edu]
Envoyé : mardi 27 janvier 2004 23:45
Ŕ : Microscopy-at-msa.microscopy.com
Objet : HRP damage to membranes in vivo

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I have used horseradish peroxidase as a tracer in vivo in the past and am
aware that it can damage cells and cross membranes with prolonged
exposure. I am now trying to find a reference that demonstrates this
fact. A literature search using Medline is difficult on this topic since
it is hard to come up with a good Boolean logic search of keywords (this is
one of two problems that I am posting that I am having a difficult time
searching the literature for). Any citations would be greatly
appreciated. TIA, tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 04:28:22 2004

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Hi everybody!
My University have received some money to buy an ion milling (with a
dimple grinder, a disc puncher, a disc grinder etc) to prepare samples
for TEM. I have to decide between Gatan and Fischione. I would
appreciate very much any opinion about these two companies because I
have to make a decision as soon as possible.
Thank you very much
Cristina Almansa
University of Alicante, Spain

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 04:38:41 2004

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Hi everybody!
My University have received some money to buy an ion milling (with a
dimple grinder, a disc puncher, a disc grinder etc) to prepare samples
for TEM. I have to decide between Gatan and Fischione. I would
appreciate very much any opinion about these two companies because I
have to make a decision as soon as possible.
Thank you very much
Cristina Almansa
University of Alicante, Spain

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 05:35:15 2004

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Martin,

It might be worthwhile to take a look at the following papers from a group
at the University in Saarbrucken in Germany. Both papers provide extensive
information on the optimal polishing of a wide range of materials.

1.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part I: Metals
Prakt. Metallogr. 38, 10, pp.547-565

2.
Katrakova, D., Mücklich, F.(2001)
Specimen Preparation for Electron Backscatter Diffraction - Part II:
Ceramics Prakt. Metallogr. 39, 12, pp.644-662

Rene de Kloe
EDAX-TSL

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, 27 January, 2004 07:11
To: Perez, Martin Gerardo (UMR-Student); Microscopy-at-MSA.Microscopy.Com

I sent the image that Gary posted to Chris Cox at Adobe. Adobe is the
caretaker of the TIFF standard and Chris is the person who is directly in charge of
the Photoshop code that reads and writes files. His reply is below. Somebody
needs to tell LEO to correct their file writing routine!

} From: Chris Cox {ccox-at-adobe.com}
} Date: January 27, 2004 10:18:56 PM EST
}
} The file in question is little endian, 16 bit/sample, 1 sample,
} uncompressed, black is zero photometric interpretation.
}
} As far as I can tell, Photoshop is reading the image 100% correctly.
}
} BUT - the file is written incorrectly.
} They handled the byte order on the tags, but failed to handle the byte
} order on the image data.
} If I change the byte order info halfway through the decode process in
} Photoshop, we read the image correctly (SEM image of what looks like a
} semiconductor wafer surface showing one trace and one partial trace
} plus some pits).
}
} So, it's up to whomever wrote this file to fix their TIFF writing code.
} I can't believe they'd make such a novice mistake.

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 06:51:40 2004

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I put the same image as 8-bit and 16-bit
here:

www.microtechnics.com/leo_td_08.tif

www.microtechnics.com/leo_td_16.tif

These are as they came off of a Supra 55.
They are named tif by the system. Windows
TIFF reader does not like the 8-bit files
but Photoshop does. The 16-bit files come
out as grey snow--all garbaged bits. ImageJ
correctly reads the image frame size (1024x768)
and has a offset but it too can't read the image
file.

For 16-bit analySIS files, save as 16-bits and
do Image/Auto Level in Photoshop.

gary g.

At 07:18 AM 1/27/2004, you wrote:
} Gary;
}
} Does the TIFF images that are saved in 16 bit format have a "TIF"
} extension or are they similar to a "composite" image as would be saved by
} PCI Quartz for example? I ask because PCI Quartz saves both the TIF image
} and the data that has annotations on it and can only be opened in that
} form by the PCI application.
}
} Peter Tomic
} Agere Systems
}
} Peter
} -----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Tuesday, January 27, 2004 12:01 AM
} To: MSA listserver
} Subject: [Microscopy] EDAX and LEO 16-bit files
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 06:53:30 2004

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Email: marc.walton-at-lacma.org
Name: Marc Walton

Organization: Los Angeles County Museum

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for a firm to service the Los Angeles County Museum's Cambridge Stereoscan 200 SEM. We are looking for a someone to assess the health of the instrument, to provide recommendations for upgrades, and then to possibly provide ongoing emergency service. Could anyone recommend such a company?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 07:06:56 2004

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Email: ecd10-at-psu.edu
Name: Prof. Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver: TEM Facility Manager Opening

Question: The Materials Research Institute at the Pennsylvania State University invites applications for a Transmission Electron Microscopist to oversee its TEM facilities. The facility supports a wide variety of materials research programs at Penn State. The Facility Manager will have primary responsibility for management and operation of the JEOL 2010F, JEOL 2010 LaB6 and Philips CM20 TEMs and auxiliary equipment, which reside in the facility. The Facility Manager will oversee training of PSU students, faculty and staff on TEM-related equipment and software and assist users with performing advanced microscopy techniques.

A MS is required with a PhD preferred in Materials, Physical Sciences or Engineering. The prospective candidate must have a strong background in the theory and practice of TEM microcharacterizaton with a minimum of 5 years post-graduate experience. The candidate should also have experience with vacuum technology, electronics, and computers. Strong interpersonal and communications skills are essential.

Interested candidates should send a resume and cover letter to Prof. Elizabeth Dickey, The Pennsylvania State University, 223 MRL Building, University Park, PA 16802. In addition, candidates should arrange to have three letters of recommendation sent to the above address.

Penn State is committed to affirmative action, equal opportunity and the diversity of its workforce.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 07:37:13 2004

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Email: ecd10-at-psu.edu
Name: Prof. Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver: TEM Facility Manager Opening

Question: The Materials Research Institute at the Pennsylvania State University invites applications for a Transmission Electron Microscopist to oversee its TEM facilities. The facility supports a wide variety of materials research programs at Penn State. The Facility Manager will have primary responsibility for management and operation of the JEOL 2010F, JEOL 2010 LaB6 and Philips CM20 TEMs and auxiliary equipment, which reside in the facility. The Facility Manager will oversee training of PSU students, faculty and staff on TEM-related equipment and software and assist users with performing advanced microscopy techniques.

A MS is required with a PhD preferred in Materials, Physical Sciences or Engineering. The prospective candidate must have a strong background in the theory and practice of TEM microcharacterizaton with a minimum of 5 years post-graduate experience. The candidate should also have experience with vacuum technology, electronics, and computers. Strong interpersonal and communications skills are essential.

Interested candidates should send a resume and cover letter to Prof. Elizabeth Dickey, The Pennsylvania State University, 223 MRL Building, University Park, PA 16802. In addition, candidates should arrange to have three letters of recommendation sent to the above address.

Penn State is committed to affirmative action, equal opportunity and the diversity of its workforce.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 08:08:10 2004

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Dear Microscopists,

I have been discussing with various people the the use of the following
words

dye
stain
label
marker

The problem has been the use of the word "label". There exists two opinion
about the proper use of it. The one states strictly that a label has always
to be coupled to the target with antibody-antigen reaction. The other school
states that a label is generally a molecule or an atom or a bead etc that
makes the target visible in an instrument (eg. a microscope). So plese
someone, give me an explanation what exactly is a "label" ?

Thank you.

Regards
Ari Kuusisto
Research physicist

PerkinElmer Life and Analytical Sciences
tel. +358-2-2678 508
fax. +358-2-2578 357
E-mail: Ari.Kuusisto-at-PerkinElmer.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 08:30:14 2004

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Email: marc.walton-at-lacma.org
Name: Marc Walton

Organization: Los Angeles County Museum

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for a firm to service the Los Angeles County Museum's Cambridge Stereoscan 200 SEM. We are looking for a someone to assess the health of the instrument, to provide recommendations for upgrades, and then to possibly provide ongoing emergency service. Could anyone recommend such a company?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 08:56:06 2004

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I sent the image that Gary posted to Chris Cox at Adobe. Adobe is the
caretaker of the TIFF standard and Chris is the person who is directly in charge of
the Photoshop code that reads and writes files. His reply is below. Somebody
needs to tell LEO to correct their file writing routine!

} From: Chris Cox {ccox-at-adobe.com}
} Date: January 27, 2004 10:18:56 PM EST
}
} The file in question is little endian, 16 bit/sample, 1 sample,
} uncompressed, black is zero photometric interpretation.
}
} As far as I can tell, Photoshop is reading the image 100% correctly.
}
} BUT - the file is written incorrectly.
} They handled the byte order on the tags, but failed to handle the byte
} order on the image data.
} If I change the byte order info halfway through the decode process in
} Photoshop, we read the image correctly (SEM image of what looks like a
} semiconductor wafer surface showing one trace and one partial trace
} plus some pits).
}
} So, it's up to whomever wrote this file to fix their TIFF writing code.
} I can't believe they'd make such a novice mistake.

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 12:52:43 2004

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On Jan 28, 2004, at 6:18 AM, Kuusisto, Ari wrote:

} I have been discussing with various people the the use of the following
} words
}
} dye
} stain
} label
} marker
}
} The problem has been the use of the word "label". There exists two
} opinion
} about the proper use of it. The one states strictly that a label has
} always
} to be coupled to the target with antibody-antigen reaction. The other
} school
} states that a label is generally a molecule or an atom or a bead etc
} that
} makes the target visible in an instrument (eg. a microscope). So plese
} someone, give me an explanation what exactly is a "label" ?

Dear Ari,
I would define a dye as a substance that imparts color to a substrate.
It need not be specific, so the color could be uniform, such as hair
or cloth dyes. A stain is a substance that imparts visibility to a
substrate, and in the context of microscopy a stain has some
specificity. For LM a stain generally imparts color (i.e., is a type
of dye), and for EM a stain is a stronger scatterer of electrons than
is the substrate. A marker is a substance that adds a recognizable
feature to a substrate. Finally, a label is a marker that is
associated with a particular component of the substrate. Thus, there
are fluorescent dyes that are lipophyllic, so these can be used as
labels for membranes, there are molecules that bind very specifically,
including biotin-avidin, so including but not restricted to
antibody-antigen pairs. These can be bound to markers, such as green
fluorescent protein or colloidal gold, and I call these labels.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 13:20:24 2004

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Colleagues

Yes, I see the duplicate messages I am attempting to sort out why it started
it may have to do with the virus attack which is going on in the USA right now.

Unfortunately, I am on the road on the way to the Australian meeting. This
may take me some time to fix as my connectivity will be intermittent.

Nestor
Your Friendly Neighborhood SysOp.

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 13:27:03 2004

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Dear Microscopists,

I have been discussing with various people the the use of the following
words

dye
stain
label
marker

The problem has been the use of the word "label". There exists two opinion
about the proper use of it. The one states strictly that a label has always
to be coupled to the target with antibody-antigen reaction. The other school
states that a label is generally a molecule or an atom or a bead etc that
makes the target visible in an instrument (eg. a microscope). So plese
someone, give me an explanation what exactly is a "label" ?

Thank you.

Regards
Ari Kuusisto
Research physicist

PerkinElmer Life and Analytical Sciences
tel. +358-2-2678 508
fax. +358-2-2578 357
E-mail: Ari.Kuusisto-at-PerkinElmer.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 14:12:26 2004

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From ESL point of view:
marker is something which left "mark". So, it's tool to make "marks".
Labels usually used to "label" something. So, you may "label" something to
make it recognizable from something else... I would think that label is
something, which someone used to mark some particular stuff. Therefore,
antibody may be a label. Gold particle or fluorochrome may be a label. In
general, I like second definition better. Sergey

At 06:18 AM 1/28/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 14:35:27 2004

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Nice definition, Bill.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Wednesday, January 28, 2004 2:05 PM
To: microscopy-at-msa.microscopy.com

On Jan 28, 2004, at 6:18 AM, Kuusisto, Ari wrote:

} I have been discussing with various people the the use of the following
} words
}
} dye
} stain
} label
} marker
}
} The problem has been the use of the word "label". There exists two
} opinion
} about the proper use of it. The one states strictly that a label has
} always
} to be coupled to the target with antibody-antigen reaction. The other
} school
} states that a label is generally a molecule or an atom or a bead etc
} that
} makes the target visible in an instrument (eg. a microscope). So plese
} someone, give me an explanation what exactly is a "label" ?

Dear Ari,
I would define a dye as a substance that imparts color to a substrate.
It need not be specific, so the color could be uniform, such as hair
or cloth dyes. A stain is a substance that imparts visibility to a
substrate, and in the context of microscopy a stain has some
specificity. For LM a stain generally imparts color (i.e., is a type
of dye), and for EM a stain is a stronger scatterer of electrons than
is the substrate. A marker is a substance that adds a recognizable
feature to a substrate. Finally, a label is a marker that is
associated with a particular component of the substrate. Thus, there
are fluorescent dyes that are lipophyllic, so these can be used as
labels for membranes, there are molecules that bind very specifically,
including biotin-avidin, so including but not restricted to
antibody-antigen pairs. These can be bound to markers, such as green
fluorescent protein or colloidal gold, and I call these labels.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 15:00:10 2004

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------------------------------------------------------------------------------
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From ESL point of view:
marker is something which left "mark". So, it's tool to make "marks".
Labels usually used to "label" something. So, you may "label" something to
make it recognizable from something else... I would think that label is
something, which someone used to mark some particular stuff. Therefore,
antibody may be a label. Gold particle or fluorochrome may be a label. In
general, I like second definition better. Sergey

At 06:18 AM 1/28/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 16:39:20 2004

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I am looking for some colleagues who are using:

Oxford INCA energy 400 w/Feature

To start up a users group.

Please respond off the list to me personally, and I will share a list
with all respondents, who wish to be shared, within the next two weeks.

Thanks all,

Fred Monson

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/
Directions
http://www.wcupa.edu/_admissions/sch_adm/directs.htm
West Chester Boro
http://www.west-chester.com/
Places to stay
http://www.hotels-motels-n-more.com/PA/West-Chester.html

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 17:08:52 2004

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Nice definition, Bill.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Wednesday, January 28, 2004 2:05 PM
To: microscopy-at-msa.microscopy.com

On Jan 28, 2004, at 6:18 AM, Kuusisto, Ari wrote:

} I have been discussing with various people the the use of the following
} words
}
} dye
} stain
} label
} marker
}
} The problem has been the use of the word "label". There exists two
} opinion
} about the proper use of it. The one states strictly that a label has
} always
} to be coupled to the target with antibody-antigen reaction. The other
} school
} states that a label is generally a molecule or an atom or a bead etc
} that
} makes the target visible in an instrument (eg. a microscope). So plese
} someone, give me an explanation what exactly is a "label" ?

Dear Ari,
I would define a dye as a substance that imparts color to a substrate.
It need not be specific, so the color could be uniform, such as hair
or cloth dyes. A stain is a substance that imparts visibility to a
substrate, and in the context of microscopy a stain has some
specificity. For LM a stain generally imparts color (i.e., is a type
of dye), and for EM a stain is a stronger scatterer of electrons than
is the substrate. A marker is a substance that adds a recognizable
feature to a substrate. Finally, a label is a marker that is
associated with a particular component of the substrate. Thus, there
are fluorescent dyes that are lipophyllic, so these can be used as
labels for membranes, there are molecules that bind very specifically,
including biotin-avidin, so including but not restricted to
antibody-antigen pairs. These can be bound to markers, such as green
fluorescent protein or colloidal gold, and I call these labels.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 17:33:15 2004

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On Jan 28, 2004, at 6:18 AM, Kuusisto, Ari wrote:

} I have been discussing with various people the the use of the following
} words
}
} dye
} stain
} label
} marker
}
} The problem has been the use of the word "label". There exists two
} opinion
} about the proper use of it. The one states strictly that a label has
} always
} to be coupled to the target with antibody-antigen reaction. The other
} school
} states that a label is generally a molecule or an atom or a bead etc
} that
} makes the target visible in an instrument (eg. a microscope). So plese
} someone, give me an explanation what exactly is a "label" ?

Dear Ari,
I would define a dye as a substance that imparts color to a substrate.
It need not be specific, so the color could be uniform, such as hair
or cloth dyes. A stain is a substance that imparts visibility to a
substrate, and in the context of microscopy a stain has some
specificity. For LM a stain generally imparts color (i.e., is a type
of dye), and for EM a stain is a stronger scatterer of electrons than
is the substrate. A marker is a substance that adds a recognizable
feature to a substrate. Finally, a label is a marker that is
associated with a particular component of the substrate. Thus, there
are fluorescent dyes that are lipophyllic, so these can be used as
labels for membranes, there are molecules that bind very specifically,
including biotin-avidin, so including but not restricted to
antibody-antigen pairs. These can be bound to markers, such as green
fluorescent protein or colloidal gold, and I call these labels.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 17:47:00 2004

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------------------------------------------------------------------------------
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Dear Microscopists,

I have been discussing with various people the the use of the following
words

dye
stain
label
marker

The problem has been the use of the word "label". There exists two opinion
about the proper use of it. The one states strictly that a label has always
to be coupled to the target with antibody-antigen reaction. The other school
states that a label is generally a molecule or an atom or a bead etc that
makes the target visible in an instrument (eg. a microscope). So plese
someone, give me an explanation what exactly is a "label" ?

Thank you.

Regards
Ari Kuusisto
Research physicist

PerkinElmer Life and Analytical Sciences
tel. +358-2-2678 508
fax. +358-2-2578 357
E-mail: Ari.Kuusisto-at-PerkinElmer.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jan 28 22:59:11 2004

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Colleagues...

I see that the messages look like they are
being replicated by an EMail pickup service based in Europe.

I'm trying to block this, but I will be offline for the next ~ 24+ hours
so I'll not be able to do anything to track success or failure until
I surface.

If the block does not cure the duplicates please bear with it until I can
get back on-line and investigate further.

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 00:50:57 2004

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Hi

I would use the word label as being that which allows us to see the
substance that we have probed the tissue for. In
immunohisto/cytochemistry/fluorescence it would be the fluorochrome (eg
FITC), enzyme (eg peroxidase) or a gold particle in immuno-EM.

For me 'marker' is a marker of disease - that is the antigen we are looking
for that tells us the lineage of the cells we see etc.
Med vänliga hälsningar/With best regards

Gareth

***Come to Stockholm in 2004 to the 26th IFBLS congress*** Take a look at
http://www.vardforbundet.se/ifbls2004

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 05:20:24 2004

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To,
MSA LIST Members,
Would like to get performance feedback, from any of
the list members, on the following L.Microscopy sample
preparation Machines of diffrent make,for a technical
review.

1)Precision Diamond sectioning m/c.
Models:-
ISOMET(Buehlers)
VC-50 (Leco)
Metacut-DCM (Metatech)
Diamiond Saw(Geologist Syndicate)
2)Heavy duty abrasive Saw.
Models:-
Lapro Slab Saw(Buehlers)
MSX-250A dual sectioning m/C(Leco)
Metacut 50 (Metatech)
Speciment cut off M/c(Geologist Syndicate)
Thanks 7Regards,
J.J.D'Mello.
ACC LTD,
RCD,Thane India.

__________________________________
Do you Yahoo!?
Yahoo! SiteBuilder - Free web site building tool. Try it!
http://webhosting.yahoo.com/ps/sb/

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 09:18:57 2004

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Here's how we, cell biologists, usually define these terms:
- Dye: substance that adds color at light microscopy level.
- Stain: substance that adds contrast for the EM. Has some
specificity for some cellular components, but is overall
non-specific as it does not differentiate between different
protein species, for example.
- Label: something used to localize specific cell components
(proteins usually, but also lipids and carbohydrates). Usually
antibodies followed by fluorescent probes or gold conjugates,
but can also refer to histo-cytochemistry.
- Marker: labels that are known to be specific for a given
organelle/cell. For example: catalase is used as a
peroxysome marker, calnexin as an ER marker, etc...

As you can see, each discipline uses its own definitions,
so it would be very hard to normalize these and come up
with a set of definitions that work for everyone. The important
thing is to use the terminology that is generally accepted
within your own discipline, so that other people understand
your work and you can understand theirs!!
Best

Marc

On Wednesday, January 28, 2004, at 09:18 AM, Kuusisto, Ari wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Dear Microscopists,
}
} I have been discussing with various people the the use of the following
} words
}
} dye
} stain
} label
} marker
}
} The problem has been the use of the word "label". There exists two
} opinion
} about the proper use of it. The one states strictly that a label has
} always
} to be coupled to the target with antibody-antigen reaction. The other
} school
} states that a label is generally a molecule or an atom or a bead etc
} that
} makes the target visible in an instrument (eg. a microscope). So plese
} someone, give me an explanation what exactly is a "label" ?
}
} Thank you.
}
}
} Regards
} Ari Kuusisto
} Research physicist
}
} PerkinElmer Life and Analytical Sciences
} tel. +358-2-2678 508
} fax. +358-2-2578 357
} E-mail: Ari.Kuusisto-at-PerkinElmer.com
}
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 09:46:13 2004

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We use Gill's.

Kathleen
Principal Lab Technician
Neurotoxicology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

mark.lewis-at-thermo.com wrote:

} Hello everyone !
}
} I'm taking a survey to find out which type of Hematoxylin is most commonly
} used in Histology and Cytology labs.
}
} Thanks !
}
} Best regards,
}
} Mark
}
} Mark Lewis
} Product Specialist
} Anatomical Pathology
} Clinical Diagnostics
} Thermo Electron Corporation
} (412) 747-4013
} (412) 788-1097
} E-mail: mark.lewis-at-thermo.com
}
}
}
}
} _______________________________________________
} Histonet mailing list
} Histonet-at-lists.utsouthwestern.edu
} http://lists.utsouthwestern.edu/mailman/listinfo/histonet
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 10:52:44 2004

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Good Afternoon Everyone,

Free to a good home:
An original Tracor Northern 5500 EDS Computer System Console (without the EDS detector). It was fully functional and working when taken out of service in 2000. You may find it useful for parts or for use if matched up to a detector. The recipient has to arrange for pickup or shipping, but we would be able to get it onto a pallet for you.

Please contact me off-list if you are interested,

Best Regards,
~Jon Dunlap

Jonathan Dunlap
Analytical Laboratory Manager
Osram Sylvania Products Inc.
Precision Materials and Components
816 Lexington Avenue
Warren, PA 16365
Ph: 814-726-6991
Fax: 814-726-6942

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 11:00:31 2004

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On Jan 29, 2004, at 7:29 AM, Marc Pypaert wrote:

Dear Mark,

} Here's how we, cell biologists, usually define these terms:
} - Dye: substance that adds color at light microscopy level.
} - Stain: substance that adds contrast for the EM. Has some
} specificity for some cellular components, but is overall
} non-specific as it does not differentiate between different
} protein species, for example.

There are also the classics, such as Gram stain, etc., that are LM
stains.

} - Label: something used to localize specific cell components
} (proteins usually, but also lipids and carbohydrates). Usually
} antibodies followed by fluorescent probes or gold conjugates,
} but can also refer to histo-cytochemistry.
} - Marker: labels that are known to be specific for a given
} organelle/cell. For example: catalase is used as a
} peroxysome marker, calnexin as an ER marker, etc...

Also colloidal gold used as a fiducial marker in tomography.
}
} As you can see, each discipline uses its own definitions,
} so it would be very hard to normalize these and come up
} with a set of definitions that work for everyone. The important
} thing is to use the terminology that is generally accepted
} within your own discipline, so that other people understand
} your work and you can understand theirs!!
}
Agreed.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 11:02:07 2004

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hello, everyone,
who has Nanoscope IV Controller manual (Revision B, Software Version
5.12r3)?
Can you send me a PDF format of this manual?
I have a manual for Nanoscope IIIa and cannot get a surface potential
imaging according to its instructions.
Since the controller has been upgraded to IV, I want to have a look at the
new manual to see what's the differences.

Thanks.

Minjun

Dept. of Electrical Engineering
Univ. of Notre Dame
574-631-4916

----- Original Message -----
} From: "JUDE Dmello" {j_dmello-at-yahoo.com}
To: "MicroscopyListserver" {microscopy-at-msa.microscopy.com}
Sent: Thursday, January 29, 2004 6:31 AM

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Here's how we, cell biologists, usually define these terms:
- Dye: substance that adds color at light microscopy level.
- Stain: substance that adds contrast for the EM. Has some
specificity for some cellular components, but is overall
non-specific as it does not differentiate between different
protein species, for example.
- Label: something used to localize specific cell components
(proteins usually, but also lipids and carbohydrates). Usually
antibodies followed by fluorescent probes or gold conjugates,
but can also refer to histo-cytochemistry.
- Marker: labels that are known to be specific for a given
organelle/cell. For example: catalase is used as a
peroxysome marker, calnexin as an ER marker, etc...

As you can see, each discipline uses its own definitions,
so it would be very hard to normalize these and come up
with a set of definitions that work for everyone. The important
thing is to use the terminology that is generally accepted
within your own discipline, so that other people understand
your work and you can understand theirs!!
Best

Marc

On Wednesday, January 28, 2004, at 09:18 AM, Kuusisto, Ari wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Dear Microscopists,
}
} I have been discussing with various people the the use of the following
} words
}
} dye
} stain
} label
} marker
}
} The problem has been the use of the word "label". There exists two
} opinion
} about the proper use of it. The one states strictly that a label has
} always
} to be coupled to the target with antibody-antigen reaction. The other
} school
} states that a label is generally a molecule or an atom or a bead etc
} that
} makes the target visible in an instrument (eg. a microscope). So plese
} someone, give me an explanation what exactly is a "label" ?
}
} Thank you.
}
}
} Regards
} Ari Kuusisto
} Research physicist
}
} PerkinElmer Life and Analytical Sciences
} tel. +358-2-2678 508
} fax. +358-2-2578 357
} E-mail: Ari.Kuusisto-at-PerkinElmer.com
}
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 15:55:16 2004

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We are a pathology lab for a research group and use Hematoxylin 2 (Richard-Allan
Scientific)for routine H & E's. We also use Gill's III.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Kathleen Roberts [mailto:kgrobert-at-rci.rutgers.edu]
Sent: Thursday, January 29, 2004 11:04 AM
To: mark.lewis-at-thermo.com; Microscopy-at-sparc5.microscopy.com

We use Gill's.

Kathleen
Principal Lab Technician
Neurotoxicology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

mark.lewis-at-thermo.com wrote:

} Hello everyone !
}
} I'm taking a survey to find out which type of Hematoxylin is most commonly
} used in Histology and Cytology labs.
}
} Thanks !
}
} Best regards,
}
} Mark
}
} Mark Lewis
} Product Specialist
} Anatomical Pathology
} Clinical Diagnostics
} Thermo Electron Corporation
} (412) 747-4013
} (412) 788-1097
} E-mail: mark.lewis-at-thermo.com
}
}
}
}
} _______________________________________________
} Histonet mailing list
} Histonet-at-lists.utsouthwestern.edu
} http://lists.utsouthwestern.edu/mailman/listinfo/histonet
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 16:13:31 2004

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} } I'm taking a survey to find out which type of Hematoxylin is most commonly
} } used in Histology and Cytology labs.

Gill's 3.

Karen Bovard
Dept. of Pathology
Creighton University
Omaha, NE

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 16:36:42 2004

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We are interested in software for a CCD camera on an optical microscope
that we use for sample screening and documentation, and experiment
design, in the course of doing TEM on microelectronic devices. We
already have the Sony ProScan CCD camera on an Olympus MX-50, but we
want software to drive the camera and rapidly facilitate measurement and
annotation of features seen in the microscope. Any suggestions would be
appreciated. Thanks.

John Mardinly
Intel

From MicroscopyL-request-at-ns.microscopy.com Thu Jan 29 18:26:06 2004

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Marc,
My reply to you got bounced, so I'll try it on the server.
Ken

-------- Original Message --------

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 30 12:05:39 2004

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If someone doesn't take this stuff its going to wind up as an artificial
reef in Lake Cayuga!

Two Gatan Duo Mills, one working, one for your imagination!

One Gatan PIPS system, it works to the best of my knowledge!

One Gatan PIMS system, what can I say! I don't know, just enjoy it for
what it is!

Two vintage VCR dimplers...they are unique!

No reasonable offer will be refused!

Will TRADE for an LKB glass knife maker!

Remember, these items are a heartbeat away from a watery grave in Lake
Cayuga.....

If you are interested please e-mail or call

John Grazul
Cornell University
607 255 6421
grazul-at-ccmr.cornell.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 30 12:33:37 2004

Contents Retrieved from Microscopy Listserver Archives
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Recently, I bought C nanotube samples from Nanostructured & Amorphous
Materials,Inc. However, it was not good for my experiments. If someone want
to buy this sample, please contact me.

I have 5 g, and I will keep it ~0.3 g. Please look at the following site.
The sample number is MWNT (95+%, OD 40-70 nm), and Stock #: 1242XH.
http://www.nanoamor.com/inc/pdetail?v=1&pid=220

I can provide some TEM images upon request next week. According to their
sample description, it is more than 95% quality. I do not promise this
quality, but there is no contamination I made. The price was 70 dollars plus
tax. My asking price is 45 dollars plus shipping cost. .

Thank you,
Hiromi Konishi, Ph.D.
The University of New Mexico

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 30 15:01:53 2004

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Dear colleagues:

I am looking for a compact pump for perfusion fixation of mouse brain, the
liquid flow of the pump needs to be controlled by pressure, unfortunately
the most products around are only gauged by the flow rate.

Can anyone help me out? Thanks in advance.

Xinran

Xinran Liu, M.D., Ph.D.
Center for Basic Neuroscience
UT Southwestern Medical Center at Dallas
Phone: 214-648-1830
Fax: 214-648-1801
E-mail: Xinran.Liu-at-utsouthwestern.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jan 30 18:52:43 2004

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Do it with gravity. 1 meter is perfectly fine for mouse brain
perfusion. You could not measure pressure in peristaltic pump commonly
used for such purpose because of pulsation. If you will see liquid coming
from the nose - it actually means the pressure is to high. Meantime it's
vary from mouse to mouse.You also could measure the flow rate. It seems to
me that 1 ml/min is optimal for perfusion. Sergey

At 01:14 PM 1/30/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 31 12:57:32 2004

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} I think the short answer will be that such materials don't diffract.
} The spacings are in a whole other realm of size. You would need a
} much longer wavelength to get diffraction. Also, the spacings are
} not so regular as to be able to generate anything like planes of
} atoms. "Peaks" would likely be poorly defined, but variation in
} their shape as well as position might lend some usable information.
}
} Warren
}

I hate to disagree but not only can you do electron diffraction in a
TEM from such structures, I have done it myself. It is even possible
to get a diffraction pattern from the bars of a grid.

As an alternative to electron diffraction, you can do light
diffraction from the negative or do an FFT from a digital image.

In all cases, you very quickly get information on the average spacing
of regular structures and avoid a lot of tedious measurements.

Regards,
--
Larry Stoter
NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Sat Jan 31 14:40:09 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rburke-at-uvic.ca) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday, January 30, 2004 at 13:53:06
---------------------------------------------------------------------------

Email: rburke-at-uvic.ca
Name: Robert D. Burke

Organization: University of Victoria

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I would like to obtain a fluorescence source for a Nikon
TMD inverted microscope. I require a lamphouse, powersupply and
parts to attach it to the microscope. I have the nosepiece and filter
cube assembly. Nikon no longer supports this equipment, but there
companies that make fluorescence units and adaptors. Is there anyone
who has experience with this or knows of a supplier that may help?

Robert Burke

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 2 09:20:03 2004

Contents Retrieved from Microscopy Listserver Archives
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John,

I can't find any information about a Sony Proscan camera. Is there another
model name or number that is used for this camera?

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Thursday, January 29, 2004 15:47
To: microscopy-at-msa.microscopy.com

I had no idea that I would get such a great response for my precious tools
of the trade. Thanks to everyone who called and e-mailed. The bad news is
that someone in our microscope community has made me an offer I couldn't
refuse (the cast comes off in two months). I'm really sorry that I couldn't
help everyone out, but the deal is done.

} Date: Fri, 30 Jan 2004 13:16:30 -0500
} To: microscopy-at-ns.microscopy.com
} From: John Grazul {grazul-at-ccmr.cornell.edu}
} Subject: [Microscopy] Surplus equipment BLOWOUT!!!!
}
} If someone doesn't take this stuff its going to wind up as an artificial
} reef in Lake Cayuga!
}
} Two Gatan Duo Mills, one working, one for your imagination!
}
} One Gatan PIPS system, it works to the best of my knowledge!
}
} One Gatan PIMS system, what can I say! I don't know, just enjoy it for
} what it is!
}
} Two vintage VCR dimplers...they are unique!
}
} No reasonable offer will be refused!
}
} Will TRADE for an LKB glass knife maker!
}
} Remember, these items are a heartbeat away from a watery grave in Lake
} Cayuga.....
}
}
} If you are interested please e-mail or call
}
} John Grazul
} Cornell University
} 607 255 6421
} grazul-at-ccmr.cornell.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 2 13:08:14 2004

Contents Retrieved from Microscopy Listserver Archives
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Happy New Year

I recently received the email below from Evex.

This isn't for real, is it?

...........down to B?
...........750,000 cps?????
............"excellent" (whatever that means) resolution??

reply off-list if you prefer

cheers

rtch

------- Forwarded message follows -------
Organization: Evex - Nanoanalysis
} From: "Evex - Nanoanalysis.com" {sales-at-nanoanalysis.com}
To: r.sims-at-auckland.ac.nz

750,000 cps would mean it would have to have an extraordinary detector and amplifier, not to mention a very short time constant. Shave off two zeros. Evex or someone made a typo. If this is true they should advertise.

"Excellent"? Is that a scalar or vector quantity?

Peter Tomic
Agere Systems

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Monday, February 02, 2004 2:22 PM
To: microscopy-at-msa.microscopy.com

Happy New Year

I recently received the email below from Evex.

This isn't for real, is it?

..........down to B?
..........750,000 cps?????
..........."excellent" (whatever that means) resolution??

reply off-list if you prefer

cheers

rtch

------- Forwarded message follows -------
Organization: Evex - Nanoanalysis
} From: "Evex - Nanoanalysis.com" {sales-at-nanoanalysis.com}
To: r.sims-at-auckland.ac.nz

Some of the new detector "chips" have gotten pretty fast. I have forgotten
the exact values claimed by the makers of some newly announced detector
chips so cannot comment directly. But...

1) Be sure that is *system* throughput, not just the detector spec.
2) Ask about the FWHM values at low/medium/high energy.
3) Ask about the peak/background ratio.
4) Think of other questions... Often, what the manufacturers *don't* tell
you are the really important things ;)

Woody

\
Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Monday, February 02, 2004 2:22 PM
To: microscopy-at-msa.microscopy.com

Happy New Year

I recently received the email below from Evex.

This isn't for real, is it?

..........down to B?
..........750,000 cps?????
..........."excellent" (whatever that means) resolution??

reply off-list if you prefer

cheers

rtch

------- Forwarded message follows -------
Organization: Evex - Nanoanalysis
} From: "Evex - Nanoanalysis.com" {sales-at-nanoanalysis.com}
To: r.sims-at-auckland.ac.nz

Dear Colleagues,
Please refer this to interested microscopists. Thank-you.

The Cell Sciences Imaging Facility (CSIF) at Stanford University's Medical
School is seeking a qualified electron microscopy technician. The position
is a Life Sciences Research Assistant I (LSRAI). At least one year of
experience working in an electron microscopy lab is desired and a minimum
of an Associate Degree in the sciences is required for this
position. Preference will be given to applicants with experience in
biological electron microscopy. The position is currently listed as a 30
hours/week position but is being re-listed as a full time (40 hours/week)
position. There is no money available for relocation. Stanford salary
range is 2P1; actual salary is dependent upon experience and
qualifications. Interested applicants can find more information at
http://hrweb.stanford.edu/jobs/openings/display.cgi?Job_Req=004273&JFam=NIL&JOBCODE=5588
Please apply directly to:

Jon Mulholland, Director
Cell Sciences Imaging Facility
Beckman Center, B050
Stanford University School of Medicine
Stanford, CA 94305-5301

fax 650-725-4951

jwm-at-stanford.edu
http://taltos.stanford.edu

Jon Mulholland, Director
Cell Sciences Imaging Facility
Beckman Center, B050
Stanford University School of Medicine
Stanford, CA 94305-5301

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 2 21:26:23 2004

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Ritchie,
Actually the numbers fit with the new detectors Rontec (I believe) has
brought out. They made a presentation at NESM's May meeting in Woods
Hole, MA. If I recall correctly, the resolution wasn't bad (140-160 eV
maybe?) and the count rates are simply mind boggling. They also
operate at considerably higher temperatures.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

Ritchie Sims wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 10:52:45 2004

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Dear Colleagues,
I am re-posting this because Stanford HR has changed the job # and
URL.
Please refer this to interested microscopists. Thank-you.

The Cell Sciences Imaging Facility (CSIF) at Stanford University's Medical
School is seeking a qualified electron microscopy technician. The position
is a Life Sciences Research Assistant I (LSRAI). At least one year of
experience working in an electron microscopy lab is desired and a minimum
of an Associate Degree in the sciences is required for this
position. Preference will be given to applicants with experience in
biological electron microscopy. The position is a full time (40
hours/week) position. There is no money available for relocation. Stanford
salary range is 2P1; actual salary is dependent upon experience and
qualifications. Interested applicants can find more information at
http://hrweb.stanford.edu/jobs/openings/display.cgi?Job_Req=004773&JFam=NIL&JOBCODE=5588
Please apply directly to:

Jon Mulholland, Director
Cell Sciences Imaging Facility
Beckman Center, B050
Stanford University School of Medicine
Stanford, CA 94305-5301

fax 650-725-4951

jwm-at-stanford.edu
http://taltos.stanford.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 11:11:36 2004

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We have been using a Nikon Coolpix 990 for several years now and
subsequently added Coolpix 4500. Other than issues with chromatic
aberration, the micrographs are quite usable.

We occasionally experience problems with being unable to retrieve our
images off of the compact flash cards. Files are written to the compact
flash cards as verified by looking at the properties (unused/used space),
however, there are no identifiable files present. Consequently, we reformat
the card and have to reshoot our photos. This is not only inconvenient, but
sometimes the samples have to be re-prepared or an unruly crowd has to sit
and wait.

This occurs with both the 990 and 4500 cameras as well as various brands of
cards and card readers (Lexar and SanDisk). It is not isolated to a
particular computer nor a particular user. Nikon tech support has never
heard of anyone else having this problem.

Anyone out there with similar experiences?

Thanks.

Alan Stone
ASTON Metallurgical Services

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 12:19:27 2004

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Alan;
I had a similar problem with a Sony camera using Memory Stick:
If I used the computer to manage the memory, i.e. clearing the memory of
old photos or formatting the card with the computer, the card would
become corrupted. If I use the CAMERA to reformat the card, I never have
any problems.

John Mardinly
Intel

-----Original Message-----
} From: Alan Stone [mailto:as-at-astonmet.com]
Sent: Tuesday, February 03, 2004 9:22 AM
To: microscopy-at-msa.microscopy.com

I've used a Coolpix for some time now, as well as several other cameras from
Canon, Pentax and Sony that use CF, memory stick and SD flash memory. With all
of them I've found that formatting the memory in the camera is the best
solution. In my case, I sometimes read the memory in a Mac and sometimes in a PC.
If I format the memory in the camera, both operating systems will read the
files without difficulty. If the memory is formatted in the computer, the camera
usually sees it OK but the other computer system sometimes has difficulties.

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 14:20:48 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Sorry, but I can't resist asking:

Has anyone reported this to NASA and JPL ? :-)

Thank you;

John W. Raffensperger, Jr.
IS Manager
Helwig Carbon Products, Inc.

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Tuesday, February 03, 2004 12:30 PM
To: Alan Stone; microscopy-at-msa.microscopy.com

Alan,

Two questions.
1) Can you see the 'missing' images using the camera's playback function
('defective' CF card in camera)?
2) If so, can you download those images from the camera to your computer
via the USB cable?

If the answer to above questions is yes than you may have an intermittent
computer/CF card management problem. I always format my cards in the
camera. CF cards do fail of course but I have taken over 1000 pix using
Lexar and Transcend cards on a Canon G3. No lost images yet.
Good luck,
Jim

} Date: Tue, 03 Feb 2004 11:22:24 -0600
} To: microscopy-at-msa.microscopy.com
} From: Alan Stone {as-at-astonmet.com}
} Subject: [Microscopy] Coolpix Compact Flash Problems

}
}
} We have been using a Nikon Coolpix 990 for several years now and
} subsequently added Coolpix 4500. Other than issues with chromatic
} aberration, the micrographs are quite usable.
}
} We occasionally experience problems with being unable to retrieve our
} images off of the compact flash cards. Files are written to the compact
} flash cards as verified by looking at the properties (unused/used space),
} however, there are no identifiable files present. Consequently, we reformat
} the card and have to reshoot our photos. This is not only inconvenient, but
} sometimes the samples have to be re-prepared or an unruly crowd has to sit
} and wait.
}
} This occurs with both the 990 and 4500 cameras as well as various brands of
} cards and card readers (Lexar and SanDisk). It is not isolated to a
} particular computer nor a particular user. Nikon tech support has never
} heard of anyone else having this problem.
}
} Anyone out there with similar experiences?
}
} Thanks.
}
} Alan Stone
} ASTON Metallurgical Services
}

James S. Romanow
The University of Connecticut
Physiology and Neurobiology Department
Electron Microscopy Facility
Unit 3242
91 North Eagleville Road
BSP Building, Room G06
Storrs, CT 06269-3242

860 486-2914 voice
860 486-6369 fax
james.romanow-at-uconn.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 15:03:19 2004

Contents Retrieved from Microscopy Listserver Archives
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I want to clarify that all of the formatting and re-formatting has been
done directly in the Coolpix cameras and never in the computers.

This is such an erratic problem that we don't see any patterns. It appears
to be some type of index writing problem, maybe the sessions are not
properly closing out. We added time between turning off the camera and
removing the chip to ensure that we give the camera enough time. It did not
help. It also is unrelated to how many pictures have been taken, whether
the card is new, used or old.

We will be doing a trial to keep the cards from being mixed between the
different cameras. I don't believe that is an issue as we have had failures
shortly after re-formatting.

If you do had similar problems, then please contact Nikon's tech support.
Again, they tell me I am the only one reporting this.

Regards,

Alan Stone
ASTON

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 15:47:20 2004

Contents Retrieved from Microscopy Listserver Archives
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Formatting in camera is generally a good idea. If you must format
in a PC with Windows XP or 2000, make sure you format the card using "FAT"
and not "FAT 32". With the exception of a few new high end models, most
cameras will not recognize media formatted FAT 32.

George

George Laing
National Graphic Supply
800.223.7130 x3109
scisales-at-ngscorp.com

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 3 18:16:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (kemmons-at-wrfseattle.org) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, February 3, 2004 at 13:19:57
---------------------------------------------------------------------------

Email: kemmons-at-wrfseattle.org
Name: Kim Emmons

Organization: Washington Research Foundation

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Can anyone tell me what the installed base of scanning
and/or transmission electron microscopes is in the U.S. or worldwide,
or otherwise point me to a resource which can do so?

I am also intersted in statistics on the number of samples processed
for a given period of time on the average machine, but I suspect it
varies widely from one user to the next. If anyone would like to
volunteer information from their own experience, it would be helpful.

Thank you,
Kim Emmons

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 03:19:17 2004

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Alan

the only other suggestion that I can make is that maybe the camera has still been powered up when you have removed the card for reading, because I know that there have been reports that this can cause problems.

Malcolm

Malcolm Haswell
e.m. unit
University of Sunderland
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Alan Stone {as-at-astonmet.com}

Focus on Microscopy 2004 Philadelphia, USA, April 4 to April 7, 2004

Dear Colleagues,

we have received a number of inquiries whether if it would still be
possible to submit abstracts to FOM2004. To accommodate these
requests we have extended the deadline to Friday, February 13.
However, this deadline will be strictly observed since we aim to have
the program ready and inform you about acceptance at the end of the
week after that.

Please use for submission our electronic system at
http://www.FocusOnMicroscopy.org/2004/abstracts.html
and submit until February 13.

Contributions will be selected for either key note presentation,
regular contribution or poster.

For further information see http://www.FocusOnMicroscopy.org

On behalf of the organizers FOM2004

Andres Kriete
Drexel University & Coriell Institute
Philadelphia, USA
G.J. (Fred) Brakenhoff
Univ. of Amsterdam, the Netherlands

E-mail: info2004-at-FocusOnMicroscopy.org
Web: www.FocusOnMicroscopy.org

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 07:59:25 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Yes Alan I have experienced this problem. Unfortunately for me this
occurred in the middle of a failure analysis while cross sectioning a
defective capacitor. I lost some irreplaceable pictures.

Anyway I as usual turned the camera off and waited 15 seconds and removed
the card from the camera inserted into the card reader connected to the
computer. At this point I move the images to the hard drive on my computer.
After this I manipulate the images from the hard drive. The problem
encountered is removing the card from the reader. If removed too soon it
will cause either the next card inserted to be corrupt or the card removed
will be corrupt (no images). Now do not get the impression I am removing
the card while the data is transferring but some 15 to 30 seconds after the
transfer. So the solution I have come up with is to keep 2 cards on hand so
that I can insert and leave one in the reader for some time, at least a few
minutes to avoid this drastic situation. Hope this helps with your
situation.

Robert Fowler
Quality Assurance Failure Analysis Technician
TDK Components USA, Inc.
Multilayer Ceramic Capacitor Division
1 TDK Boulevard
Peachtree City GA 30269-2051
Telephone: (770) 631-0410 Ext.249
Fax: (770) 487-1460
email: robert.fowler-at-tdktca.com
www.component.tdk.com

Alan Stone
{as-at-astonmet.com}
To
02/04/2004 08:47 AM Robert.Fowler-at-tdktca.com
cc

Subject
Re: Fw: Follow Up to
Coolpix Compact Flash Posting

Robert,

We initially format the cards in the cameras or re-format after a card
failure. Our routine is to
take our pictures, turn off the cameras & wait a minimum of 15 seconds. We
then remove the cards, bring them over to our desktop computers and insert
the cards into the card readers. Occasionally, the images are not
retrievable. After not having a problem for several months, I had three
failures last week while hosting a legal project and then twice again
yesterday and on Monday. We cannot pin this down to a particular card,
camera, computer, user nor card reader.

Alan

At 07:26 AM 2/4/2004, you wrote:

} Alan are you using a card reader on the computer? If this is the case I
} will send a response to the listserver.
}
} Robert Fowler
} Quality Assurance Failure Analysis Technician
} TDK Components USA, Inc.
} Multilayer Ceramic Capacitor Division
} 1 TDK Boulevard
} Peachtree City GA 30269-2051
} Telephone: (770) 631-0410 Ext.249
} Fax: (770) 487-1460
} email: robert.fowler-at-tdktca.com
} www.component.tdk.com
} ----- Forwarded by Robert Fowler/TCU/TDK-US on 02/04/2004 08:24 AM -----
}
} Alan Stone
} {as-at-astonmet.com}
}
To
} 02/03/2004 04:14 PM microscopy-at-msa.microscopy.com
}
cc
}
}
Subject
} Follow Up to Coolpix
} Compact Flash Posting
}
}
}
}
}
}
}
}
}
}
}
}
}
------------------------------------------------------------------------------

}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

}
}
}
}
} I want to clarify that all of the formatting and re-formatting has been
} done directly in the Coolpix cameras and never in the computers.
}
} This is such an erratic problem that we don't see any patterns. It appears
} to be some type of index writing problem, maybe the sessions are not
} properly closing out. We added time between turning off the camera and
} removing the chip to ensure that we give the camera enough time. It did
not
} help. It also is unrelated to how many pictures have been taken, whether
} the card is new, used or old.
}
} We will be doing a trial to keep the cards from being mixed between the
} different cameras. I don't believe that is an issue as we have had
failures
} shortly after re-formatting.
}
} If you do had similar problems, then please contact Nikon's tech support.
} Again, they tell me I am the only one reporting this.
}
} Regards,
}
} Alan Stone
} ASTON
}
}
}
}
}
}
} THIS TRANSMISSION IS INTENDED FOR THE SOLE USE OF THE INDIVIDUAL AND
ENTITY
} TO WHOM IT IS ADDRESSED AND MAY CONTAIN PRIVILEGED AND/OR CONFIDENTIAL
} INFORMATION.
}
} If you are not the intended recipient, be advised that any
use,
} dissemination, distribution or duplication of this transmission is
strictly
} prohibited. If you received this transmission in error, please notify
the
} sender immediately by electronic reply to this transmission or by
phone
} (847-803-6100). Thank you.

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 08:51:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Listers,
I am interested in measuring quantitatively the chitin
(N-acetylglucosamin) in fungal cell wall (Aspergillus spp.). We are
looking for antibody(ies)(monoclonal or polyclonal) against chitin. I
would very much appreciate any clue.

Haixin Xu (PhD)
Dept of Biological Sciences
University of Maryland Baltimore County
Baltimore, MD 21228

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 09:11:49 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Yes Alan I have experienced this problem. Unfortunately for me this
occurred in the middle of a failure analysis while cross sectioning a
defective capacitor. I lost some irreplaceable pictures.

Anyway I as usual turned the camera off and waited 15 seconds and removed
the card from the camera inserted into the card reader connected to the
computer. At this point I move the images to the hard drive on my computer.
After this I manipulate the images from the hard drive. The problem
encountered is removing the card from the reader. If removed too soon it
will cause either the next card inserted to be corrupt or the card removed
will be corrupt (no images). Now do not get the impression I am removing
the card while the data is transferring but some 15 to 30 seconds after the
transfer. So the solution I have come up with is to keep 2 cards on hand so
that I can insert and leave one in the reader for some time, at least a few
minutes to avoid this drastic situation. Hope this helps with your
situation.

Robert Fowler
Quality Assurance Failure Analysis Technician
TDK Components USA, Inc.
Multilayer Ceramic Capacitor Division
1 TDK Boulevard
Peachtree City GA 30269-2051
Telephone: (770) 631-0410 Ext.249
Fax: (770) 487-1460
email: robert.fowler-at-tdktca.com
www.component.tdk.com

Alan Stone
{as-at-astonmet.com}
To
02/04/2004 08:47 AM Robert.Fowler-at-tdktca.com
cc

Subject
Re: Fw: Follow Up to
Coolpix Compact Flash Posting

Robert,

We initially format the cards in the cameras or re-format after a card
failure. Our routine is to
take our pictures, turn off the cameras & wait a minimum of 15 seconds. We
then remove the cards, bring them over to our desktop computers and insert
the cards into the card readers. Occasionally, the images are not
retrievable. After not having a problem for several months, I had three
failures last week while hosting a legal project and then twice again
yesterday and on Monday. We cannot pin this down to a particular card,
camera, computer, user nor card reader.

Alan

At 07:26 AM 2/4/2004, you wrote:

} Alan are you using a card reader on the computer? If this is the case I
} will send a response to the listserver.
}
} Robert Fowler
} Quality Assurance Failure Analysis Technician
} TDK Components USA, Inc.
} Multilayer Ceramic Capacitor Division
} 1 TDK Boulevard
} Peachtree City GA 30269-2051
} Telephone: (770) 631-0410 Ext.249
} Fax: (770) 487-1460
} email: robert.fowler-at-tdktca.com
} www.component.tdk.com
} ----- Forwarded by Robert Fowler/TCU/TDK-US on 02/04/2004 08:24 AM -----
}
} Alan Stone
} {as-at-astonmet.com}
}
To
} 02/03/2004 04:14 PM microscopy-at-msa.microscopy.com
}
cc
}
}
Subject
} Follow Up to Coolpix
} Compact Flash Posting
}
}
}
}
}
}
}
}
}
}
}
}
}
------------------------------------------------------------------------------

}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

}
}
}
}
} I want to clarify that all of the formatting and re-formatting has been
} done directly in the Coolpix cameras and never in the computers.
}
} This is such an erratic problem that we don't see any patterns. It appears
} to be some type of index writing problem, maybe the sessions are not
} properly closing out. We added time between turning off the camera and
} removing the chip to ensure that we give the camera enough time. It did
not
} help. It also is unrelated to how many pictures have been taken, whether
} the card is new, used or old.
}
} We will be doing a trial to keep the cards from being mixed between the
} different cameras. I don't believe that is an issue as we have had
failures
} shortly after re-formatting.
}
} If you do had similar problems, then please contact Nikon's tech support.
} Again, they tell me I am the only one reporting this.
}
} Regards,
}
} Alan Stone
} ASTON
}
}
}
}
}
}
} THIS TRANSMISSION IS INTENDED FOR THE SOLE USE OF THE INDIVIDUAL AND
ENTITY
} TO WHOM IT IS ADDRESSED AND MAY CONTAIN PRIVILEGED AND/OR CONFIDENTIAL
} INFORMATION.
}
} If you are not the intended recipient, be advised that any
use,
} dissemination, distribution or duplication of this transmission is
strictly
} prohibited. If you received this transmission in error, please notify
the
} sender immediately by electronic reply to this transmission or by
phone
} (847-803-6100). Thank you.

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 13:01:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We are in the final stages of acquiring a new scope. I am looking for
comments, feedback, etc. - the good, the bad and the ugly - from
users/owners/managers of FEI Quanta (ESEM) FEG scopes.

Best done with direct emailings to me rather than back to the list. Or if
you would like I would be happy to call anyone wishing to talk rather than
email.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 13:03:27 2004

Contents Retrieved from Microscopy Listserver Archives
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On Feb 4, 2004, at 9:44 AM, Christopher Gilpin wrote:

} I was wondering what people were using to pump the dewars of TEM cryo
} holders. I have been using a line to a standard Denton coating unit but
} this is becoming impractical. I am aware of dedicated solutions as
} produced by Gatan but would be interested in how creative users have
} been.
}
Dear Chris,
We had a set-up on the HVEM with lines from the airlock mechanical
pump and the column high-vacuum pump that was used to pump out the
dewars of the cryo holder and the GATAN anticontaminator. We did not
experience any microscope vacuum problems as a result of using this
system, although the column vacuum was not as high as that in many
more-modern TEMs.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 13:40:21 2004

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------------------------------------------------------------------------------
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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Yes Alan I have experienced this problem. Unfortunately for me this
occurred in the middle of a failure analysis while cross sectioning a
defective capacitor. I lost some irreplaceable pictures.

Anyway I as usual turned the camera off and waited 15 seconds and removed
the card from the camera inserted into the card reader connected to the
computer. At this point I move the images to the hard drive on my computer.
After this I manipulate the images from the hard drive. The problem
encountered is removing the card from the reader. If removed too soon it
will cause either the next card inserted to be corrupt or the card removed
will be corrupt (no images). Now do not get the impression I am removing
the card while the data is transferring but some 15 to 30 seconds after the
transfer. So the solution I have come up with is to keep 2 cards on hand so
that I can insert and leave one in the reader for some time, at least a few
minutes to avoid this drastic situation. Hope this helps with your
situation.

Robert Fowler
Quality Assurance Failure Analysis Technician
TDK Components USA, Inc.
Multilayer Ceramic Capacitor Division
1 TDK Boulevard
Peachtree City GA 30269-2051
Telephone: (770) 631-0410 Ext.249
Fax: (770) 487-1460
email: robert.fowler-at-tdktca.com
www.component.tdk.com

Alan Stone
{as-at-astonmet.com}
To
02/04/2004 08:47 AM Robert.Fowler-at-tdktca.com
cc

Subject
Re: Fw: Follow Up to
Coolpix Compact Flash Posting

Robert,

We initially format the cards in the cameras or re-format after a card
failure. Our routine is to
take our pictures, turn off the cameras & wait a minimum of 15 seconds. We
then remove the cards, bring them over to our desktop computers and insert
the cards into the card readers. Occasionally, the images are not
retrievable. After not having a problem for several months, I had three
failures last week while hosting a legal project and then twice again
yesterday and on Monday. We cannot pin this down to a particular card,
camera, computer, user nor card reader.

Alan

At 07:26 AM 2/4/2004, you wrote:

} Alan are you using a card reader on the computer? If this is the case I
} will send a response to the listserver.
}
} Robert Fowler
} Quality Assurance Failure Analysis Technician
} TDK Components USA, Inc.
} Multilayer Ceramic Capacitor Division
} 1 TDK Boulevard
} Peachtree City GA 30269-2051
} Telephone: (770) 631-0410 Ext.249
} Fax: (770) 487-1460
} email: robert.fowler-at-tdktca.com
} www.component.tdk.com
} ----- Forwarded by Robert Fowler/TCU/TDK-US on 02/04/2004 08:24 AM -----
}
} Alan Stone
} {as-at-astonmet.com}
}
To
} 02/03/2004 04:14 PM microscopy-at-msa.microscopy.com
}
cc
}
}
Subject
} Follow Up to Coolpix
} Compact Flash Posting
}
}
}
}
}
}
}
}
}
}
}
}
}
------------------------------------------------------------------------------

}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

}
}
}
}
} I want to clarify that all of the formatting and re-formatting has been
} done directly in the Coolpix cameras and never in the computers.
}
} This is such an erratic problem that we don't see any patterns. It appears
} to be some type of index writing problem, maybe the sessions are not
} properly closing out. We added time between turning off the camera and
} removing the chip to ensure that we give the camera enough time. It did
not
} help. It also is unrelated to how many pictures have been taken, whether
} the card is new, used or old.
}
} We will be doing a trial to keep the cards from being mixed between the
} different cameras. I don't believe that is an issue as we have had
failures
} shortly after re-formatting.
}
} If you do had similar problems, then please contact Nikon's tech support.
} Again, they tell me I am the only one reporting this.
}
} Regards,
}
} Alan Stone
} ASTON
}
}
}
}
}
}
} THIS TRANSMISSION IS INTENDED FOR THE SOLE USE OF THE INDIVIDUAL AND
ENTITY
} TO WHOM IT IS ADDRESSED AND MAY CONTAIN PRIVILEGED AND/OR CONFIDENTIAL
} INFORMATION.
}
} If you are not the intended recipient, be advised that any
use,
} dissemination, distribution or duplication of this transmission is
strictly
} prohibited. If you received this transmission in error, please notify
the
} sender immediately by electronic reply to this transmission or by
phone
} (847-803-6100). Thank you.

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 14:04:27 2004

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I've inherited an MT-5000 ultramicrotome that hasn't been used in a number of years. RMC/Boeckler won't offer service on this model. Some parts are still available.

Does anyone know who does microtome repair in the Seattle, Washington area?

Thanks,

Paulette Brunner
Center for Cell Dynamics
Friday Harbor Labs, University of Washington

(206) 616-0895
(206) 616-6804 (fax)
pbrunner-at-u.washington.edu
http://raven.zoology.washington.edu/celldynamics/

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 14:07:26 2004

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Hi Listers,
I am interested in measuring quantitatively the chitin
(N-acetylglucosamin) in fungal cell wall (Aspergillus spp.). We are
looking for antibody(ies)(monoclonal or polyclonal) against chitin. I
would very much appreciate any clue.

Haixin Xu (PhD)
Dept of Biological Sciences
University of Maryland Baltimore County
Baltimore, MD 21228

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 14:41:42 2004

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Hi Haixin,

Did you try searching through abcam? This is the link: http://www.abcam.com/

Cheers,

Jacqui.

Haixin Xu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi Listers,
} I am interested in measuring quantitatively the chitin
} (N-acetylglucosamin) in fungal cell wall (Aspergillus spp.). We are
} looking for antibody(ies)(monoclonal or polyclonal) against chitin. I
} would very much appreciate any clue.
}
} Haixin Xu (PhD)
} Dept of Biological Sciences
} University of Maryland Baltimore County
} Baltimore, MD 21228

Jacqueline Ross
Biomedical Imaging Research Unit
Division of Anatomy with Radiology
Faculty of Medical & Health Sciences
The University of Auckland
Private Bag 92019
Auckland, NEW ZEALAND

Tel: 64 9 373 7599 Ext 7438
Fax: 64 9 373 7484

http://www.health.auckland.ac.nz/biru/

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 15:16:21 2004

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Listers: I've got a Spicer Consulting SC12 Magnetic Field
Canceling System, but no manual to go with it. If anybody
on the list has one they will loan me or copy for me? I
will be glad to pay postage and/or copy costs. Please reply
off-list.

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 15:59:43 2004

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A friend has sent me a really nice calendar as a late Christmas
present. It's got photos of old light microscopes, micrographs (all
pathology), microscopes on postage stamps, and microscopy-related
quotations (some are from the Project MICRO collection). The price
is right - it's free. Here's the description:

The National Museum of Health and Medicine of the Armed Forces
Institute of Pathology in Washington, D.C. is offering the 2004
American Registry of Pathology/Armed Forces Institute of Pathology
calendar on a first-come, first-served basis. The calendar features
photographs of the microscopes in the museum's Billings Microscope
Collection. For a free copy, send your name, address, and affiliation
by e-mail only to nmhminfo-at-afip.osd.mil. Requests for multiple copies
cannot be accommodated.
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 16:31:55 2004

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I'm sorry if someone has already suggested this, but why don't you just take the
camera to the computer, or vice-versa, and download off the camera with the Nikon
USB cable?

Maybe not everyone's setup allows this, but we've been running a Coolpix 4500 for
some months now, we never remove the card from the camera, and we've never had
any problems at all. The nikon download s/w kicks in automatically and works a treat.

cheers

rtch

Tech Forum Professional Technical Staff Awards (PTSA)

Are you an MSA member and planning to submit an abstract for M & M
2004 in Savannah? If so, consider submitting an application for the
Tech Forum's PTSA. This award consists of complimentary full meeting
registration and travel reimbursement up to $600.00. The
requirements are simple: 1. submit a paper/poster abstract at the
meeting website, 2. send a copy of the abstract to the TF Chair at
the address below, and 3. send a support letter from your
manager/supervisor confirming your position as full-time technical
support staff. Deadline is February 16, 2004. Either hardcopy or
electronic copy of abstract & support letter will be accepted.

Submit Applications to:

Cathy Johnson
TF Chair
cjohnmicro-at-aol.com
6422 Simms St. #66
Arvada, CO 80004
(303) 420-6373

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 4 17:28:32 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rpowell-at-nanoprobes.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Wednesday, February 4, 2004 at 12:09:24
---------------------------------------------------------------------------

Email: rpowell-at-nanoprobes.com
Name: Rick Powell at Nanoprobes

Organization: Nanoprobes, Incorporated

Title-Subject: [Microscopy] searching for antibody to chitin

Question: Hello Haixin:

Can't recommend any specific antibodies, but the best place to look
is Linscott's Directory of Immunological and Biological Reagents:

http://www.linscottsdirectory.com/

USA:
4877 Grange Road
Santa Rosa, CA 95404
Tel: (707) 763-7098
Fax: (707) 763-8372

Europe:
Stalkvarn
S-54017 Lerdala SWEDEN
Tel: +46 511-80081
Fax: +46 511-80081

You could also try Abcam (may need to register first):

http://www.abcam.com/

Hope this helps,

Rick Powell

*****************************************************************************************
Richard D. Powell * rpowell-at-nanoprobes.com * www.nanoprobes.com
NANOPROBES, Incorporated
95 Horse Block Road, Yaphank, NY 11980-9710, USA

US Toll-free: (877) 447-6266 * Tel: (919) 845-6324 * Fax:
(631) 980-3608

Sign up for our newsletter: http://www.nanoprobes.com/Newsletter.html
*****************************************************************************************

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 09:42:59 2004

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I must be wacky.... I remember prepping chloroform suspensions on carbon
coated formvar copper grids without any problems 5 years ago. Now my films
are dissolving and my particles left behind. Has the polymer structure of
"formvar" changed? I prefer to use chloroform for my suspensions, so does
this means I must resign myself to the more fragile (I can be pretty
ham-handed at times) carbon film grids?

Suggestion and advice are welcome!!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 13:40:57 2004

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Hi,
We use formvar in diethylene chloride all the time and have no problem.
We use them for students because it is so durable. Generally for
standard 80 or 100 kV we use 0.25% formvar in diethylene chloride.
Good luck,
Judy

Judy Murphy, PhD
San Joaquin Delta College
Microscopy Technology
5151 Pacific Ave
Stockton, CA 95207
209-954-5284
FAX 209-954-5600
jmurphy-at-deltacollege.edu
http://www.sjdccd.cc.ca.us/dept/electmicro/index.html

Frank.Karl-at-degussa.com wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I must be wacky.... I remember prepping chloroform suspensions on carbon
} coated formvar copper grids without any problems 5 years ago. Now my films
} are dissolving and my particles left behind. Has the polymer structure of
} "formvar" changed? I prefer to use chloroform for my suspensions, so does
} this means I must resign myself to the more fragile (I can be pretty
} ham-handed at times) carbon film grids?
}
} Suggestion and advice are welcome!!!
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 14:15:02 2004

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Hi,

I haven't done formvar grids in a long time, but when I did, I also made them up
in diethylene chloride.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Judy Murphy [mailto:jmurphy-at-deltacollege.org]
Sent: Thursday, February 05, 2004 2:54 PM
To: Frank.Karl-at-degussa.com
Cc: microscopy-at-msa.microscopy.com

Hi,
We use formvar in diethylene chloride all the time and have no problem.
We use them for students because it is so durable. Generally for
standard 80 or 100 kV we use 0.25% formvar in diethylene chloride.
Good luck,
Judy

Judy Murphy, PhD
San Joaquin Delta College
Microscopy Technology
5151 Pacific Ave
Stockton, CA 95207
209-954-5284
FAX 209-954-5600
jmurphy-at-deltacollege.edu
http://www.sjdccd.cc.ca.us/dept/electmicro/index.html

Frank.Karl-at-degussa.com wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------
}
} I must be wacky.... I remember prepping chloroform suspensions on carbon
} coated formvar copper grids without any problems 5 years ago. Now my films
} are dissolving and my particles left behind. Has the polymer structure of
} "formvar" changed? I prefer to use chloroform for my suspensions, so does
} this means I must resign myself to the more fragile (I can be pretty
} ham-handed at times) carbon film grids?
}
} Suggestion and advice are welcome!!!
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 14:43:40 2004

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Long ago we did use chloroform as a solvent for Formvar, so I'm not
surprised that when you apply your suspensions in chloroform the Formvar
breaks or dissolves. I'm betting that 1) you've forgotten that you had to
switch to something other than chloroform, 2) you had thicker Formvar
and a smaller volume of chloroform that you left on for less time, or
3) most likely, you used carbon-stabilized Formvar coated grids and the
chloroform did not get to the Formvar. Try the latter, making sure you put
your suspensions on the carbon side.

Good luck!

Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 14:56:20 2004

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} At 12:33 PM 1/31/2004, you wrote:
} } } I think the short answer will be that such materials don't
} } } diffract. The spacings are in a whole other realm of size. You
} } } would need a much longer wavelength to get diffraction. Also, the
} } } spacings are not so regular as to be able to generate anything
} } } like planes of atoms. "Peaks" would likely be poorly defined, but
} } } variation in their shape as well as position might lend some
} } } usable information.
} } }
} } } Warren
} }
} } I hate to disagree but not only can you do electron diffraction in
} } a TEM from such structures, I have done it myself. It is even
} } possible to get a diffraction pattern from the bars of a grid.
} }
} } As an alternative to electron diffraction, you can do light
} } diffraction from the negative or do an FFT from a digital image.
} }
} } In all cases, you very quickly get information on the average
} } spacing of regular structures and avoid a lot of tedious
} } measurements.
} }
} } Regards,
} } --
} } Larry Stoter
} Point taken. I was thinking x-ray diffraction more than other
} methods. I would still wonder how well diffraction works with only
} semi-regular arrangement, but I suppose some diffraction pattern
} should result with any periodicity. The challenge is finding a beam
} of the right wavelength.
}
} I have not played around with FFTs on images yet. Most of our
} samples are not near that regular, but I may have to look into it.
}
} Warren
}
I must say, I don't understand the physics but, in a TEM, you really
can get electron diffraction from periodic structures which are many
order of magnitude larger than any wavelength involved (although,
atomic spacings are quite abit larger than the electron wavelength
anyway). And the regularity doesn't need to be that good - muscle can
give some very nice diffraction patterns.

Going back to the orginal question, why isn't electron diffraction
used to measure spacings in periodic biological structures - muscle
and myelin being the two most obvious.

regards,
--
Larry Stoter
NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 15:01:18 2004

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this is a test since all my messages in the last few months have been
returned. I am sorry for any inconvenience. QC Yu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 15:18:01 2004

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Listers: One of our colleagues was nice enough to fax me a copy of his manual, so
I'm all set. Thanks for the replies. This list is a great asset. Way to go,
Nestor!

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Listers: I've got a Spicer Consulting SC12 Magnetic Field
} Canceling System, but no manual to go with it. If anybody
} on the list has one they will loan me or copy for me? I
} will be glad to pay postage and/or copy costs. Please reply
} off-list.
}
} --
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} Becky Holdford (r-holdford-at-ti.com)
} 972-995-2360
} 972-648-8743 (pager)
} SC Packaging FA Development
} Texas Instruments, Inc.
} Dallas, TX
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 15:42:19 2004

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We would recommend a pure carbon coated grid where all the traces of plastic
are removed. We produce them for non-aqueous solutions so solvents will not
harm the carbon support film.
This would eliminate the dissolving of the formvar by the solvent.

John Arnott

Disclaimer: Ladd Research sell carbon coated grids that are described in
this e-mail

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com
----- Original Message -----
} From: "Judy Murphy" {jmurphy-at-deltacollege.org}
To: {Frank.Karl-at-degussa.com}
Cc: {microscopy-at-msa.microscopy.com}
Sent: Thursday, February 05, 2004 2:53 PM

Hi, all

A word from a light microscopist:
Diffraction happens all the time. You can even do a neat diffraction
experiment with your hand. If you hold your hand between your eye and a
distant light source (palm toward you seems to work best, looking at, for
instance, the ceiling light) and leave just a small space between your
fingers, you will see the bright/dark/bright fringes which result from the
interference of light diffracting around your fingers.

Using diffraction patterns to measure periodic structures is well known in
interferometry. I have measured structures below the limit of resolution
by calibrating a special eyepiece micrometer (ex: a "Wright" eyepiece) and
viewing the diffraction pattern of a slightly sheared image in the back
focal plane of the objective (many many years ago, now).

I also used X-ray diffraction to measure spacing in liquid crystals (also
many years ago).

The challenge is to get enough of the periodic structure so that its
diffraction pattern is not washed out by the overlaying of the diffraction
patterns from other, non-periodic structures.

All of this is based in fundamental physics (Young's far-field diffraction
experiment, and Bragg's Law).

For anyone interested in trying... let me know how the experiment comes out!

Best regards,
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^
Don't forget: the American Chem Society's Applied Optical Microscopy
Course, March 5-7, Chicago, Ill.
Visit our website for details and registration. NOT JUST FOR CHEMISTS!!!!
^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^

At 09:00 PM 2/5/04 +0000, Larry Stoter wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 16:07:58 2004

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Although most people use ethylene dichloride for Formvar, chloroform
will also dissolve Butvar and Formvar. Some companies, in fact,
provide various concentrations of the plastic dissolved in
chloroform. We use 0.25% Butvar in chloroform.

I believe that what you are experiencing is, indeed, the dissolution
of the underlying Formvar layer leaving a very fragile carbon layer
that breaks upon drying of your particulate suspension. So, either
change the liquid you are suspending the particles in (try methanol,
acentone) or put a heavier layer of carbon on the Formvar.

} I must be wacky.... I remember prepping chloroform suspensions on carbon
} coated formvar copper grids without any problems 5 years ago. Now my films
} are dissolving and my particles left behind. Has the polymer structure of
} "formvar" changed? I prefer to use chloroform for my suspensions, so does
} this means I must resign myself to the more fragile (I can be pretty
} ham-handed at times) carbon film grids?
}
} Suggestion and advice are welcome!!!
}
} Frank Karl
} Degussa Corporation

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 5 17:29:48 2004

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Dear Listers:
I recently ordered Epofix as an alternative to LR White, since it supposedly
cures at RT and is purported not to infiltrate samples. After polymerizing
in various molds, at low pressure, waiting for days, I do not get blocks
hard enough for ultramicrotomy. After numerous emails to the manufacturer,
the gist is that it DOES require some heat to get a hard block (one that a
fingernail doesn't go through). I found a post from about a year ago
mentioning Epofix; I am wondering if anyone does get this resin to harden at
room temp?
Thanks,
Jessica

Bend Research, Inc
64550 Research Rd
Bend, OR 97701
(541) 382-4100 page
(541) 382-0212 x240

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 6 01:22:48 2004

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Hi Jessica, I have been using Epofix resin without problems. It hardens at 22şC in
about 24 hours. You have to control carefully the proportion of resin and hardener.
I mix 15 parts by volume of resin with 2 parts by volume of hardener and I get
blocks hard enough for ultramicrotomy. I buy Epofix to EMS (Electron Microscopy
Science).
Cristina Almansa
University of Alicante
SPAIN
jcervantes-at-bendres.com ha escrito:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear Listers:
} I recently ordered Epofix as an alternative to LR White, since it supposedly
} cures at RT and is purported not to infiltrate samples. After polymerizing
} in various molds, at low pressure, waiting for days, I do not get blocks
} hard enough for ultramicrotomy. After numerous emails to the manufacturer,
} the gist is that it DOES require some heat to get a hard block (one that a
} fingernail doesn't go through). I found a post from about a year ago
} mentioning Epofix; I am wondering if anyone does get this resin to harden at
} room temp?
} Thanks,
} Jessica
}
} Bend Research, Inc
} 64550 Research Rd
} Bend, OR 97701
} (541) 382-4100 page
} (541) 382-0212 x240

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 6 02:02:15 2004

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I'm having serious problems achieving adequate development of the new Kodak
4489 EM film. We have no facilities to carry out development on site and
have to send film packages to another lab, subsequently, the quality of
development is at the discretion of the other (non-commercial) lab.
Basically its a hit or miss even using new development protocols.
Its got to the stage Id be willing to send our film anywhere in the UK
(maybe Europe) to be developed commercially if consistently good quality can
be achieved.
Does anyone know of somewhere which offers this service?

Thanks.

Veterinary Laboratories Agency (VLA)

This email and any attachments is intended for the named recipient only. Its
unauthorised use, disclosure, storage or copying is not permitted. If you have
received it in error, please destroy all copies and inform the sender. Whilst this
email and associated attachments will have been checked for known viruses
whilst within VLA systems we can accept no responsibility once it has left our
systems. Communications on VLA's computer systems may be monitored
and/or recorded to secure the effective operation of the system and for other
lawful purposes.

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 6 05:32:48 2004

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Dear Listers,

We use a Cameca SU-30 as SEM and need to coat some fresh fruits with carbon.
Can anyone send me an information about coating and sample preparation
instructions for organic materials? Thanks.

Orkun ERSOY

Hacettepe University

Geological Engineering

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 6 10:06:02 2004

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Thanks to all the replies on Epofix. It is definitely true that I am using
a much smaller volume than the plugs or mounts mentioned by some of you, so
the temperature of the resin never rises above RT (I did measure this,
looking for an exotherm). I will try larger molds and heating slightly as
suggested; thanks to everyone again for being a good resource.

Jessica Cervantes
Bend Research, Inc
64550 Research Rd
Bend, OR 97701
(541) 382-4100 page

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 6 12:42:10 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thanks to all the replies on Epofix. It is definitely true that I am using
a much smaller volume than the plugs or mounts mentioned by some of you, so
the temperature of the resin never rises above RT (I did measure this,
looking for an exotherm). I will try larger molds and heating slightly as
suggested; thanks to everyone again for being a good resource.

Jessica Cervantes
Bend Research, Inc
64550 Research Rd
Bend, OR 97701
(541) 382-4100 page

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 6 13:37:22 2004

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**FIRST CALL FOR PAPERS**

The 2004 Spring Meeting of
THE TEXAS SOCIETY FOR MICROSCOPY
“Embracing All Forms of Microscopy”

April 22, 23, 24, 2004

ABSTRACTS MUST BE RECEIVED BY: MARCH 11, 2004
Mail abstracts to: Camelia G.-A. Maier, Ph.D.
Department of Biology
Texas Woman's University
Denton, TX 76204-5799
Tel.: 940-898-2358 (office)
E-mail: cmaier-at-twu.edu

The Doubletree Hotel - Post Oak
2001 Post Oak Blvd.
Houston, TX 77056
(713)961-9300
(800)245-7299

RATES: $85.00 Single, Double, Triple and Quad
Mention that you are with the Texas Society for Microscopy
when making your reservations.

HOTEL RESERVATION DEADLINE: MARCH 25, 2004
After this date reservations will be accepted on a space
available basis,
convention rates not guaranteed.

THURSDAY WORKSHOP
Spectrum Imaging for Materials Characterization
Presented by John J. Friel
Princeton Gamma - Tech

Please see our website (http://www.texasmicroscopy.org) for
registration forms and author's instructions.

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (webmaster-at-texasmicroscopy.org)
TSM Webmaster
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 7 20:47:47 2004

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Hi,

our group is studying interaction of microbial cells (yeast and bacteria) to
several kinds of biomaterials. We conduct physico/chemical analysis of the
involved surfaces (mainly throgh surface thermodynamical analysis: contact
angles with several liquids) and have also an atomic force microscopy for
high resolution mapping of the surface topography and force measurements.

At this moment, we are interested in seeing what is happening with the
contact side of the cell with the substratum. For this reason, we are now
interested in applying optical methods to analyse cell deposition/adhesion,
in order to complete a set of experiments already performed with other
techniques with Candida, Enterococcus and Staphyloccocus strains.

I am planning now to acquire such a type of instrument, and I am specially
interested in

1. Total internal reflection microscopy
2. Confocal Laser scanning microscopy (CLSM)

I would very much appreciate your advice on which of these two techniques
have been proven to be more useful for this kind of experiments, and also
advice on some good and cost-effective equipment (model).

Of course if some of you have already experience in this kind of experiments
and are open to a collaboration to get more insight into these adhesion
phenomena, I will be mostly grateful if you contact me to discuss it
further.

Best wishes,

Antonio Méndez Vilas
Interfacial Phenomena and Biosurfaces Group
Department of Physics
Universidad de Extremadura
Avda de Elvas s/n
06001 Badajoz
SPAIN
E-mail: amvilas-at-unex.es

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 7 22:33:37 2004

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I miss that orange paint! I used to work on it when was in Germany! I
hope you'll find good home for it. Sergey

At 10:39 AM 1/8/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Sun Feb 8 20:11:24 2004

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The simplest IRM is with a confocal in refelction mode. We do both
widefield and confocal (BioRad Radiance 2000 and Leica AOBS); the latter
method is simpler even taking into account the possibility of regular
reflectance muddying the interpretation.

Confocal may be fine for thick samples. With thin samples the resolution
in the Z axis is insufficent to know whether you really are at the
substrate.

If the substrate materials are thin, transparent, uniform and the index of
refraction different enough from the sample, maybe fluorescence with TIRF
could be a way to go.

-Michael Cammer

___________________________________
WORK: http://www.aecom.yu.edu/aif/
PERSONAL: http://www.art-studio.us/

On Sun, 8 Feb 2004, Advanced Materials wrote:

} Search the CONFOCAL archive at
} http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
}
} Hi,
}
} our group is studying interaction of microbial cells (yeast and bacteria) to
} several kinds of biomaterials. We conduct physico/chemical analysis of the
} involved surfaces (mainly throgh surface thermodynamical analysis: contact
} angles with several liquids) and have also an atomic force microscopy for
} high resolution mapping of the surface topography and force measurements.
}
} At this moment, we are interested in seeing what is happening with the
} contact side of the cell with the substratum. For this reason, we are now
} interested in applying optical methods to analyse cell deposition/adhesion,
} in order to complete a set of experiments already performed with other
} techniques with Candida, Enterococcus and Staphyloccocus strains.
}
} I am planning now to acquire such a type of instrument, and I am specially
} interested in
}
} 1. Total internal reflection microscopy
} 2. Confocal Laser scanning microscopy (CLSM)
}
} I would very much appreciate your advice on which of these two techniques
} have been proven to be more useful for this kind of experiments, and also
} advice on some good and cost-effective equipment (model).
}
} Of course if some of you have already experience in this kind of experiments
} and are open to a collaboration to get more insight into these adhesion
} phenomena, I will be mostly grateful if you contact me to discuss it
} further.
}
} Best wishes,
}
} Antonio Méndez Vilas
} Interfacial Phenomena and Biosurfaces Group
} Department of Physics
} Universidad de Extremadura
} Avda de Elvas s/n
} 06001 Badajoz
} SPAIN
} E-mail: amvilas-at-unex.es
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 06:57:25 2004

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Dear Colleagues,
I would like to ask you for advice regarding the following problem:
We are trying to section (preferentially cryo section) a highly porous
collagen
scaffold (sponge like) soaked with water.
Problem 1: We have tried to make 8-12 µm cryo sections, but
unfortunately the section always collapses. Sectioning pFA fixed
collagene scaffold

was also not successful.
Problem 2: Apart from this it is not possible to keep it fixed on

a slide during antibody staining procedures.

Does anybody have experience with such a “difficult” object?

Which other fixation method could be used to make the sponge stiffer to
improve integrity of the sections?

Any suggestions would be helpful,

thanks in advance

Daniel.

--
(-)-(-)
--------------------------- \"/ ---
Dr. Daniel Eberhard =V=

Developmental Biology
& Molecular Pathology

Graduate Programe on Pattern Formation

University of Bielefeld
D 33501 Bielefeld/Germany

FAX: xx49(0)521-106-5654 (-)-(-)
--------------------------- \"/ ---
=V=

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 08:42:17 2004

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Daniel

about 15 years ago i did thin cross sections of cells grown on filter
inserts coated with collagen. there was no end of trouble, especially
at the interface of the filter and cells. after investigation i
discovered that the species of collagen used, type IV, was actually
quite hydrophilic. i ascribed my problems to interference with the
whole processing system. no matter how hard i tried, it looked like i
could not infiltrate through and across the barrier. i never did try
any water based resins, though. i have durcupan around and it would
have been easy to confirm.

i do not know if the hydrophilicity/hydrophobicity of the collagen type
you are using could be a factor in your preparation methods, but you
might want to check it out.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 09:54:54 2004

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You need a professional photo lab that will develop the the film the
way you want it done, not with whatever film developer they have on
hand. Custom black and white services might cost more than you expect,
shop around. Select a few labs (if you can't find a lab go to a photo
shop that caters to professionals, Jessops or Robert White, and ask
them) and show them what you have and what you want. You may find it is
faster, easier, cheaper and more consistant to learn to process the film
yourself. Fancy equipment with nitrogen burst agitation is not
necessary, fresh chemicals, film racks, several tanks and a light-tight
room with a sink is all you need.

Geoff

McGovern, Gillian wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 10:34:04 2004

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You might also consider sending your negatives to an EM lab that would
agree to process them for you. First, the lab should have all the
proper sized holders, etc. Second, they are probably already familiar
with this #$&%^$!!! film. Third, they may very well charge
substantially less than a custom black and white processor would.

Just a thought.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---Nano's R'Us!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

-----Original Message-----
} From: Geoff McAuliffe [mailto:mcauliff-at-umdnj.edu]
Sent: Monday, February 09, 2004 1:05 PM
To: McGovern, Gillian
Cc: 'Microscopy-at-MSA.Microscopy.Com'

You need a professional photo lab that will develop the the film the

way you want it done, not with whatever film developer they have on
hand. Custom black and white services might cost more than you expect,
shop around. Select a few labs (if you can't find a lab go to a photo
shop that caters to professionals, Jessops or Robert White, and ask
them) and show them what you have and what you want. You may find it is
faster, easier, cheaper and more consistant to learn to process the film

yourself. Fancy equipment with nitrogen burst agitation is not
necessary, fresh chemicals, film racks, several tanks and a light-tight
room with a sink is all you need.

Geoff

McGovern, Gillian wrote:

} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 10:58:57 2004

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Fellow List Members,

Members in the Greater New York City area are cordially invited to "Cryoultramicrotomy Techniques for The Biomedical and Biological Sciences."

When:
Thursday, Feb. 26, 9:30am - 5:00pm
Friday, Feb. 27, 9:30am - 2:00pm

Where:
Forcheimer Building, 3rd Floor Lecture Hall
Albert Einstein College of Medicine of Yeshiva University
1300 Morris Park Avenue
Bronx, NY

What:
A two-day "mini-workshop" with lectures, guest speakers, presentations, demonstrations and hands-on sessions for cryoultramicrotomy and associated techniques (cryo tool making, glass knife making, evaluation of glass knives, care and cleaning of diamond knives, operation of the ultramicrotome and immunoelectronmicroscopy).

Important Info:
Attendance is open for all of the presentations and demonstrations on Thursday, February 26th. However, attendance is limited for the cryoultramicrotomy hands-on sessions on Friday, February 27th.

Contacts:
For additional details, to RSVP or to reserve a spot for the hands-on sessions, please contact either Gloria Stephney at Albert Einstein College of Medicine ( {stephney-at-aecom.yu.edu} , 718.430.4027) or Kim Megaw at Boeckeler Instruments, Inc. ( {Kim-at-boeckeler.com} , 800.552.2262).

Sponsors and Organizers:
RMC Products Group, Boeckeler Instruments, Inc.,
Albert Einstein College of Medicine and
The New York Society of Experimental Microscopists (NYSEM).

Hope to see you there!

Bob Chiovetti
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 11:55:37 2004

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Sorry, but I have to disagree with Geoff about the last part of his
message:
with the new formulation of the 4489 film, a nitrogen burst system seems
to be necessary. We have discussed problems with the 4489 film before
on this listserver, and the main conclusion seemed to be that proper
agitation during development was crucial to get good results. If I
recall well, all the people who use appropriate agitation system (like
we do in our lab) seemed to avoid the problems that have been reported
with the 4489 films. When it comes to quality of development, I don't
agree
that we should go for the cheapest or easiest option, but instead look
for reproducibility and quality.

Marc

On Monday, February 9, 2004, at 02:04 PM, Geoff McAuliffe wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} You need a professional photo lab that will develop the the film
} the way you want it done, not with whatever film developer they have
} on hand. Custom black and white services might cost more than you
} expect, shop around. Select a few labs (if you can't find a lab go to
} a photo shop that caters to professionals, Jessops or Robert White,
} and ask them) and show them what you have and what you want. You may
} find it is faster, easier, cheaper and more consistant to learn to
} process the film yourself. Fancy equipment with nitrogen burst
} agitation is not necessary, fresh chemicals, film racks, several tanks
} and a light-tight room with a sink is all you need.
}
} Geoff
}
} McGovern, Gillian wrote:
}
} } ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------
} } ---------
} }
} }
} } I'm having serious problems achieving adequate development of the new
} } Kodak
} } 4489 EM film. We have no facilities to carry out development on site
} } and
} } have to send film packages to another lab, subsequently, the quality
} } of
} } development is at the discretion of the other (non-commercial) lab.
} } Basically its a hit or miss even using new development protocols. Its
} } got to the stage Id be willing to send our film anywhere in the UK
} } (maybe Europe) to be developed commercially if consistently good
} } quality can
} } be achieved. Does anyone know of somewhere which offers this service?
} }
} } Thanks.
} }
} } Veterinary Laboratories Agency (VLA)
} }
} } This email and any attachments is intended for the named recipient
} } only. Its
} } unauthorised use, disclosure, storage or copying is not permitted. If
} } you have
} } received it in error, please destroy all copies and inform the
} } sender. Whilst this
} } email and associated attachments will have been checked for known
} } viruses
} } whilst within VLA systems we can accept no responsibility once it has
} } left our
} } systems. Communications on VLA's computer systems may be monitored
} } and/or recorded to secure the effective operation of the system and
} } for other
} } lawful purposes.
} }
} }
} }
}
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 12:28:10 2004

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Hi Marc:

In my hands, nitrogen burst is not needed to get good results with
the new 4489 film. I use fresh chemicals (mixed in distilled water),
proper temperature, and agitation by hand. I agree that quality and
consistancy is the top priority which is why I suggested she learn to do
it at her facility.
I know that problems with processing the new 4489 have been
discussed on this forum before, I just have not had any.

Geoff

Marc Pypaert wrote:

} Sorry, but I have to disagree with Geoff about the last part of his
} message:
} with the new formulation of the 4489 film, a nitrogen burst system seems
} to be necessary. We have discussed problems with the 4489 film before
} on this listserver, and the main conclusion seemed to be that proper
} agitation during development was crucial to get good results. If I
} recall well, all the people who use appropriate agitation system (like
} we do in our lab) seemed to avoid the problems that have been reported
} with the 4489 films. When it comes to quality of development, I don't
} agree
} that we should go for the cheapest or easiest option, but instead look
} for reproducibility and quality.
}
} Marc
}
}
} On Monday, February 9, 2004, at 02:04 PM, Geoff McAuliffe wrote:
}
} }
} }
} } -----------------------------------------------------------------------
} } -------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------
} } --------
} }
} } You need a professional photo lab that will develop the the film
} } the way you want it done, not with whatever film developer they have
} } on hand. Custom black and white services might cost more than you
} } expect, shop around. Select a few labs (if you can't find a lab go
} } to a photo shop that caters to professionals, Jessops or Robert
} } White, and ask them) and show them what you have and what you want.
} } You may find it is faster, easier, cheaper and more consistant to
} } learn to process the film yourself. Fancy equipment with nitrogen
} } burst agitation is not necessary, fresh chemicals, film racks,
} } several tanks and a light-tight room with a sink is all you need.
} }
} } Geoff
} }
} } McGovern, Gillian wrote:
} }
} } } ----------------------------------------------------------------------
} } } --------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } ----------------------------------------------------------------------
} } } ---------
} } }
} } }
} } } I'm having serious problems achieving adequate development of the
} } } new Kodak
} } } 4489 EM film. We have no facilities to carry out development on
} } } site and
} } } have to send film packages to another lab, subsequently, the
} } } quality of
} } } development is at the discretion of the other (non-commercial) lab.
} } } Basically its a hit or miss even using new development protocols.
} } } Its got to the stage Id be willing to send our film anywhere in the UK
} } } (maybe Europe) to be developed commercially if consistently good
} } } quality can
} } } be achieved. Does anyone know of somewhere which offers this service?
} } }
} } } Thanks.
} } }
} } } Veterinary Laboratories Agency (VLA)
} } }
} } } This email and any attachments is intended for the named recipient
} } } only. Its
} } } unauthorised use, disclosure, storage or copying is not permitted.
} } } If you have
} } } received it in error, please destroy all copies and inform the
} } } sender. Whilst this
} } } email and associated attachments will have been checked for known
} } } viruses
} } } whilst within VLA systems we can accept no responsibility once it
} } } has left our
} } } systems. Communications on VLA's computer systems may be monitored
} } } and/or recorded to secure the effective operation of the system and
} } } for other
} } } lawful purposes.
} } }
} } }
} } }
} }
} }
} }
} }
}
} --
} Marc Pypaert
} Department of Cell Biology
} Center for Cell and Molecular Imaging
} Ludwig Institute for Cancer Research
} Yale University School of Medicine
} 333 Cedar Street, PO Box 208002
} New Haven, CT 06520-8002
} TEL 203-785 3681
} FAX 203-785 7446
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 12:51:37 2004

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We have been manually agitating our films since we started and have had good luck.
We do a "lift-tilt rigt-tilt then tap down" about every 10 sec for the four minutes
of developing to get good negatives.
We also discovered (with help through the list-server) that using "Indicator
Stop-Bath" caused some streaking. Once we stopped using that and started washing
in running tap-water for 1 minute after developing and before "Rapid Fix", the
streaking went away.
My advise - make sure you agitate well - on a regular schedule.
Stan

Marc Pypaert wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Sorry, but I have to disagree with Geoff about the last part of his
} message:
} with the new formulation of the 4489 film, a nitrogen burst system seems
} to be necessary. We have discussed problems with the 4489 film before
} on this listserver, and the main conclusion seemed to be that proper
} agitation during development was crucial to get good results. If I
} recall well, all the people who use appropriate agitation system (like
} we do in our lab) seemed to avoid the problems that have been reported
} with the 4489 films. When it comes to quality of development, I don't
} agree
} that we should go for the cheapest or easiest option, but instead look
} for reproducibility and quality.
}
} Marc
}
} On Monday, February 9, 2004, at 02:04 PM, Geoff McAuliffe wrote:
}
} }
} }
} } -----------------------------------------------------------------------
} } -------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------
} } --------
} }
} } You need a professional photo lab that will develop the the film
} } the way you want it done, not with whatever film developer they have
} } on hand. Custom black and white services might cost more than you
} } expect, shop around. Select a few labs (if you can't find a lab go to
} } a photo shop that caters to professionals, Jessops or Robert White,
} } and ask them) and show them what you have and what you want. You may
} } find it is faster, easier, cheaper and more consistant to learn to
} } process the film yourself. Fancy equipment with nitrogen burst
} } agitation is not necessary, fresh chemicals, film racks, several tanks
} } and a light-tight room with a sink is all you need.
} }
} } Geoff
} }
} } McGovern, Gillian wrote:
} }
} } } ----------------------------------------------------------------------
} } } --------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } America
} } } To Subscribe/Unsubscribe --
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} } } On-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } ----------------------------------------------------------------------
} } } ---------
} } }
} } }
} } } I'm having serious problems achieving adequate development of the new
} } } Kodak
} } } 4489 EM film. We have no facilities to carry out development on site
} } } and
} } } have to send film packages to another lab, subsequently, the quality
} } } of
} } } development is at the discretion of the other (non-commercial) lab.
} } } Basically its a hit or miss even using new development protocols. Its
} } } got to the stage Id be willing to send our film anywhere in the UK
} } } (maybe Europe) to be developed commercially if consistently good
} } } quality can
} } } be achieved. Does anyone know of somewhere which offers this service?
} } }
} } } Thanks.
} } }
} } } Veterinary Laboratories Agency (VLA)
} } }
} } } This email and any attachments is intended for the named recipient
} } } only. Its
} } } unauthorised use, disclosure, storage or copying is not permitted. If
} } } you have
} } } received it in error, please destroy all copies and inform the
} } } sender. Whilst this
} } } email and associated attachments will have been checked for known
} } } viruses
} } } whilst within VLA systems we can accept no responsibility once it has
} } } left our
} } } systems. Communications on VLA's computer systems may be monitored
} } } and/or recorded to secure the effective operation of the system and
} } } for other
} } } lawful purposes.
} } }
} } }
} } }
} }
} }
} }
} }
}
} --
} Marc Pypaert
} Department of Cell Biology
} Center for Cell and Molecular Imaging
} Ludwig Institute for Cancer Research
} Yale University School of Medicine
} 333 Cedar Street, PO Box 208002
} New Haven, CT 06520-8002
} TEL 203-785 3681
} FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 14:14:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (lee4502us-at-yahoo.com) from
http://www.msa.microscopy.com/Ask-A-Microscopist.html on Monday,
February 9, 2004 at 11:05:16
---------------------------------------------------------------------------

Email: lee4502us-at-yahoo.com
Name: Sridhar Srinivasan

Organization: Anna University

Education: Graduate College

Location: Chennai, Tamilnadu, India

Question:
Our group is currently using an Optiphot 200 C microscope that is
fitted for episcopic investigation. I would like to include an
external lighting source (fiber optic maybe) to enable tranmitted
light microscopy. What are the issues (like lenses and apertures) I
need to be mindful of in order to set up a diascopic illumination
system? I look forward to your response. Thank you.
Sridhar

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 17:44:21 2004

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I am curious how other software handles 12 to 8 bit conversion of
data. Improvision apparently scales directly from 4096 to 255 and 0
to 0 regardless of the image data. It seems to me that you should
take the maximum value in 12 bits and scale that to 255 and the
minimum value and scale that to 0. Does other software do this
differently, or allow you control of the conversion process? I
thought that if you needed to highlight low and high values, it would
be nice to be able to do this interactively in the conversion process.
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 18:31:51 2004

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There are several different issues here, and hence different answers.
Autoscaling the image into an 8 bit space will give you the maximum contrast, but it
means that each picture will have a different relationship between the
original pixel value and the final result, which would make densitometry or anything
related to pixel value impossible to calibrate, so absolute conversion by
simple division would be preferred in that case. Also, of course, it is much
faster, taking only a single pass through the data and that just being a bit shift
instead of subtraction and division.

Further, there is no good reason to restrict the scaling process to linear.
You should perform any gamma correction, equalization, etc. on the full 12 bits
before truncating to 8, in order to lose as little of the precision as
possible.

But why do you want to go to 8 bits anyway? If you have a software package
that does not handle 12 bits directly, you would do better to multiply the data
up to a 16 bit range and preserve all of the information present. Most modern
programs, even the newest version of Photoshop, provide pretty full
capabilities for processing and measuring 16 bit per channel images.

====

In a message dated 2/9/04 6:59:35 PM, knecht-at-uconn.edu writes:

} I am curious how other software handles 12 to 8 bit conversion of
} data. Improvision apparently scales directly from 4096 to 255 and 0
} to 0 regardless of the image data. It seems to me that you should
} take the maximum value in 12 bits and scale that to 255 and the
} minimum value and scale that to 0. Does other software do this
} differently, or allow you control of the conversion process? I
} thought that if you needed to highlight low and high values, it would
} be nice to be able to do this interactively in the conversion process.

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 19:09:11 2004

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DEPARTMENT OF CHEMICAL ENGINEERING AND MATERIALS SCIENCE
UNIVERSITY OF CALIFORNIA-DAVIS

A postdoctoral position is available in the Electron Microscopy Facility
at the University of California-Davis (UCD). This position is tied to
the recent purchase of a 200kV Field-Emission JEOL 2500SE equipped with
Noran EDS and Gatan Imaging Filter, which will be installed at UCD in
May 2004. This microscope will support varied research programs within
the Nanophases in the Environment, Agriculture and Technology (NEAT)
initiative at UCD, with the successful postdoctoral candidate expected
to establish collaborative research efforts with both expert and novice
users of advanced electron microscopes. Successful candidates will be
recent Ph.D. graduates in physics, metallurgy, or materials science with
a sound background in the relevant materials issues and an ambition to
be part of a developing microscopy facility. Please send a resume and
publication list to Professor Nigel D. Browning at the address below.
Prior experience with the many analytical and imaging methods used in
both STEM and TEM is essential, and experience with the expectations of
multi-user facilities in the US is desirable. The position is for one
year initially, with possibilities existing for further years. It is
also expected that UCD will hire a full-time staff member to perform
similar duties in the very near future. Salary is commensurate with
experience.

Nigel D. Browning

Department of Chemical Engineering and Materials Science
University of California-Davis
One Shields Ave
Davis, CA 95616

AND

National Center for Electron Microscopy, MS 72-150
Lawrence Berkeley National Laboratory
Berkeley, CA 94720

Tel: 530-754-5358 (Davis)
510-486-4612 (NCEM)
Fax: 530-752-9554 (Davis)
510-486-5888 (NCEM)
e-mail: nbrowning-at-ucdavis.edu
ndbrowning-at-lbl.gov

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 9 19:10:55 2004

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DEPARTMENT OF CHEMICAL ENGINEERING AND MATERIALS SCIENCE
UNIVERSITY OF CALIFORNIA-DAVIS

A postdoctoral position is available in the Interface Physics Group at
the University of California-Davis (UCD) to work on novel developments
in ultrafast TEM. This position is linked to the major new program
being initiated at Lawrence Livermore National Laboratory (LLNL)
involving the development of a new dynamic TEM (DTEM) to study materials
with a time resolution in the nano- to femto-second regime. This
position is intended to initially spend 6-9 months in Berlin working on
the existing state-of-the-art instrument at TU-Berlin, before
transferring back to UCD/LLNL to work on a new instrument that will be
installed at LLNL. In addition to becoming expert in the use of the
DTEM, the aim of the first years work is to use the microscope to study
phase transformations. Successful candidates will be recent Ph.D.
graduates in physics, metallurgy, or materials science with a sound
background in the relevant materials issues and an ambition to be part
of a developing program pushing at the frontiers of interface science.
Please send a resume and publication list to Professor Nigel D. Browning
at the address below. Prior experience in STEM or TEM is essential.
However, consideration will be based on the candidates overall potential
for success in the field and applicants with prior experience in related
fields are encouraged to apply. The position is for one year initially,
with possibilities existing for further years. In addition, the dynamic
TEM project is expected to become a major new program at LLNL, offering
the strong possibility of a permanent staff position in the future.
Salary is commensurate with experience.

**********************************************************************************************

Nigel D. Browning, PhD

Professor of Materials Science
Department of Chemical Engineering and Materials Science
University of California-Davis
One Shields Ave
Davis, CA 95616

AND

National Center for Electron Microscopy, MS 72-150
Lawrence Berkeley National Laboratory
Berkeley, CA 94720

Tel: 530-754-5358 (Davis)
510-486-4612 (NCEM)

Fax: 530-752-9554 (Davis)
510-486-5888 (NCEM)

e-mail: nbrowning-at-ucdavis.edu
ndbrowning-at-lbl.gov

***********************************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 10 14:25:05 2004

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Below is the result of your feedback form
(NJZFM-ultra-55). It was submitted by
(alvarobq-at-fcien.edu.uy) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html
on Tuesday, February 10, 2004 at 12:29:00
---------------------------------------------------------------------------

Email: alvarobq-at-fcien.edu.uy
Name: alvaro d. olivera

Organization: sciences university

Education: Graduate College

Location: montevideo, montevideo, uruguay

Question: IĄm cutting 61 nm sections of rat nerve
tissue perfussion fixed and post fixed by
immersion in PAF 4% Glutaraldehyde 0,25% Picric
acid 15%.
embbedig media: LRWhite (SPI supplies) medium
grade just for use( include benzoyl peroxide)
whithout accelerator.
mounting: 300 mesh Ni grids whithout film, covered with Coat-Grid Pen.
buffer: PBS 0,1M + BSA 0,1% + Triton x-100 0,05%
The problem is after the immunoreaction whith
gold conjugate antibody...the sections looks too
much dry under the magnifying glass and 80% of
sections disappear. Even when we put the grid
into the T.E.M. the image is horrible, we canĄt
recognize nothing and we see a rare artifact what
i think itĄs a tissue rests stick over the grid.
staining: uranium acetate 2% water(milli-q)diluted.
Please, I need a solution for this problem.
hope for your reply, many thanks...Alvaro.
ATTN: the same tissue mounted over Cu grids and
stained whit uranium acetate and Pb citrate, NO
immunoreaction!!!, are great in T.E.M.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 10 14:25:08 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (guffey1-at-inter-linc.net) from
http://www.msa.microscopy.com/Ask-A-Microscopist.html on Tuesday,
February 10, 2004 at 12:43:10
---------------------------------------------------------------------------

Email: guffey1-at-inter-linc.net
Name: Jennifer Guffey

Organization: southwest missouri state university

Education: Undergraduate College

Location: springfield, missouri, USA

Question: why is the image dimmer when you switch from a low power to
a high power objective?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 10 14:25:01 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (zeriena-at-yahoo.com) from
http://www.msa.microscopy.com/Ask-A-Microscopist.html on Tuesday,
February 10, 2004 at 12:20:12
---------------------------------------------------------------------------

Email: zeriena-at-yahoo.com
Name: rose zareen george

Organization: quens college

Education: Undergraduate College

Location: flushing, NY,USA

Question: 1. in the objective 4x, what does the number .12
indicate(numerical Aparature)
(eg. for 10x this number is .25 and 20 it is .50 and so on..
2.how many micro meter per objective is 43x..

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 10 14:25:07 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mparthiban-at-rediffmail.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, February 10, 2004 at 12:41:32
---------------------------------------------------------------------------

Email: mparthiban-at-rediffmail.com
Name: Parthi

Organization: University of Manitoba

Title-Subject: [Microscopy] [Filtered] Bacterial Samples

Question: I need to send some pathogenic bacterial samples for SEM.
So I need to kill the bacteria with either formaldehyde or
gluteraldehyde before sending. Can any one say the concentration I
should use or where can i find the prodedure for sending bacterial
samples for electron microscopy.
Parthi

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 10 16:31:27 2004

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Alvaro:

When you use uncoated grids the first thing to change is the thickness of
your sections. Cut the sections so they are light-medium gold in color.
Your 61nm sections are too delicate and therefore when you do all of those
different incubations and washes they break(just staining them with UA and
lead doesn't have the same effect). Remember the LR White sections are
extremely hydrophilic and swell up when placed into any aqueous solution.

If you can, try using formvar coated nickel grids. The sections will stay
on and won't disappear or loosen with the formvar. I always use 200 mesh
formvar coated nickel grids for all my ImmunoEM labeling procedures.

One more thing is to be very careful not to let the grids become dry at any
time during the entire labeling procedure.

Good Luck!

Karen Bentley
Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

-----Original Message-----
} From: alvarobq-at-fcien.edu.uy [mailto:alvarobq-at-fcien.edu.uy]
Sent: Tuesday, February 10, 2004 3:28 PM
To: MicroscopyListserver

Below is the result of your feedback form
(NJZFM-ultra-55). It was submitted by
(alvarobq-at-fcien.edu.uy) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html
on Tuesday, February 10, 2004 at 12:29:00
---------------------------------------------------------------------------

Email: alvarobq-at-fcien.edu.uy
Name: alvaro d. olivera

Organization: sciences university

Education: Graduate College

Location: montevideo, montevideo, uruguay

Question: IĄm cutting 61 nm sections of rat nerve
tissue perfussion fixed and post fixed by
immersion in PAF 4% Glutaraldehyde 0,25% Picric
acid 15%.
embbedig media: LRWhite (SPI supplies) medium
grade just for use( include benzoyl peroxide)
whithout accelerator.
mounting: 300 mesh Ni grids whithout film, covered with Coat-Grid Pen.
buffer: PBS 0,1M + BSA 0,1% + Triton x-100 0,05%
The problem is after the immunoreaction whith
gold conjugate antibody...the sections looks too
much dry under the magnifying glass and 80% of
sections disappear. Even when we put the grid
into the T.E.M. the image is horrible, we canĄt
recognize nothing and we see a rare artifact what
i think itĄs a tissue rests stick over the grid.
staining: uranium acetate 2% water(milli-q)diluted.
Please, I need a solution for this problem.
hope for your reply, many thanks...Alvaro.
ATTN: the same tissue mounted over Cu grids and
stained whit uranium acetate and Pb citrate, NO
immunoreaction!!!, are great in T.E.M.

---------------------------------------------------------------------------

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 10 18:26:22 2004

Contents Retrieved from Microscopy Listserver Archives
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I can't speak for other software, but here is how we do this in analySIS:

Let me first make the observation, that (to my knowledge) there are no
monitors that can actually display more than 8 bit of gray levels. This
alone makes a bit reduction necessary for display purposes.
When we open an image that is more than 8 bit (12-bit or 16-bit, for
example), the software must calculate new values for the display which fall
between 0 and 255. We typically do that by matching the highest pixel value
with 255, the lowest to 0. There are some finer details that have to do with
hot and dead pixels, but I won't go into that. This automatically results in
a contrast maximized image on the screen.
At this point you have several options: 1) You can manipulate the underlying
image data, which are still 12 bit, and keep the way the data is displayed,
or 2) you keep the underlying data and change the way they are displayed.
Both have methods have their justifications.
When it comes to actually create an 8-bit image from the 12-bit original,
you only need to "read" the display data (which are 8-bit), and create a new
image. Done.

The question remains: should you do this conversion? In general, it is
better to keep the 12-bit image until the end of a process, and only convert
it to 8-bit if really necessary. There is definitely data loss during this
process, be it through rounding errors or range compression. My personal
rule of thumb: If you need to further analyze the image, don't change the
bit depth. If the image is only used for display (such as in a paper or on
the web), reducing the bit depth is probably not a big problem.

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: David Knecht [mailto:knecht-at-uconn.edu]
Sent: Monday, February 09, 2004 16:02
To: microscopy-at-sparc5.microscopy.com

I am curious how other software handles 12 to 8 bit conversion of
data. Improvision apparently scales directly from 4096 to 255 and 0
to 0 regardless of the image data. It seems to me that you should
take the maximum value in 12 bits and scale that to 255 and the
minimum value and scale that to 0. Does other software do this
differently, or allow you control of the conversion process? I
thought that if you needed to highlight low and high values, it would
be nice to be able to do this interactively in the conversion process.
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 12:23:29 2004

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Hello Listers,

I have just inherited an old LKB 2078 Histo Knifemaker. Not the instruction book, just the machine. It looks similar to a 7800, but very different at the same time.

Does anyone have a copy of the instruction book they can let me copy? Has anyone used one of these for making 45 degree knives with 10mm glass? Does this thing handle just like a 7800?

If you know anything about this 2078 please let me know.

On the "cutting" edge of science,

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 13:30:41 2004

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In a message dated 2/11/2004 1:31:14 PM Eastern Standard Time, patpxs-at-gwumc.edu writes:

} I have just inherited an old LKB 2078 Histo Knifemaker. Not the instruction book, just the machine. It looks similar to a 7800, but very different at the same time.
}
} Does anyone have a copy of the instruction book they can let me copy? Has anyone used one of these for making 45 degree knives with 10mm glass? Does this thing handle just like a
} 7800?
}
} If you know anything about this 2078 please let me know.
}
} On the "cutting" edge of science,
}
} Paula :-)

Hi Paula,

Sorry, I can't help on the manual. Maybe someone else can?

Unless I'm mistaken, the 2078 was used to make Ralph knives from rectangles (thus it was called the "2078 Histo" knifemaker).

The stage may not be set up for triangular knives, but I suppose you could get creative and make some homemade guides that might make triangular knives.

As far as glass thickness, most of the LKB vintage instruments had trouble with glass that was thicker than about 6 - 8mm. Don't know if it's going to have enough "oomph" to break 10mm glass. I'd suspect not, though.

Hope the above info isn't completely useless!

Bob Chiovetti

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 14:52:50 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello Paula,

I have the directions for this instrument and will mail a xerox copy to you.

You should have it in a couple days.

JB

} I have just inherited an old LKB 2078 Histo Knifemaker. Not the
} instruction book, just the machine. It looks similar to a 7800, but
} very different at the same time.
}
} Does anyone have a copy of the instruction book they can let me
} copy? Has anyone used one of these for making 45 degree knives with
} 10mm glass? Does this thing handle just like a 7800?
}
} If you know anything about this 2078 please let me know.
}
} On the "cutting" edge of science,
}
} Paula :-)
}
} Paula Sicurello
} George Washington Univ. Medical Center
} Electron Microscope Lab
} Washington, DC 20037
} 202-994-2930 phone
} 202-994-2518 fax

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 15:18:58 2004

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Jennifer,
Assuming that the light source intensity is held constant, this is one
way to look at it.

1.) At the lower mag you are accepting light from a given circle (the
field of view) and then projecting that light onto a much larger circle
(your retina, or a piece of film). The intensity is reduced by the
ratio of the areas of the 2 circles.

2.) At the higher mag you are accepting light from a smaller circle
but projecting it onto the same size circle as before, hence the further
reduction in brightness at higher magnifications.

In terms of conservation of energy (assuming no losses due to the
optics, and that the aperture is the same size) the amount of light
available from the field of view is equal to the area x intensity. That
same amount of light is then spread over a larger area to give you your
magnified image. The intensity at that circle is the total light/area.
As your magnification increases, the area illuminated decreases in an
inverse square relationship, i.e. if you double your magnification you
will have 1/4 the area and therefore 1/4 the total light available to
spread over your retina or film. That is why things look darker, or
need stronger illumination, at higher magnifications.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

by way of MicroscopyListServer wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
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}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (guffey1-at-inter-linc.net) from
} http://www.msa.microscopy.com/Ask-A-Microscopist.html on Tuesday,
} February 10, 2004 at 12:43:10
} ---------------------------------------------------------------------------
}
}
} Email: guffey1-at-inter-linc.net
} Name: Jennifer Guffey
}
} Organization: southwest missouri state university
}
} Education: Undergraduate College
}
} Location: springfield, missouri, USA
}
} Question: why is the image dimmer when you switch from a low power to
} a high power objective?
}
} ---------------------------------------------------------------------------
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 15:25:56 2004

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A very good description of numerical aperture can be found on:

http://microscopy.fsu.edu/primer/anatomy/numaperture.html

and the magnification question would be covered by:

http://micro.magnet.fsu.edu/primer/anatomy/magnification.html

They may seem a bit complicated, but that's the way light microscopes work!
Best is if you can put a graticule on the specimen stage; this graticule
might be marked in divisions of 10 micrometers from 0 to 1 millimeter, and
then compare that with your image in some way. If you're not taking
photographs, one way is to put in an eyepiece with its own graticule inside,
and then count how many divisions in the eyepiece graticule correspond to,
say, 0.1 mm in the specimen graticule.

-----------------------------------
Robert H. Olley
Reply to: R.H.Olley-at-reading.ac.uk
URL: http://www.rdg.ac.uk/~spsolley
-----------------------------------

} From: zeriena-at-yahoo.com (by way of MicroscopyListServer)
} To: MicroscopyListserver {microscopy-at-msa.microscopy.com}
} Subject: [Microscopy] AskAMicroscopist: LM question about Lenses
} Date: Wed, 11 Feb 2004 07:27:37 +1100
}
}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

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From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 16:02:21 2004

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Hello All,

For years, I have been using Kimble "Opticlear" 5 dram vials with a *closed
bottom* poly stopper to store my 12.5mm pin-style SEM (Etec)
stubs/specimens. The pin can be pushed into the bottom of the closure,
making the stopper hold the stub. Works well - More or less airtight,
cheap, and suspends the specimen out of harm's way. I still use the pin
stubs with an adapter for my Hitachi SEM. I also use a lot of similar stubs
with a 25.4mm diameter.

I have never found a similar vial (closed bottom poly stopper) that is large
enough to accept my 25.4mm stubs. I am aware of commercially available
plastic boxes (w/inserts), but they are very expensive for what you get and
do little to protect specimens.

Any ideas about where to find large vials similar to the small ones (with
closed bottom cap)?

Thanks,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 16:23:05 2004

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I have an older Leitz Pol microscope that has served me well for many years.
I've taken thousands of photographs of mineral thin sections in polarized
light. Recently I fitted the scope with a Coolpix digital camera and noticed
a "spot" in the center of the image that was lighter and had a greenish
cast. After virtually disassembling the scope looking for the source of the
problem, I finally discovered that it is only present when I cross the
polars (Nicol prisms). Examination of the prisms shows a faint pale colored
spot in the center of both the substage polarizer and the swing-in analyzer.
I never detected this problem with film, but it is decidedly evident with
the digital camera. I can remove and replace the polarizer, but still have
the spot because of the analyzer. Can anyone suggest a retrofit for the
analyzer using modern polaroid or some other technique? I love the Nicols,
but can't live with the spot.

Henry Barwood
Associate Professor of Science, Earth Science
Department of Math and Physics
MSCX 312G
Troy State University
Troy, Alabama 36082
hbarwood-at-troyst.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 16:25:21 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (cmeyer911-at-yahoo.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, February 10, 2004 at 17:51:43
---------------------------------------------------------------------------

Email: cmeyer911-at-yahoo.com
Name: Chris Meyer

Organization: Boeing

Title-Subject: [Microscopy] [Filtered] TEM Electrolyte Procedure Requested

Question: Hello,

I'm looking for a titanium electropolish procedure that does not
include perchloric acid. I have perchloric, and a procedure for it,
but I'm looking for alternatives for safety reasons.

The alloy is Ti-5Al-5V-5Mo-3Cr and will have alpha and beta phase.
I'm looking for electrolyte recipie, temperature and voltage.

Thank you.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 16:25:24 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (iand-at-clemson.edu) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, February 10, 2004 at 15:49:23
---------------------------------------------------------------------------

Email: iand-at-clemson.edu
Name: ian davenport

Organization: clemson university

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi
I would like to trace the general pathway from blood vessels through
the follicle cells and in to the oocyte, though various stages in
oogenesis. I am not looking for any specific protien/molecule, I just
want to prove/show that something travels through the follicle cell,
across the zona pellucida into the egg. it will need to cross at
least one membrane,(into the follicle cell.

I would like to use fluorescence or TEM.
Any suggestions please.
thanks
ian

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 11 16:25:28 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (ldemp-at-mse.ufl.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Wednesday, February 11, 2004 at 08:12:08
---------------------------------------------------------------------------

Email: ldemp-at-mse.ufl.edu
Name: Luisa Amelia Dempere

Organization: University of Florida

Title-Subject: [Microscopy] [Filtered] MListserver: SEM-TEM Workshop

Question: Dear all:
The Latin American School of Electron Microscopy (LASEM), sponsored
by the Committee of Inter American Societies for Electron Microscopy
(CIASEM), will be offering a 3-day workshop at the University of
Central Florida in Orlando from March 10 to March 12. This workshop
is part of the 2004 Joint Symposium of the Florida Chapter of the AVS
Science and Technology Society (FLAVS), the Florida Society for
Microscopy (FSM) and the Florida Section of the American Ceramic
Society (FL-ACerS). The 3-day workshop includes fundamentals and
applications of Scanning Electron Microscopy (SEM), Transmission
Electron Microscopy (TEM) and associated techniques. A certificate of
attendance will be given to all participants. For more information
and registration please visit the symposium web-page at www.flavs.org
and go to the LASEM workshop link (www.flavs.org/LASEM.htm).

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From MicroscopyL-request-at-ns.microscopy.com Thu Feb 12 09:42:58 2004

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This comes up every year in my histology class:

Are all Pseudostratified columnar epithelial cells ciliated? I think so
but I don't want to say so based on a gut feeling. Does anyone know of a
pseudostratified epithelium that is not ciliated?

The converse is not true (i.e., not all cilia are on pseudostratifed
epithelium since the oviduct has cilia on its simple columnar epithelium).

Thanks, Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 12 10:26:04 2004

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Hi Ian:

Hmmm...... sort of a ...... (searching for the right word here and
not finding it) .... question. Since the oocyte does not exist in a
vacuum it must be nourished somehow. How else if not via the follicular
cells? I think you need to be more specific. Do you want to show that
only certain things go into oocytes? Is this some sort of class project
(design an experiment to demonstrate xyz) or ? TEM and fluorescence are
very different tools with very different capabilities, pick one.

Geoff

by way of MicroscopyListServer wrote:

} ---------------------------------------------------------------------------
}
}
} Email: iand-at-clemson.edu
} Name: ian davenport
}
} Organization: clemson university
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: Hi
} I would like to trace the general pathway from blood vessels through
} the follicle cells and in to the oocyte, though various stages in
} oogenesis. I am not looking for any specific protien/molecule, I just
} want to prove/show that something travels through the follicle cell,
} across the zona pellucida into the egg. it will need to cross at least
} one membrane,(into the follicle cell.
}
} I would like to use fluorescence or TEM.
} Any suggestions please.
} thanks
} ian
}
} ---------------------------------------------------------------------------
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 12 10:52:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We not sure from your data that this is an application for Mercox, but it
just might be. I'll refer you to a paper by Dr. Fred Hossler at East
Tennessee who's got great experience with Mercox. Read the paper and see if
it is what you are looking for.
See
http://www.laddresearch.com/Key_Products/Mercox/HosslerPaper/hosslerpaper.ht
ml

John Arnott

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com
----- Original Message -----
} From: "by way of MicroscopyListServer" {iand-at-clemson.edu}
To: "MicroscopyListserver" {microscopy-at-msa.microscopy.com}
Sent: Wednesday, February 11, 2004 5:23 PM

Hi Tom:

I would say yes, all pseudostratified cloumnar epithelia are
ciliated. By that I mean each cell has at least one cilium. I have seen
(via TEM) cilia on many types of epithelia (simple cuboidal and simple
columnar) that are not normally thought of as ciliated. I read something
recently (don't remember where) that the cilium is a polarity signal for
cell orientation and cell division.

Geoff

Tom Phillips wrote:

} This comes up every year in my histology class:
}
} Are all Pseudostratified columnar epithelial cells ciliated? I think
} so but I don't want to say so based on a gut feeling. Does anyone
} know of a pseudostratified epithelium that is not ciliated?
}
} The converse is not true (i.e., not all cilia are on pseudostratifed
} epithelium since the oviduct has cilia on its simple columnar
} epithelium).
}
} Thanks, Tom
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 12 13:13:14 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear all,

I have a couple questions regarding the illumination stability of mercury
burners:

1- When a new burner is installed, is there a period of time (within a few
hours) where the intensity increases to a plateau? With an older lamp,
everytime we turn the lamp on, we have observed that it takes about 40
minutes to reach a plateau. We installed a new burner recently, and images
have been brighter from day to day for the first 3 days and remained stable
afterwards. Is it just a coincidence?

2- To solve the stability problems we have with the mercury burners, we’re
considering the use of xenon lamps. Is there somewhere a comparative
stability study of the 2 types of burners?

Thank you.

Marie-Claude Belanger

_________________________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Thu Feb 12 14:07:28 2004

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Since I will be giving the histology lecture on the male reproductive
system to medical students in a couple of weeks, I should mention that one
of the classic pseudostratified columnar epithelia, that of the epididymis,
has abundant long microvilli ("stereocilia" to the old classical
microscopists) at the apical surface but, to my knowledge, no cilia. Of
course, I can't exclude the possibility that a single cilium is hidden away
somewhere among all those microvilli. --Kent

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
A. Kent Christensen, Professor Emeritus
Department of Cell and Developmental Biology, Medical Science II Building
University of Michigan Medical School, Ann Arbor, MI 48109-0616
Tel (work) (734) 763-1287, Fax (work) (734) 763-1166
akc-at-umich.edu http://www.umich.edu/~akc/
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

--On Thursday, February 12, 2004 1:23 PM -0800 Geoff McAuliffe
{mcauliff-at-umdnj.edu} wrote:

}
} Hi Tom:
}
} I would say yes, all pseudostratified cloumnar epithelia are
} ciliated. By that I mean each cell has at least one cilium. I have seen
} (via TEM) cilia on many types of epithelia (simple cuboidal and simple
} columnar) that are not normally thought of as ciliated. I read something
} recently (don't remember where) that the cilium is a polarity signal for
} cell orientation and cell division.
}
} Geoff
}
} Tom Phillips wrote:
}
} } This comes up every year in my histology class:
} }
} } Are all Pseudostratified columnar epithelial cells ciliated? I think
} } so but I don't want to say so based on a gut feeling. Does anyone
} } know of a pseudostratified epithelium that is not ciliated?
} }
} } The converse is not true (i.e., not all cilia are on pseudostratifed
} } epithelium since the oviduct has cilia on its simple columnar
} } epithelium).
} }
} } Thanks, Tom
} }
} } Thomas E. Phillips, PhD
} } Professor of Biological Sciences
} } Director, Molecular Cytology Core
} } 3 Tucker Hall
} } University of Missouri
} } Columbia, MO 65211-7400
} }
} } 573-882-4712 (office)
} } 573-882-0123 (fax)
} } PhillipsT-at-missouri.edu
} }
} **********************************************
} Geoff McAuliffe, Ph.D.
} Neuroscience and Cell Biology
} Robert Wood Johnson Medical School
} 675 Hoes Lane, Piscataway, NJ 08854
} voice: (732)-235-4583; fax: -4029 mcauliff-at-umdnj.edu
} **********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 12 14:45:12 2004

Contents Retrieved from Microscopy Listserver Archives
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} Dear Tom and Geoff,
Tom's referring, I think, to the primary cilium, see-
http://www.bowserlab.org/primarycilia/ciliumpage2.htm or
http://www.primary-cilium.co.uk/ - this is web site relating to the
primary cilium (called by some the 'forgotten organelle'), which is
found, as I recently learned, in most mammalian cells.

Regards,

Richard

} Hi Tom:
}
} I would say yes, all pseudostratified cloumnar epithelia are
} ciliated. By that I mean each cell has at least one cilium. I have
} seen (via TEM) cilia on many types of epithelia (simple cuboidal and
} simple columnar) that are not normally thought of as ciliated. I read
} something recently (don't remember where) that the cilium is a
} polarity signal for cell orientation and cell division.
}
} Geoff
}
} Tom Phillips wrote:
}
} } This comes up every year in my histology class:
} }
} } Are all Pseudostratified columnar epithelial cells ciliated? I think
} } so but I don't want to say so based on a gut feeling. Does anyone
} } know of a pseudostratified epithelium that is not ciliated?
} }
} } The converse is not true (i.e., not all cilia are on pseudostratifed
} } epithelium since the oviduct has cilia on its simple columnar
} } epithelium).
} }
} } Thanks, Tom
} }
} } Thomas E. Phillips, PhD
} } Professor of Biological Sciences
} } Director, Molecular Cytology Core
} } 3 Tucker Hall
} } University of Missouri
} } Columbia, MO 65211-7400
} }
} } 573-882-4712 (office)
} } 573-882-0123 (fax)
} } PhillipsT-at-missouri.edu
} }
} }
} }
}
} --
} --
} **********************************************
} Geoff McAuliffe, Ph.D.
} Neuroscience and Cell Biology
} Robert Wood Johnson Medical School
} 675 Hoes Lane, Piscataway, NJ 08854
} voice: (732)-235-4583; fax: -4029 mcauliff-at-umdnj.edu
} **********************************************
}
}
}
}
}
Richard Easingwood
Otago Centre for Electron Microscopy
c/- Department of Anatomy & Structural Biology
University of Otago
ph: 0064 3 479 7301
fax: 0064 3 479 7254
cell: 021 222 4759

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 06:13:03 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Jennifer,

The intensity you see through different objective lenses does not only
depend on the magnification of the lens, but also its numerical aperture,
which, roughly speaking, is how wide is the cone of rays entering the lens.
Here are some values for a set of polarizing lenses we use:

n.a. mag n.a./mag squared
0.08 2.5 0.032 0.001024
0.22 10 0.022 0.000484
0.6 25 0.024 0.000576
0.85 40 0.02125 0.000452

If everything is set up correctly, then the intensity will be roughly
proportional to (n.a./mag)squared as in the last column. Generally, this
factor will decrease a bit with increasing lens power, but note that our 25x
lens is a bit better than the one above and below. This is because it is a
high quality Zeiss Neofluar lens.

However, these factors will only apply if you have a condenser which
delivers an even intensity of rays over the whole numerical aperture. For
example, the 0.63 n.a. condenser we normally use will not deliver a full
cone to the 40x lens, so things do appear noticeably dimmer in that one.

I'm don't know what kind of condenser you are using. One thing you can do
is to dim your light source somewhat, and then take out the eyepiece and
look down the tube. You will see a circle of light corresponding to the
cone of rays going through your lenses. If this is cut down by an aperture,
it may be that your higher power lenses are not getting their full ration in
terms of incoming cone of rays. Then things will appear noticeably dimmer,
and moreover you will not be getting the full resolution that your objective
lens is capable of.

One other thing if you are doing polarized light microscopy. If you have a
wide cone of rays coming through, say, a mineral rock section, then the
colour transmitted through the polarizing system will be different for
different path lengths through the specimen between the centre and outside
of the cone. This is why polarizing colours tend to look much more
wishy-washy through a high-power lens.

-----------------------------------
Robert H. Olley
Reply to: R.H.Olley-at-reading.ac.uk
URL: http://www.rdg.ac.uk/~spsolley
-----------------------------------

} From: guffey1-at-inter-linc.net (by way of MicroscopyListServer)
} To: MicroscopyListserver {microscopy-at-msa.microscopy.com}
} Subject: [Microscopy] [Filtered] AskAMicroscopist: Imaging question
} Date: Wed, 11 Feb 2004 07:29:07 +1100
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

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From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 06:46:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Thanks to everyone who replied with their suggestions to prevent image
retrieval failures.

There was one particular procedure which we were unaware of and most
Windows users do not seem to know this control feature. I would like to
pass this along to the group.

While the compact flash cards are typically read by USB devices and in
theory, are swappable, we have not had failures since software "ejecting"
the card. Some card readers require physically ejecting the card much like
the camera card eject. We simply pull the cards out of the card
readers. Apparently, Windows does not always know that the card has been
removed and that the files have changed, hence the files are corrupted and
not readable. The solution (hopefully in the long run) is go open My
Computer, right click on the card reader device and eject the card. While I
recalled seeing this previously, I did not think it was relevant. We never
had this problem with our USB jump drives.

I hope this helps everyone else who had similar problems.

Alan Stone
ASTON Metallurgical Services

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 08:01:34 2004

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So far as I know, the epithelium of the epididymus is pseudostratified,
with STEROCILIA (which are actually elongate microvilli). I do not
recall any descriptions - on it - of cilia, primary or otherwise. MRA

Mark R. Adelman, Ph.D.
Associate Professor of Anatomy, Physiology & Genetics
Uniformed Services University of the Health Sciences
4301 Jones Bridge Road
Bethesda, MD 20814-4799
USA
Phone: 301-295-3208
FAX: 301-295-1786
Email: madelman-at-usuhs.mil
Website: http://bicmra.usuhs.mil/
On Thursday, February 12, 2004, at 04:23 PM, Geoff McAuliffe wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Hi Tom:
}
} I would say yes, all pseudostratified cloumnar epithelia are
} ciliated. By that I mean each cell has at least one cilium. I have
} seen (via TEM) cilia on many types of epithelia (simple cuboidal and
} simple columnar) that are not normally thought of as ciliated. I read
} something recently (don't remember where) that the cilium is a
} polarity signal for cell orientation and cell division.
}
} Geoff
}
} Tom Phillips wrote:
}
} } This comes up every year in my histology class:
} }
} } Are all Pseudostratified columnar epithelial cells ciliated? I think
} } so but I don't want to say so based on a gut feeling. Does anyone
} } know of a pseudostratified epithelium that is not ciliated?
} }
} } The converse is not true (i.e., not all cilia are on pseudostratifed
} } epithelium since the oviduct has cilia on its simple columnar
} } epithelium).
} }
} } Thanks, Tom
} }
} } Thomas E. Phillips, PhD
} } Professor of Biological Sciences
} } Director, Molecular Cytology Core
} } 3 Tucker Hall
} } University of Missouri
} } Columbia, MO 65211-7400
} }
} } 573-882-4712 (office)
} } 573-882-0123 (fax)
} } PhillipsT-at-missouri.edu
} }
} }
} }
}
} --
} --
} **********************************************
} Geoff McAuliffe, Ph.D.
} Neuroscience and Cell Biology
} Robert Wood Johnson Medical School
} 675 Hoes Lane, Piscataway, NJ 08854
} voice: (732)-235-4583; fax: -4029 mcauliff-at-umdnj.edu
} **********************************************
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 09:30:36 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello,

I am contemplating attempting to assemble a UV fluorescence microscope. I
want Ex ~ 305 nm and Em ~350 to 400. I have found the necessary filters and
plan to assemble a set for ($800+), we have a quartz objective and UV lamp
and camera. My questions are... Is anyone imaging tryptophan fluorescence so
I can go there and try my idea before I spend a lot of money, or has anyone
ever tried to do this and can offer words of wisdom or caution.

thanks,
heather

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 12:40:25 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,
I have a request from a science museum to take a few SEM photos of a
microproceessor from a cell phone. I was wondering if anyone has any
recommendations on methods to remove the packaging material to get to the
actual silicon.

It looks like a Texas instruments chip with number MAD2WD1, if that helps.
Any comments appreciated.
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 13:02:19 2004

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Gordon;

I can give you very specific information on that. However, I must caution you that this procedure should only be performed in a fume hood, with full protective clothing, eyewear and someone with training in doing this..

The mold compound may be dissolved in a either red fuming nitric acid heated to +80C or a combination of 90% nitric/ 10% sulfuric. The process is by immersion. Bear in mind that this is a very hazardous procedure, so now that I told you some specifics, let me make an alternate suggestion. Simply take a "ceramic" device, one that has a soldered lid on it and grind the lid off. This way you won't have to deal with any of this dangerous material and I assure you that unless your audience are semiconductor engineers, they won't know one circuit from the next.

Let me know if there is something specific about this or if you just want to show the general construction of an IC. I have some archived photos I'd be happy to pass along if you'd simply need something as an example.

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Gordon Vrololjak [mailto:gvrdolja-at-nature.Berkeley.EDU]
Sent: Friday, February 13, 2004 1:51 PM
To: Microscopy-at-MSA.Microscopy.Com

Hello,
I have a request from a science museum to take a few SEM photos of a
microproceessor from a cell phone. I was wondering if anyone has any
recommendations on methods to remove the packaging material to get to the
actual silicon.

It looks like a Texas instruments chip with number MAD2WD1, if that helps.
Any comments appreciated.
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 17:10:49 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (sue.tyler-at-noaa.gov) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday,
February 13, 2004 at 13:30:11
---------------------------------------------------------------------------

Email: sue.tyler-at-noaa.gov
Name: Sue Tyler

Organization: Cooperative Oxford Laboratory

Title-Subject: [Microscopy] [Filtered] MListserver: neutralization of osmium tetroxide

Question: I recently submitted a container of neutralized
(2% Osmium in 20ml of corn oil)Osmium Tetroxide to
our waste disposal and safety person and it was rejected.
The reason for the rejection was that we are not licensed to
treat our waste in this facility. Has anyone else run into
this problem? I would think that it would be safer to have
it neutralized in case of a spill etc. Any opinions would
be nice.

Reference: Cooper, K. (1988) Neutralization of
Osmium Tetroxide in case of accidental spillage
and for disposal.
Bulletin of The Microscopical Soxiety of Canada. 8:24-28

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 13 17:30:46 2004

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we also are not allowed to treat our used materials (we aren't allowed to
call it waste). we can do something as part of an approved
protocol. maybe you need to "test" your osmium is reactive afterwards by
putting it in corn oil and see if it turns black! that makes it part of
the experiment and not part of the disposal. see if that is an approved
reason for doing what you do.

At 07:14 AM 2/14/2004 +0800, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 14 18:11:08 2004

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A postdoctoral position is available to work on problems
related to surface reconstructions, charge density and electron
crystallography. A strong background in electron microscopy
is necessary. Additional experience in UHV equipment, and
strong computer skills and expertise in density functional
methods would be positive points.

-----------------------------------------------
Laurence Marks
Department of Materials Science and Engineering
Northwestern University
Evanston, IL 60201, USA
Tel: (847) 491-3996 Fax: (847) 491-7820
mailto:ldm2-at-risc4.numis.nwu.edu
http://www.numis.nwu.edu
-----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Feb 15 16:39:53 2004

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Dear Rose,

Yes, the number after the magnification is the magnification is the Numerical Aperture or NA.

Three quick equations which you might find helpful.

1. NA = n sin a
where
n = refractive index of the immersing liquid between the top of the sample and the front element of the lens
a = 1/2 of the collecting angle of the objective

From this equation, you can quickly see that, the larger the collecting angle, the greater the NA.
Also, the refractive index of air is 1.00, so using immersing fluids like water (1.33), glycerin (1.47), or immersion oil (1.5212) has tremendous effect on improving the NA. Reminder: use only the fluid for which the lens is engineered. Trying to use immersion oil with a "dry" (air) objective, is a disaster. Lenses built for immersing liquids are specially sealed so that the liquid does not creep into the internal construction of the lenses.

2. Why is NA important? The reasons are derived from Diffraction Theory. Every object produces a diffraction pattern (see Young's slit experiments in any physics book for details). For simple objects like stage micrometers and diatoms like pleurasigma angulatum, you can see the diffraction pattern by removing the eyepiece and peering deep down the tube into the Back Focal Plane of the objective. (You also need to close down the condernser as far as it will go, to make the source of light a very small opening or, alternatively, remove it and put a pinhole over the light port in the base of your microscope). If the NA is big enough to capture 2 adjacent spots from the diffraction pattern, enough information is present to determine spacing in the original object. The basic equation for resolution summarizes:

Rxy = (1.22x wavelength)/ (NAobjective+NAcondenser).
R = the size (in the XY plane, typically in micrometers) of the smallest resolvable particle
1.22 = a shape function (assuming round apertures in the microscope)
Wavelength = you can use 500 nm or 0.500 micrometers as sort of the center of the visible spectrum
NA = real working NAs (note: just because a lens is engraved with a value, does not mean that that is the working NA. Closing down an iris in the back focal plane of the objective or closing down the condenser aperture iris reduces the real working NA).

If the NA is big enough to capture THREE adjacent diffraction spots (the set of -1/0/+1 only counts as 2), you will begin to get better edge definition. So, the bigger the NA, the smaller the particle that you can resolve and the better the edge quality will be.

3. As for your other question: micrometers
Are you referring to the working distance (distance from the front of the lense to the top of the sample) or Field of View?
If working distance: you can either measure that directly or can look up the specs in the literature from the manufacturer.
If Field of view (the diameter of the territory you see when looking through the eyepieces):
F. O. V = (field number)/Mobjective
The field number is the value written on the EYEPIECE, following the magnification. It refers to the distance across a small ridge or baffle typically mounted about 1/3 of the way up the inside wall from the BOTTOM of the eyepiece and typically ranges from about 18mm to 25 mm (old Reichert Polyvars and some others had ultra wide field of view and went to 32mm). Convert to micrometers by multiplying by 1000.
Mobjective is the Magnification of the OBJECTIVE multiplied by any other auxiliary lenses between the objective and the bottom of the eyepiece.
Ex: If you were working with eyepieces which had field number 22 (22 mm or 22,000 micrometers) and a 10x objective, the size of the field of view is simply 22,000/10 or 2,000micrometers.

Note: the eyepiece going to the camera is often a different magnification than the eyepieces you look through and the chip in the camera has its own equivalent of a "magnification", so what you see in the eyepieces will often be a larger FOV than you can capture with your camera.

You might find my book, "Optimizing Light Microscopy", helpful. A description and ordering information are on our website: www.MicroscopyEducation.com

Good hunting!
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^
Don't forget: the American Chem Society's Applied Optical Microscopy Course, March 5-7, Chicago, Ill.
Visit our website for details and registration. NOT JUST FOR CHEMISTS!!!!
^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^
Best regards

At 07:27 AM 2/11/04 +1100, zeriena-at-yahoo.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Sun Feb 15 17:55:47 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I am looking for the make and size of the Ion pump that is on the Philips
CM12.
It seems easier to ask rather than pull the covers off the scope as the EDS
is in the way.

I am also looking for any used PSEM 75's for sale
Please contact me at the below e-mail address.

Thanks in advance
Hank Beebe

Manager Instrument Services
hbeebe-at-rjlg.com
RJLee Group, Inc.
350 Hochberg Rd.
Monroeville, PA 15146
(724) 325-1776 voice
(724) 733-1799 fax

From MicroscopyL-request-at-ns.microscopy.com Sun Feb 15 18:44:43 2004

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Colleagues

Just a reminder the deadline for submitting papers to the Microscopy
& Microanalysis 2004
meeting in Savannah is 17:00 PST , Monday Feb 16, 2004.

All the information you need to submit a paper is on-line at

http://mm2004.microscopy.org

Cheers...

Nestor
Your Friendly Neighborhood SysOp.

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 16 02:35:52 2004

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}
} 3DPTV 2004, Thessaloniki - Greece
} http://www.umiacs.umd.edu/conferences/3dpvt04/
}
}
============================================================================
}
} Call for Papers
}
} The second International Symposium on 3DPTV (3D Data Processing,
} Visualization, and
} Transmission) will be held on September 6 to 9, 2004 in the city of
} Thessaloniki, Greece.
}
} The goal of this meeting is to present and discuss new research ideas and
} results related to the capture, representation, compact storage,
} transmission, processing, editing, optimization and visualization or 3D
} data. These topics span a number of research fields from applied
} mathematics, computer science, and engineering: computer vision, computer
} graphics, geometric modeling, signal and image processing, bionformatics,
} and statistics.
}
} This symposium follows the highly successful 1st International Symposium
on
} 3D Data Processing, Visualization, and Transmission
} 3DPVT'02 (http://www.dei.unipd.it/conferences/3DPVT) which took place in
} 2003 in Padova, Italy. The proceedings of the symposium will be published
in
} the IEEE Proceedings Series, in cooperation with Eurographics and ACM
} SIGGRAPH.
}
} A list of topics of interest includes but is not limited to:
}
} - 3D scanning technologies and devices
} - 3D photography algorithms
} - 3D view registration and surface modeling
} - Surface reflectance recovery and modeling
} - 3D texture processing
} - Image-based rendering and modeling
} - Multi-view image and geometry processing
} - Stereo and motion reconstruction
} - Augmented reality
} - Compression, transmission and visualization of 3D data
} - 3D Content-based retrieval and recognition
} - Man/machine interaction with 3D data
} - 3D printing and rapid prototyping
} - Psychophysics of 3D sensing and haptics
} - 3D imaging in biomedicine
} - Structural analysis and pattern discovery in bioinformatics
} - 3D imaging in virtual heritage and virtual archeology
} - 3D imaging in e-commerce.
} - 3D Television
} - Teleimmersion and remote collaboration
}
} Paper submission
}
} Papers submitted for review must follow the IEEE CS Press Proceedings
} two-column format. The papers must be submitted for review in final form.
} The maximum paper length for review as well as for publication is 8 pages,
} including the bibliography and the figures. Electronic manuscripts must
be
} submitted in Adobe Acrobat PDF format. In exceptional circumstances,
} PostScript files will be accepted and converted to PDF: you must contact
the
} conference in advance if you intend to do so.
}
} The paper must have the full author contact information. All accepted
papers
} will be published in the Proceedings of the Symposium (on a CD-ROM).
} The symposium language will be English.
}
} Important Dates
}
} Abstracts : April 2
} Full Papers : April 7
} Reviews due : May 15
} Author notification : May 25
} Deadline for price
} reduced hotel
} booking : June 10
} Camera-ready Papers : June 15
} and Registration of at
} least one author per
} paper
}
} Hotel reservations : May 25 to August 30
} Registration deadline : June 30
} for reduced price
}
} Tutorials : September 6
} Symposium : September 7-9
}
}
}
} --------------------------------------------------------------------------
--
} ---
}
} General chairs
}
} - Aloimonos, Yiannis, University of Maryland, USA {yiannis-at-cfar.umd.edu}
} - Taubin, Gabriel, Brown University, USA {taubin-at-brown.edu}
}
} Finance and registration chair
}
} - Duraiswami, Ramani, University of Maryland, {ramani-at-umiacs.umd.edu}
}
} Local arrangements
}
} - Petrou, Maria {M.Petrou-at-ee.surrey.ac.uk}
} - Strintzis, Michael {strintzi-at-eng.auth.gr}
} - Mpountanour, Kalliope {kalm-at-iti.gr}
} - George Triantafyllidis {gatrian-at-iti.gr}
}
} Publication
}
} - Kimia, Ben, Brown University, USA {kimia-at-lems.brown.edu}
}
}
} Publicity
}
} - Niovi Pavlidou, Aristotelian University of Thessaloniki
} {niovi-at-vergina.eng.auth.gr}
}
}
}
} Steering Committee
}
} - Yiannis Aloimonos, University of Maryland, USA
} - Guido Cortelazzo, University of Padova, Italy
} - Concettina Guerra, University of Padova, Italy
} - Avi Kak, Purdue University, USA
} - Jan Koenderink, Utrecht University, Holland
} - Pietro Perona, Caltech, USA
} - Gabriel Taubin, Brown University, USA
} - Luc Van Gool, University of Leuven-ETH Zentrum, Belgium-Switzerland
}
} Keynote speakers:
}
} Nadia Magnenat-Thalmann, Geneva
} Vladimir Brajovic, CMU {brajovic-at-cs.cmu.edu}
} Jan Koenderink, Utrecht {j.j.koenderink-at-phys.uu.nl}
} Markus Gross, ETH Zurich {grossm-at-inf.ethz.ch}
} Craig Gotsman, Harvard {gotsman-at-eecs.harvard.edu}
} Demetri Terzopoulos, Courant {dt-at-cs.nyu.edu}
} George Barbastathis, MIT {gbarb-at-mit.edu}
} Andrew Fitzgibbon, Oxford
} Patrick Cavanagh, Harvard (patrick-at-wjh.harvard.edu)
}
}
} Special session organizers include:
}
} Gotsman, Craig (geometry processing) {gotsman-at-eecs.harvard.edu}
} Pollefeys, Marc (multiple view geometry) {marc-at-cs.unc.edu}
}
} Tutorials include:
}
} Marc Pollefeys, 3D Photography
}
} If you are interested in giving a tutorial, please
} contact the Chairs.
}
} Program committee:
}
} 1 Marc Alexa {alexa-at-informatik.tu-darmstadt.de}
} 2 Nina Amenta {amenta-at-cs.ucdavis.edu}
} 3 Anup Basu {anup-at-cs.ualberta.ca}
} 4 Alexander Belyaev {belyaev-at-mpi-sb.mpg.de}
} 5 Fausto Bernardini {fausto-at-us.ibm.com}
} 6 Jean-Daniel Boissonat {Jean-Daniel.Boissonnat-at-inria.fr}
} 7 Vladimir Brajovic {brajovic-at-cs.cmu.edu}
} 8 Pere Brunet {pere-at-lsi.upc.es}
} 9 Daniel Cohen-Or {dcor-at-tau.ac.il}
} 10 David Cooper {cooper-at-lems.brown.edu}
} 11 Guido Cortelazzo {corte-at-dei.unipd.it}
} 12 Kostas Daniilidis {kostas-at-cis.upenn.edu}
} 13 Larry Davis {lsd-at-umiacs.umd.edu
} 14 Leila DeFloriani {deflo-at-disi.unige.it}
} 15 Tamal Dey {tamaldey-at-cis.ohio-state.edu}
} 16 Craig Gotsman {gotsman-at-eecs.harvard.edu}
} 17 Markus Gross {grossm-at-inf.ethz.ch}
} 18 Concettina Guerra {guerra-at-dei.unipd.it}
} 19 Martial Hebert {hebert-at-ri.cmu.edu}
} 20 David Jacobs {djacobs-at-cs.umd.edu}
} 21 Avi Kak {kak-at-ecn.purdue.edu}
} 22 Myung-Soo Kim {mskim-at-cse.snu.ac.kr
} 23 Leif Kobbelt {kobbelt-at-cs.rwth-aachen.de}
} 24 Jan Koenderink {j.j.koenderink-at-phys.uu.nl}
} 25 Jana Kosecka {kosecka-at-cs.gmu.edu}
} 26 Frederic Leymarie {leymarie-at-lems.brown.edu}
} 27 Yi Ma {yima-at-uiuc.edu}
} 28 Nadia Magnenat-Thalmann {thalmann-at-miralab.unige.ch}
} 29 Roberto Manduchi {manduchi-at-soe.ucsc.edu}
} 30 Dinesh Manocha {dm-at-cs.unc.edu}
} 31 Ioana Martin {ioana-at-us.ibm.com}
} 32 Ralph Martin {ralph-at-cs.cf.ac.uk}
} 33 Takashi Matsuyama {tm-at-i.kyoto-u.ac.jp}
} 34 Randal Nelson {nelson-at-cs.rochester.edu}
} 35 Ko Nishino {kon-at-cs.columbia.edu}
} 36 Valerio Pascucci {pascucci1-at-llnl.gov}
} 37 Yannis Pitas {pitas-at-zeus.csd.auth.gr}
} 38 Marc Pollefeys {marc-at-cs.unc.edu}
} 39 Jean Ponce {ponce-at-cs.uiuc.edu}
} 40 Martin Rumpf {rumpf-at-math.uni-duisburg.de}
} 41 Holly Rushmeier {hertjwr-at-us.ibm.com}
} 42 Szymon Rusinkiewicz {smr-at-cs.princeton.edu}
} 43 Francis Schmitt {schmitt-at-ima.enst.fr}
} 44 Peter Schroeder {ps-at-cs.caltech.edu}
} 45 Hans-Peter Seidel {hpseidel-at-mpi-sb.mpg.de}
} 46 Claudio Silva {csilva-at-cs.utah.edu}
} 47 Yoshishisa Shinagawa {sinagawa-at-uiuc.edu}
} 48 Harry Shum {hshum-at-microsoft.com}
} 49 Stefano Soatto {soatto-at-cs.ucla.edu}
} 50 Carlo Tomasi {tomasi-at-cs.duke.edu}
} 51 Luc VanGool {vangool-at-vision.ee.ethz.ch}
} 52 Luiz Velho {lvelho-at-impa.br}
} 53 Denis Zorin {dzorin-at-mrl.nyu.edu}
} 54 Naokazu Yokoya {yokoya-at-is.aist-nara.ac.jp}
} 55 Peter Belhumeur {belhumeur-at-cs.columbia.edu}
} 56 Brian Curless {curless-at-cs.washington.edu}
} 57 Leonard McMillan {mcmillan-at-cs.unc.edu}
} 58 Davi Geiger {geiger-at-cs.nyu.edu}
} 59 Helder Jesus Araujo, Portugal
} 60 Daniel Cremers, UCLA
} 61 Nikos Paragios, Siemens/France
}
} _______________________________________________
} 3dpvt2004 mailing list
} 3dpvt2004-at-umiacs.umd.edu
} http://lists.umiacs.umd.edu/mailman/listinfo/3dpvt2004

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 16 02:42:20 2004

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}
} IASTED International Newsletter on Modelling and Simulation
} February 3, 2004
}
} UPCOMING DEADLINES
}
} 2 WEEKS REMAINING TO SUBMIT PAPERS
}
} 1. The IASTED International Conference on Applied Simulation and
Modelling - ASM 2004
} June 28-30, 2004, Rhodes, Greece
}
} Important Deadlines:
} **Submissions Due: Feb. 15, 2004**
} Notification of Acceptance: Apr. 1, 2004
} Registration Deadline: May 1, 2004
}
} To submit a paper, tutorial or special session or for more information
visit our website at http://www.iasted.org/conferences/2004/greece/asm.htm
}
} **Special Session Announcement**
} "Modelling and Simulation of Complex Biomechanical Systems" organized by
Prof. Philippe Gorce, University of Toulon-Var, France and Dr. Philippe
Pudlo, University of Valenciennes, France.
}
}
} 2. The 4th IASTED International Conference on Modelling, Simulation, and
Optimization - MSO 2004
} August 16-18, 2004, Kauai, Hawaii, USA
}
} Important Deadlines:
} **Submissions Due: Mar. 5, 2004**
} Notification of Acceptance: Apr. 15, 2004
} Registration Deadline: June 1, 2004
} To submit a paper, tutorial or special session or for more information
visit our website at http://www.iasted.org/conferences/2004/hawaii/mso.htm
}
} UPCOMING MODELLING AND SIMULATION CONFERENCE
} The submission deadline for the 15th IASTED International Conference on
Modelling and Simulation - MS 2004 being held March 1-3, 2004 in Marina Del
Rey, CA, USA has passed. Delegates without papers (attendees) are still
welcome to register.
}
} For registration information visit our website at
http://www.iasted.org/conferences/2004/marina/ms.htm
}
} MS 2004 Keynote Address
} "Modeling and Simulation of Chemically Reactive Systems at High Pressure"
by Dr. Francis H. Ree, Lawrence Livermore National Laboratory, Livermore,
USA. For additional information visit
http://www.iasted.org/conferences/2004/marina/ms-keynote.htm.
}
} MS 2004 Tutorial
} "Simulation-Based Engineering of Complex Systems Using EXTEND+OpEMCSS"
} Presented by Dr. John R. Clymer - California State University, Fullerton,
USA
} For additional information visit
http://www.iasted.org/conferences/2004/marina/ms-tutorial1.htm
}
} MS 2004 Special Session
} "Intelligent Reconfigurable Simulation" Organized by Dr. Tudor
Niculiu -University "Politehnica" of Bucharest, Romania. For additional
information visit
http://www.iasted.org/conferences/2004/marina/ms-specialsessions.htm
}
}
} JOURNAL SUBMISSION
} Selected papers accepted to our conferences will be considered for review
for inclusion in the IASTED International Journal of Modelling and
Simulation (IJMS). Authors must submit an expanded version of their
conference papers for peer review consideration to
http://www.actapress.com/journals/submission.htm, following the standard
procedure as described on the web site: www.actapress.com. All papers
considered for peer review in the International Journal of Modelling and
Simulation must be of the highest quality and demonstrate a novel
contribution to the literature.
}
}
} FUTURE CONFERENCES
} Mark your calendars! The IASTED International Conference on Environmental
Modelling and Simulation - EM&S 2004 will be held Nov. 22-24, 2004 in St.
Thomas, Virgin Islands, USA.
}
}
} MODELLING AND SIMULATION JOURNAL FROM ACTA PRESS
} The International Journal of Modelling and Simulation - First published in
1981, this journal covers all aspects of modelling, simulation, languages,
software, hardware, methodology, numerical and graphical methods, virtual
reality, statistical techniques, tutorials, surveys, and applications. It
also includes book reviews, conference notices, call for papers, and new
publications.
} Editor-in-Chief: Prof. A. Houshyar
} Frequency: 4 issues per year
} 2003 Rate: US$256.00
} Postage & Handling: US$25.00
} ISSN: 0228-6203 (205)
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}
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}
}
} CONFERENCE PROCEEDINGS AVAILABLE
} Forward this information to your University library in order to stay up to
date! Past conference proceedings in the area of modelling and simulation
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}
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From MicroscopyL-request-at-ns.microscopy.com Mon Feb 16 05:08:52 2004

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I am looking for the make and size of the Ion pump that is on the Philips
CM12.
It seems easier to ask rather than pull the covers off the scope as the EDS
is in the way.

I am also looking for any used PSEM 75's for sale
Please contact me at the below e-mail address.

Thanks in advance
Hank Beebe

Manager Instrument Services
hbeebe-at-rjlg.com
RJLee Group, Inc.
350 Hochberg Rd.
Monroeville, PA 15146
(724) 325-1776 voice
(724) 733-1799 fax

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 16 05:08:29 2004

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Colleagues

Just a reminder the deadline for submitting papers to the Microscopy
& Microanalysis 2004
meeting in Savannah is 17:00 PST , Monday Feb 16, 2004.

All the information you need to submit a paper is on-line at

http://mm2004.microscopy.org

Cheers...

Nestor
Your Friendly Neighborhood SysOp.

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 16 05:12:14 2004

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Dear Rose,

Yes, the number after the magnification is the magnification is the Numerical Aperture or NA.

Three quick equations which you might find helpful.

1. NA = n sin a
where
n = refractive index of the immersing liquid between the top of the sample and the front element of the lens
a = 1/2 of the collecting angle of the objective

From this equation, you can quickly see that, the larger the collecting angle, the greater the NA.
Also, the refractive index of air is 1.00, so using immersing fluids like water (1.33), glycerin (1.47), or immersion oil (1.5212) has tremendous effect on improving the NA. Reminder: use only the fluid for which the lens is engineered. Trying to use immersion oil with a "dry" (air) objective, is a disaster. Lenses built for immersing liquids are specially sealed so that the liquid does not creep into the internal construction of the lenses.

2. Why is NA important? The reasons are derived from Diffraction Theory. Every object produces a diffraction pattern (see Young's slit experiments in any physics book for details). For simple objects like stage micrometers and diatoms like pleurasigma angulatum, you can see the diffraction pattern by removing the eyepiece and peering deep down the tube into the Back Focal Plane of the objective. (You also need to close down the condernser as far as it will go, to make the source of light a very small opening or, alternatively, remove it and put a pinhole over the light port in the base of your microscope). If the NA is big enough to capture 2 adjacent spots from the diffraction pattern, enough information is present to determine spacing in the original object. The basic equation for resolution summarizes:

Rxy = (1.22x wavelength)/ (NAobjective+NAcondenser).
R = the size (in the XY plane, typically in micrometers) of the smallest resolvable particle
1.22 = a shape function (assuming round apertures in the microscope)
Wavelength = you can use 500 nm or 0.500 micrometers as sort of the center of the visible spectrum
NA = real working NAs (note: just because a lens is engraved with a value, does not mean that that is the working NA. Closing down an iris in the back focal plane of the objective or closing down the condenser aperture iris reduces the real working NA).

If the NA is big enough to capture THREE adjacent diffraction spots (the set of -1/0/+1 only counts as 2), you will begin to get better edge definition. So, the bigger the NA, the smaller the particle that you can resolve and the better the edge quality will be.

3. As for your other question: micrometers
Are you referring to the working distance (distance from the front of the lense to the top of the sample) or Field of View?
If working distance: you can either measure that directly or can look up the specs in the literature from the manufacturer.
If Field of view (the diameter of the territory you see when looking through the eyepieces):
F. O. V = (field number)/Mobjective
The field number is the value written on the EYEPIECE, following the magnification. It refers to the distance across a small ridge or baffle typically mounted about 1/3 of the way up the inside wall from the BOTTOM of the eyepiece and typically ranges from about 18mm to 25 mm (old Reichert Polyvars and some others had ultra wide field of view and went to 32mm). Convert to micrometers by multiplying by 1000.
Mobjective is the Magnification of the OBJECTIVE multiplied by any other auxiliary lenses between the objective and the bottom of the eyepiece.
Ex: If you were working with eyepieces which had field number 22 (22 mm or 22,000 micrometers) and a 10x objective, the size of the field of view is simply 22,000/10 or 2,000micrometers.

Note: the eyepiece going to the camera is often a different magnification than the eyepieces you look through and the chip in the camera has its own equivalent of a "magnification", so what you see in the eyepieces will often be a larger FOV than you can capture with your camera.

You might find my book, "Optimizing Light Microscopy", helpful. A description and ordering information are on our website: www.MicroscopyEducation.com

Good hunting!
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^
Don't forget: the American Chem Society's Applied Optical Microscopy Course, March 5-7, Chicago, Ill.
Visit our website for details and registration. NOT JUST FOR CHEMISTS!!!!
^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^
Best regards

At 07:27 AM 2/11/04 +1100, zeriena-at-yahoo.com wrote:

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}
} 3DPTV 2004, Thessaloniki - Greece
} http://www.umiacs.umd.edu/conferences/3dpvt04/
}
}
============================================================================
}
} Call for Papers
}
} The second International Symposium on 3DPTV (3D Data Processing,
} Visualization, and
} Transmission) will be held on September 6 to 9, 2004 in the city of
} Thessaloniki, Greece.
}
} The goal of this meeting is to present and discuss new research ideas and
} results related to the capture, representation, compact storage,
} transmission, processing, editing, optimization and visualization or 3D
} data. These topics span a number of research fields from applied
} mathematics, computer science, and engineering: computer vision, computer
} graphics, geometric modeling, signal and image processing, bionformatics,
} and statistics.
}
} This symposium follows the highly successful 1st International Symposium
on
} 3D Data Processing, Visualization, and Transmission
} 3DPVT'02 (http://www.dei.unipd.it/conferences/3DPVT) which took place in
} 2003 in Padova, Italy. The proceedings of the symposium will be published
in
} the IEEE Proceedings Series, in cooperation with Eurographics and ACM
} SIGGRAPH.
}
} A list of topics of interest includes but is not limited to:
}
} - 3D scanning technologies and devices
} - 3D photography algorithms
} - 3D view registration and surface modeling
} - Surface reflectance recovery and modeling
} - 3D texture processing
} - Image-based rendering and modeling
} - Multi-view image and geometry processing
} - Stereo and motion reconstruction
} - Augmented reality
} - Compression, transmission and visualization of 3D data
} - 3D Content-based retrieval and recognition
} - Man/machine interaction with 3D data
} - 3D printing and rapid prototyping
} - Psychophysics of 3D sensing and haptics
} - 3D imaging in biomedicine
} - Structural analysis and pattern discovery in bioinformatics
} - 3D imaging in virtual heritage and virtual archeology
} - 3D imaging in e-commerce.
} - 3D Television
} - Teleimmersion and remote collaboration
}
} Paper submission
}
} Papers submitted for review must follow the IEEE CS Press Proceedings
} two-column format. The papers must be submitted for review in final form.
} The maximum paper length for review as well as for publication is 8 pages,
} including the bibliography and the figures. Electronic manuscripts must
be
} submitted in Adobe Acrobat PDF format. In exceptional circumstances,
} PostScript files will be accepted and converted to PDF: you must contact
the
} conference in advance if you intend to do so.
}
} The paper must have the full author contact information. All accepted
papers
} will be published in the Proceedings of the Symposium (on a CD-ROM).
} The symposium language will be English.
}
} Important Dates
}
} Abstracts : April 2
} Full Papers : April 7
} Reviews due : May 15
} Author notification : May 25
} Deadline for price
} reduced hotel
} booking : June 10
} Camera-ready Papers : June 15
} and Registration of at
} least one author per
} paper
}
} Hotel reservations : May 25 to August 30
} Registration deadline : June 30
} for reduced price
}
} Tutorials : September 6
} Symposium : September 7-9
}
}
}
} --------------------------------------------------------------------------
--
} ---
}
} General chairs
}
} - Aloimonos, Yiannis, University of Maryland, USA {yiannis-at-cfar.umd.edu}
} - Taubin, Gabriel, Brown University, USA {taubin-at-brown.edu}
}
} Finance and registration chair
}
} - Duraiswami, Ramani, University of Maryland, {ramani-at-umiacs.umd.edu}
}
} Local arrangements
}
} - Petrou, Maria {M.Petrou-at-ee.surrey.ac.uk}
} - Strintzis, Michael {strintzi-at-eng.auth.gr}
} - Mpountanour, Kalliope {kalm-at-iti.gr}
} - George Triantafyllidis {gatrian-at-iti.gr}
}
} Publication
}
} - Kimia, Ben, Brown University, USA {kimia-at-lems.brown.edu}
}
}
} Publicity
}
} - Niovi Pavlidou, Aristotelian University of Thessaloniki
} {niovi-at-vergina.eng.auth.gr}
}
}
}
} Steering Committee
}
} - Yiannis Aloimonos, University of Maryland, USA
} - Guido Cortelazzo, University of Padova, Italy
} - Concettina Guerra, University of Padova, Italy
} - Avi Kak, Purdue University, USA
} - Jan Koenderink, Utrecht University, Holland
} - Pietro Perona, Caltech, USA
} - Gabriel Taubin, Brown University, USA
} - Luc Van Gool, University of Leuven-ETH Zentrum, Belgium-Switzerland
}
} Keynote speakers:
}
} Nadia Magnenat-Thalmann, Geneva
} Vladimir Brajovic, CMU {brajovic-at-cs.cmu.edu}
} Jan Koenderink, Utrecht {j.j.koenderink-at-phys.uu.nl}
} Markus Gross, ETH Zurich {grossm-at-inf.ethz.ch}
} Craig Gotsman, Harvard {gotsman-at-eecs.harvard.edu}
} Demetri Terzopoulos, Courant {dt-at-cs.nyu.edu}
} George Barbastathis, MIT {gbarb-at-mit.edu}
} Andrew Fitzgibbon, Oxford
} Patrick Cavanagh, Harvard (patrick-at-wjh.harvard.edu)
}
}
} Special session organizers include:
}
} Gotsman, Craig (geometry processing) {gotsman-at-eecs.harvard.edu}
} Pollefeys, Marc (multiple view geometry) {marc-at-cs.unc.edu}
}
} Tutorials include:
}
} Marc Pollefeys, 3D Photography
}
} If you are interested in giving a tutorial, please
} contact the Chairs.
}
} Program committee:
}
} 1 Marc Alexa {alexa-at-informatik.tu-darmstadt.de}
} 2 Nina Amenta {amenta-at-cs.ucdavis.edu}
} 3 Anup Basu {anup-at-cs.ualberta.ca}
} 4 Alexander Belyaev {belyaev-at-mpi-sb.mpg.de}
} 5 Fausto Bernardini {fausto-at-us.ibm.com}
} 6 Jean-Daniel Boissonat {Jean-Daniel.Boissonnat-at-inria.fr}
} 7 Vladimir Brajovic {brajovic-at-cs.cmu.edu}
} 8 Pere Brunet {pere-at-lsi.upc.es}
} 9 Daniel Cohen-Or {dcor-at-tau.ac.il}
} 10 David Cooper {cooper-at-lems.brown.edu}
} 11 Guido Cortelazzo {corte-at-dei.unipd.it}
} 12 Kostas Daniilidis {kostas-at-cis.upenn.edu}
} 13 Larry Davis {lsd-at-umiacs.umd.edu
} 14 Leila DeFloriani {deflo-at-disi.unige.it}
} 15 Tamal Dey {tamaldey-at-cis.ohio-state.edu}
} 16 Craig Gotsman {gotsman-at-eecs.harvard.edu}
} 17 Markus Gross {grossm-at-inf.ethz.ch}
} 18 Concettina Guerra {guerra-at-dei.unipd.it}
} 19 Martial Hebert {hebert-at-ri.cmu.edu}
} 20 David Jacobs {djacobs-at-cs.umd.edu}
} 21 Avi Kak {kak-at-ecn.purdue.edu}
} 22 Myung-Soo Kim {mskim-at-cse.snu.ac.kr
} 23 Leif Kobbelt {kobbelt-at-cs.rwth-aachen.de}
} 24 Jan Koenderink {j.j.koenderink-at-phys.uu.nl}
} 25 Jana Kosecka {kosecka-at-cs.gmu.edu}
} 26 Frederic Leymarie {leymarie-at-lems.brown.edu}
} 27 Yi Ma {yima-at-uiuc.edu}
} 28 Nadia Magnenat-Thalmann {thalmann-at-miralab.unige.ch}
} 29 Roberto Manduchi {manduchi-at-soe.ucsc.edu}
} 30 Dinesh Manocha {dm-at-cs.unc.edu}
} 31 Ioana Martin {ioana-at-us.ibm.com}
} 32 Ralph Martin {ralph-at-cs.cf.ac.uk}
} 33 Takashi Matsuyama {tm-at-i.kyoto-u.ac.jp}
} 34 Randal Nelson {nelson-at-cs.rochester.edu}
} 35 Ko Nishino {kon-at-cs.columbia.edu}
} 36 Valerio Pascucci {pascucci1-at-llnl.gov}
} 37 Yannis Pitas {pitas-at-zeus.csd.auth.gr}
} 38 Marc Pollefeys {marc-at-cs.unc.edu}
} 39 Jean Ponce {ponce-at-cs.uiuc.edu}
} 40 Martin Rumpf {rumpf-at-math.uni-duisburg.de}
} 41 Holly Rushmeier {hertjwr-at-us.ibm.com}
} 42 Szymon Rusinkiewicz {smr-at-cs.princeton.edu}
} 43 Francis Schmitt {schmitt-at-ima.enst.fr}
} 44 Peter Schroeder {ps-at-cs.caltech.edu}
} 45 Hans-Peter Seidel {hpseidel-at-mpi-sb.mpg.de}
} 46 Claudio Silva {csilva-at-cs.utah.edu}
} 47 Yoshishisa Shinagawa {sinagawa-at-uiuc.edu}
} 48 Harry Shum {hshum-at-microsoft.com}
} 49 Stefano Soatto {soatto-at-cs.ucla.edu}
} 50 Carlo Tomasi {tomasi-at-cs.duke.edu}
} 51 Luc VanGool {vangool-at-vision.ee.ethz.ch}
} 52 Luiz Velho {lvelho-at-impa.br}
} 53 Denis Zorin {dzorin-at-mrl.nyu.edu}
} 54 Naokazu Yokoya {yokoya-at-is.aist-nara.ac.jp}
} 55 Peter Belhumeur {belhumeur-at-cs.columbia.edu}
} 56 Brian Curless {curless-at-cs.washington.edu}
} 57 Leonard McMillan {mcmillan-at-cs.unc.edu}
} 58 Davi Geiger {geiger-at-cs.nyu.edu}
} 59 Helder Jesus Araujo, Portugal
} 60 Daniel Cremers, UCLA
} 61 Nikos Paragios, Siemens/France
}
} _______________________________________________
} 3dpvt2004 mailing list
} 3dpvt2004-at-umiacs.umd.edu
} http://lists.umiacs.umd.edu/mailman/listinfo/3dpvt2004

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}
} IASTED International Newsletter on Modelling and Simulation
} February 3, 2004
}
} UPCOMING DEADLINES
}
} 2 WEEKS REMAINING TO SUBMIT PAPERS
}
} 1. The IASTED International Conference on Applied Simulation and
Modelling - ASM 2004
} June 28-30, 2004, Rhodes, Greece
}
} Important Deadlines:
} **Submissions Due: Feb. 15, 2004**
} Notification of Acceptance: Apr. 1, 2004
} Registration Deadline: May 1, 2004
}
} To submit a paper, tutorial or special session or for more information
visit our website at http://www.iasted.org/conferences/2004/greece/asm.htm
}
} **Special Session Announcement**
} "Modelling and Simulation of Complex Biomechanical Systems" organized by
Prof. Philippe Gorce, University of Toulon-Var, France and Dr. Philippe
Pudlo, University of Valenciennes, France.
}
}
} 2. The 4th IASTED International Conference on Modelling, Simulation, and
Optimization - MSO 2004
} August 16-18, 2004, Kauai, Hawaii, USA
}
} Important Deadlines:
} **Submissions Due: Mar. 5, 2004**
} Notification of Acceptance: Apr. 15, 2004
} Registration Deadline: June 1, 2004
} To submit a paper, tutorial or special session or for more information
visit our website at http://www.iasted.org/conferences/2004/hawaii/mso.htm
}
} UPCOMING MODELLING AND SIMULATION CONFERENCE
} The submission deadline for the 15th IASTED International Conference on
Modelling and Simulation - MS 2004 being held March 1-3, 2004 in Marina Del
Rey, CA, USA has passed. Delegates without papers (attendees) are still
welcome to register.
}
} For registration information visit our website at
http://www.iasted.org/conferences/2004/marina/ms.htm
}
} MS 2004 Keynote Address
} "Modeling and Simulation of Chemically Reactive Systems at High Pressure"
by Dr. Francis H. Ree, Lawrence Livermore National Laboratory, Livermore,
USA. For additional information visit
http://www.iasted.org/conferences/2004/marina/ms-keynote.htm.
}
} MS 2004 Tutorial
} "Simulation-Based Engineering of Complex Systems Using EXTEND+OpEMCSS"
} Presented by Dr. John R. Clymer - California State University, Fullerton,
USA
} For additional information visit
http://www.iasted.org/conferences/2004/marina/ms-tutorial1.htm
}
} MS 2004 Special Session
} "Intelligent Reconfigurable Simulation" Organized by Dr. Tudor
Niculiu -University "Politehnica" of Bucharest, Romania. For additional
information visit
http://www.iasted.org/conferences/2004/marina/ms-specialsessions.htm
}
}
} JOURNAL SUBMISSION
} Selected papers accepted to our conferences will be considered for review
for inclusion in the IASTED International Journal of Modelling and
Simulation (IJMS). Authors must submit an expanded version of their
conference papers for peer review consideration to
http://www.actapress.com/journals/submission.htm, following the standard
procedure as described on the web site: www.actapress.com. All papers
considered for peer review in the International Journal of Modelling and
Simulation must be of the highest quality and demonstrate a novel
contribution to the literature.
}
}
} FUTURE CONFERENCES
} Mark your calendars! The IASTED International Conference on Environmental
Modelling and Simulation - EM&S 2004 will be held Nov. 22-24, 2004 in St.
Thomas, Virgin Islands, USA.
}
}
} MODELLING AND SIMULATION JOURNAL FROM ACTA PRESS
} The International Journal of Modelling and Simulation - First published in
1981, this journal covers all aspects of modelling, simulation, languages,
software, hardware, methodology, numerical and graphical methods, virtual
reality, statistical techniques, tutorials, surveys, and applications. It
also includes book reviews, conference notices, call for papers, and new
publications.
} Editor-in-Chief: Prof. A. Houshyar
} Frequency: 4 issues per year
} 2003 Rate: US$256.00
} Postage & Handling: US$25.00
} ISSN: 0228-6203 (205)
} http://www.actapress.com/journals/journals.htm#Modelling
}
}
} IASTED MEMBERSHIP
} It pays to be a member! One of the benefits of your IASTED membership is
a complimentary subscription to an ACTA Press journal of your choice.
Become a member today! http://www.iasted.org/member/OnlineMembershipForm.pdf
}
}
} CONFERENCE PROCEEDINGS AVAILABLE
} Forward this information to your University library in order to stay up to
date! Past conference proceedings in the area of modelling and simulation
are available for purchase from ACTA Press -
http://www.actapress.com/proceedings/proceedings.htm.
}
} For more information, to be removed from our mailing list, or to join one
of the following mail groups: Power, Telecommunication, Bio-Medicine, Signal
and Image Processing, Artificial Intelligence, Business, Software
Engineering, Education, Databases and Knowledge Engineering, Internet and
Applications, Parallel and Distributed Computing, please contact:
} IASTED
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} Canada T3B 0M6
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We are in need of a working Oxford XP3 pulse processor. Please email
with details and availability.
Thanks,
Ken
--
Kenneth JT Livi, Ph.D.
Department of Earth and Planetary Sciences
3400 N. Charles St.
Johns Hopkins University
Baltimore, MD 21218
(410) 516-8342
(410) 516-7933 fax

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 04:01:28 2004

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Dear all,
I am trying to open files obtained with a Noran confocal microscope (.mv file)with Image J, a software freely available on the net and equivalent to NIH image but running on a PC. Would anybody have any idea as how to do that ?
Thanks for any help,
Hervé.

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 08:30:54 2004

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I am in possession of a movie by Hitachi that is over 25 years old and
features the HU-11E TEM. I am about to toss it. If there is anyone out
there who would like to have it, let me know and I will be happy to send it
to you.

Greg Erdos

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 10:26:56 2004

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It's been so long since we dumped the Noran that I don't remember the
details, but I can tell you this:

I think the files were 512 X 484.

The header was of variable length consisting of keywords, that you can see
by ASCII, followed by the parameter value.

I typically did the math of 484 X 512 X Z and then subtracted off the
remainder as the header. Iterating on possible Z's finds the size.

} Dear all,
} I am trying to open files obtained with a Noran confocal microscope (.mv
} file)with Image J, a software freely available on the net and equivalent
} to NIH image but running on a PC. Would anybody have any idea as how to
} do that ?
} Thanks for any help,
} Hervé.

____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 10:46:37 2004

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The movie that I offered earlier today has been claimed by a lucky
individual. I never thought that it would generate so much interest.

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 11:03:55 2004

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Hello,

My name is Thomas Sadowski and I am currently a Computer Science and Physics
majorat Southern Connecticut State University. I am persuing an independent
study in the field of CT Scanning more specifically micro CT and invivo CT
scanning. I was wondering if anybody knew of any research sights,
individuals, or sources that would be able to provide me with any amount of
information concerning the process of these types of scans, the physics
behind them, or the data collection and interpretation process.

Thank you in advance for any help that you can provide.

Thomas Sadowski
Southern Connecticut State University

_________________________________________________________________
Stay informed on Election 2004 and the race to Super Tuesday.
http://special.msn.com/msn/election2004.armx

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 12:17:14 2004

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we would love to have it for the reference library here at the museum.

Thanks!

Ed Sharpe Archivist for SMECC

See the Southwest Museum of Engineering, Communications and Computation
online at:
http://www.smecc.org
----- Original Message -----
} From: "Greg Erdos" {gwe-at-biotech.ufl.edu}
To: {Microscopy-at-sparc5.microscopy.com}
Sent: Tuesday, February 17, 2004 7:41 AM

Have you tried the library? There are books, journals and websites on
this topic.

Geoff

Thomas Sadowski wrote:

} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hello,
}
} My name is Thomas Sadowski and I am currently a Computer Science and
} Physics majorat Southern Connecticut State University. I am persuing
} an independent study in the field of CT Scanning more specifically
} micro CT and invivo CT scanning. I was wondering if anybody knew of
} any research sights, individuals, or sources that would be able to
} provide me with any amount of information concerning the process of
} these types of scans, the physics behind them, or the data collection
} and interpretation process.
}
} Thank you in advance for any help that you can provide.
}
}
} Thomas Sadowski
} Southern Connecticut State University
}
} _________________________________________________________________
} Stay informed on Election 2004 and the race to Super Tuesday.
} http://special.msn.com/msn/election2004.armx
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 16:50:52 2004

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The University of Texas Health Science Center with support from
Hamamatsu Photonics KK
will offer a course on

Optical Microscopy in the Biological Sciences
June 2-9, 2004

at The University of Texas Health Sciences Center

Tuition is $2,100 and includes room, board, course materials and
registration for the
FRET/FLIM/Spectral Imaging Symposium (June 5-6, 2004)

A limited number of scholarships are available.

Application Deadline is March 1, 2004

Topics to be covered:
Microscope Optics: Phase Contrast, Dark-field, DIC, Polarization
Detectors * Digital Processing * Fluorescence Filters and Probes
Spectral Imaging * FRET * FLIM * Green Fluorescent Proteins
Confocal * Multiphoton * Deconvolution * 3-D Reconstruction

****************************************************************************
***************************************************

Application form: Application Deadline: March 1, 2004
Optical Microscopy Course Notification of Admission: March 15,2004
At
The University of Texas Health Science Center at San Antonio
June 2-9, 2004

Applicant's Name:________________________________________________________
Principle
Investigator:______________________________________________________
Affiliation:_______________________________________________________________
_______________________________________________________________
Address:________________________________________________________________

_________________________________________________________________

_________________________________________________________________
Phone: ______________________________ Fax:______________________________
Email:________________________________
Degree: _______ Academic Yes / No Commercial
Yes / No

Please consider my application for one of the 4 available scholarships. Yes
/ No

Note that Registration for the FRET/FLIM/Spectral Imaging Symposium is
included in the tuition.

Upon admission to the Optical Microscopy Course you will be required to
submit payment $2100 (US) on or before May 3, 2004 to reserve your spot in
the workshop.
This fee includes workshop material, symposium registration, room and board
for June 2-9, 2004.

Briefly describe your interests in Optical Microscopy an how attending this
course will further your research efforts.

Return to: Microscopy Course, Mail Code 7762
7703 Floyd Curl Dr.
San Antonio, TX 78229-3900
Fax to: (210) 567-3803
Email to: Frohlich-at-uthscsa.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 17 17:06:40 2004

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Hi Hervé,

You can export movies from ImageJ in AVI format if you use the AVI
writer plugin, so I would suggest that you use that in future and export
to AVI rather than save as .mv files. You may be able to open the .mv
file in VirtualDub (http://www.virtualdub.com/) but I'm not sure. If so,
you can subsequently write to AVI.

Good luck

Cheers,

Jacqui.

haptel-at-univ-montp2.fr wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Tel: 64 9 373 7599 Ext 87438
Fax: 64 9 373 7484

http://www.health.auckland.ac.nz/biru/

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 07:38:29 2004

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We use PGT eds detector and the light elements detection has decreased
significantly. Has anyone cleaned the detectors window? Is it possible?

Pavel Lozovyy
ATC SEM Lab
(216)692-6637
www.atclabs.com

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 08:31:51 2004

Contents Retrieved from Microscopy Listserver Archives
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I clean a window of a PRIZM detector systematically with
Vertel XF solvent (according to manufacturer's instructions).
I let detector to warm up, dismount it, and slowly put solvent
drop after drop on the top of the metal ring surrounding
the window, so that solvent will run over window. The window
is very fragile, it could be damaged by single drop,
if it goes directly on the window.

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

} We use PGT eds detector and the light elements detection has decreased
} significantly. Has anyone cleaned the detectors window? Is it
} possible?
}
} Pavel Lozovyy
} ATC SEM Lab
} (216)692-6637
} www.atclabs.com
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 11:37:00 2004

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I would appreciate any information concerning an introductory TEM training/course (USA) in the first or early in the second quarter of 2004. We need to get the trainee up to speed quickly and the Lehigh course in mid-June occurs too late in the year for our needs.

TIA

Fred A. Stewart-Davis
Engineering Specialist
Materials Characterization Lab
Glass Technology Center
Harmarville, PA 15238
fstewartdavis-at-ppg.com
*************************************************************************
*************************************************************************
*************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 12:26:02 2004

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Fred,

Take a look at this website. It is an introductory online course on TEM
Basics
http://www.matter.org.uk/tem/

And the following is an "on-site" training/lecture course (You would
probably have to call or e-mail to find out dates available):
http://www.emcourses.com/lecture1.htm

Kelly A. Ramos
Metallurgical Engineer / Supervisor
Argo-Tech Materials Laboratories
23555 Euclid Avenue
Cleveland, OH 44117
216-692-5904 or 216-692-5446
(fax) 216-692-5816
http://www.atclabs.com

"Stewart-Davis
, Fred A." To: "'Microscopy-at-MSA.Microscopy.Com'"
{fstewartdavis {Microscopy-at-MSA.Microscopy.Com}
-at-ppg.com} cc:
Subject: [Microscopy] TEM Courses/Training
02/18/04 12:47
PM

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I would appreciate any information concerning an introductory TEM
training/course (USA) in the first or early in the second quarter of 2004.
We need to get the trainee up to speed quickly and the Lehigh course in
mid-June occurs too late in the year for our needs.

TIA

Fred A. Stewart-Davis
Engineering Specialist
Materials Characterization Lab
Glass Technology Center
Harmarville, PA 15238
fstewartdavis-at-ppg.com
*************************************************************************
*************************************************************************
*************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 13:55:02 2004

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Is this on an UTW or Be?

I have been cleaning Be windows for years now using a similar technique (but with
Freon) but have often wondered if this would be OK if I had an UTW.

Some years ago, before UTWs, Oxford used to recommend dipping the end of the
detector into a beaker of ethanol.

cheers

rtch

} ---------
}
} I clean a window of a PRIZM detector systematically with
} Vertel XF solvent (according to manufacturer's instructions).
} I let detector to warm up, dismount it, and slowly put solvent
} drop after drop on the top of the metal ring surrounding
} the window, so that solvent will run over window. The window
} is very fragile, it could be damaged by single drop,
} if it goes directly on the window.
}
} Vladimir M. Dusevich, Ph.D.
} Electron Microscope Lab Manager
} 3127 School of Dentistry
} 650 E. 25th Street
} Kansas City, MO 64108-2784
}
} Phone: (816) 235-2072
} Fax: (816) 235-5524
} Web: http://www.umkc.edu/dentistry/microscopy
}
} } We use PGT eds detector and the light elements detection has
} } decreased significantly. Has anyone cleaned the detectors window? Is
} } it possible?
} }
} } Pavel Lozovyy
} } ATC SEM Lab
} } (216)692-6637
} } www.atclabs.com
} }

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 13:59:31 2004

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This is an UTW.

Vladimir

}
} Is this on an UTW or Be?
}
} I have been cleaning Be windows for years now using a similar
} technique (but with
} Freon) but have often wondered if this would be OK if I had an UTW.
}
} Some years ago, before UTWs, Oxford used to recommend dipping
} the end of the
} detector into a beaker of ethanol.
}
} cheers
}
} rtch
}
}
}
} } ---------
} }
} } I clean a window of a PRIZM detector systematically with
} } Vertel XF solvent (according to manufacturer's instructions).
} } I let detector to warm up, dismount it, and slowly put solvent
} } drop after drop on the top of the metal ring surrounding
} } the window, so that solvent will run over window. The window
} } is very fragile, it could be damaged by single drop,
} } if it goes directly on the window.
} }
} } Vladimir M. Dusevich, Ph.D.
} } Electron Microscope Lab Manager
} } 3127 School of Dentistry
} } 650 E. 25th Street
} } Kansas City, MO 64108-2784
} }
} } Phone: (816) 235-2072
} } Fax: (816) 235-5524
} } Web: http://www.umkc.edu/dentistry/microscopy
} }
} } } We use PGT eds detector and the light elements detection has
} } } decreased significantly. Has anyone cleaned the detectors
} window? Is
} } } it possible?
} } }
} } } Pavel Lozovyy
} } } ATC SEM Lab
} } } (216)692-6637
} } } www.atclabs.com
} } }
}
} --
} Ritchie Sims Ph D Phone : 64 9
} 3737599 ext 87713
} Microanalyst Fax :
} 64 9 3737435
} Department of Geology email :
} r.sims-at-auckland.ac.nz
} The University of Auckland
} Private Bag 92019
} Auckland
} New Zealand
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 14:30:00 2004

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Fellow List Members,

This year we will be hosting the 9th Annual RMC Materials Microtomy Short Course in Tucson, Arizona from April 27 - 30.

Join us and our internationally renowned course faculty in sunny Tucson to participate in this unique event.

This short course is designed specifically for researchers in the field of materials science who wish to gain exposure to advances in specimen preparation for electron microscopy.

E-mail Kim Megaw at {kim-at-boeckeler.com} to receive full details and a course brochure.

Best Regards,

Robert (Bob) Chiovetti
Senior Product Specialist
RMC Products
Boeckeler Instruments, Inc.
4650 South Butterfield Drive
Tucson, AZ 85714 USA
Tel. 520.745.0001
Fax 520.745.0004
{www.rmcproducts.com}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 18 17:56:51 2004

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JOB TITLE: TEM sample prep technician

COMPANY: FASL, LLC / Advanced Micro Devices

LOCATION: Sunnyvale, CA

DESCRIPTION OF POSITION: This job mainly involves using FIB to make TEM samples. However, the applicant should also be able to perform routine technical tasks in support of materials analysis activities. Should be skilled in optical microscopy, electron microscopy, micro cross-sectioning, FIB, wet/dry deprocessing. Specific site or defect locations FA. Supports material analysis through direct customer interaction.

SPECIFIC JOB FUNCTIONS: TEM sample prep by FIB. Close interaction with TEM engineers and requesting customers. Good computer skills needed.

PREFERRED EDUCATION AND EXPERIENCE: AS degree in a science field. Some semiconductor is preferred. Experience in the theory and operation of scanning electron microscopes and focussed ion beams is a real plus. Good manual skills for fine detailed work is required. Resourcefulness. Independent worker that can complete tasks with limited guidence. Should know PC's and internet.

For faster consideration, send your resume to jazylette.windell-at-amd.com and please cc:jobs-at-spansion.com.
(Please do not send resumes to alline-at-earthlink.net; you may send them instead to alline.myers-at-spansion.com.)

Requisition Number
FC52734

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 01:42:40 2004

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The are some courses in Sheffield, UK in April. Maybe they can be of interest. See: http://www.microscopie.nl/19-23April.pdf

Erik Johnson
Department of Materials Research
Risř
DK-4000 Roskilde
Denmark

-----Original Message-----
} From: Stewart-Davis, Fred A. [mailto:fstewartdavis-at-ppg.com]
Sent: 18 February 2004 18:47
To: 'Microscopy-at-MSA.Microscopy.Com'

Hi,
I have processed a large batch of mouse femurs (after decalcification)
into epoxy resin for LM examination only. I have done this before and
infiltration was good throughout the thickness of the sample (which can be
3mm max dimension). This last time a proportion of them are poorly
infiltrated (air spaces) and the resin internally is a bit soft and
sticky. Does anyone know if there is anyway I can remove the polymerised
resin and attempt to get more in now that I have removed half the block by
sectioning, (the actual tissue preservation looks fine)?

Thanks in anticipation

Gill Brown

Histopathology Group
Asthma and Allergy Disease Biology
ri- CEDD.
GlaxoSmithKline Medicines Research Centre,

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 07:07:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sswaffe-at-abv.bg) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Tuesday, February 17, 2004 at 12:38:16
---------------------------------------------------------------------------

Email: sswaffe-at-abv.bg
Name: Veselin

Organization: 54th. st.Ivan Rilski

Education: 6-8th Grade Middle School

Location: Sofia, Bulgaria

Question: What are actually infininity optical systems and how do they differentiate from the normal optical systems?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 08:32:20 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (EPablo-at-Polese.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 18, 2004 at 14:10:15
---------------------------------------------------------------------------

Email: EPablo-at-Polese.com
Name: Elmer Pablo

Organization: Polese Company Inc.

Title-Subject: [Microscopy] [Filtered] ASTM E112 Grain Size

Question: I am looking for ASTM E112 (Order #PCN 12-501122-28) or equivalent to determine average grain size. Does anyone have any information where I can buy or get a copy? This item is no longer available from ASTM. Anyone that can provide information for this item is greatly appreciated. Thank you in advance

Elmer Pablo
Materials Lab. Tech
Polese Co.
San Diego, Ca
858-348-1202 (Phone)
413-513-2527 (EFax)

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 08:32:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jderyk-at-dpi.radiology.uiowa.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 18, 2004 at 15:32:49
---------------------------------------------------------------------------

Email: jderyk-at-dpi.radiology.uiowa.edu
Name: Jessica deryk

Title-Subject: [Microscopy] [Filtered] MListserver:Confusing calculations

Question: Hi,
I was hoping someone could help me find, what I thought would be fundamental relationships for microscopy but are proving to be difficult to determine.
I have a LeicaMz16a steromicroscope with;
7.11x to 155x mag
FOV range: 29.5mm to 1.82mm

This is coupled to a CCD camera with;
1300x1030 pixel array
pixel spacing: 6.7microns
FOW: 8.7 x 6.9 mm

I'm wondering how I can accurately calculate the effective FOV as seen by the rectangular CCD. Also the relationship between magnification in the microscope and resulting pixel spacing of my digital images??

I would appreciate any advice in these calculations or references to texts which may contain information regarding interaction between CCD cameras and microscopes.
Thanks
Jess

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 08:33:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Julie.Glasscock-at-csiro.au) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 18, 2004 at 23:09:51
---------------------------------------------------------------------------

Email: Julie.Glasscock-at-csiro.au
Name: Julie Glasscock

Organization: CSIRO

Title-Subject: [Microscopy] [Filtered] Faraday cup

Question: I am using a JEOL 6300F SEM for e-beam lithography using Nabity's Nano-Pattern Generation System (NPGS). I need to use a Faraday cup to check the beam current. Apparently there is a Faraday cup attachment (on a movable arm) in our SEM that was purchased from Oxford Instruments. Unfortunately no-one here or at Oxford has any memory of where the attachment is placed or how to use it. We have found a BNC connector coming out of the specimen exchange chamber that may be the connection for an ammeter. Does anyone else have such an attachment and know where it may be located within the SEM and how it works? Any information will be gratefully received!

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 08:31:53 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (amy.snodgrass-at-eyetk.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, February 17, 2004 at 14:16:55
---------------------------------------------------------------------------

Email: amy.snodgrass-at-eyetk.com
Name: Amy Snodgrass

Organization: Eyetech Pharmaceuticals

Title-Subject: [Microscopy] [Filtered] MListserver: Sputter coater sought

Question: I would like to buy a used sputter coater for coating SEM samples with metal and carbon. Anybody selling one? Boston/New England area preferred.

Thanks,
Amy

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 09:06:32 2004

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You might be able to remove it by soaking the blocks in sodium ethoxide and
then reprocessing from absolute alcohol into new epoxy. There seems to be a
possibility that this will affect antigens, though.

Lesley Weston.

on 19/02/2004 12:58 AM, gillian.2.brown-at-gsk.com at gillian.2.brown-at-gsk.com
wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Hi,
} I have processed a large batch of mouse femurs (after decalcification)
} into epoxy resin for LM examination only. I have done this before and
} infiltration was good throughout the thickness of the sample (which can be
} 3mm max dimension). This last time a proportion of them are poorly
} infiltrated (air spaces) and the resin internally is a bit soft and
} sticky. Does anyone know if there is anyway I can remove the polymerised
} resin and attempt to get more in now that I have removed half the block by
} sectioning, (the actual tissue preservation looks fine)?
}
} Thanks in anticipation
}
} Gill Brown
}
}
} Histopathology Group
} Asthma and Allergy Disease Biology
} ri- CEDD.
} GlaxoSmithKline Medicines Research Centre,
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 09:15:24 2004

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This standard is active and available from ASTM. It can be ordered on
line with a credit card direct from ASTM. Go to www.astm.org, click on
Standards on the left menu, then click on Individual Standards to get
the Standard Search form.

--
Larry D. Hanke, P.E.
Materials Evaluation and Engineering, Inc.
Practical Solutions Through Technology and Innovation
http://www.mee-inc.com (763) 449-8870

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 10:51:05 2004

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Until recently we were running a PGT thin window detector on an ISI-40 SEM.
We ran it for about 13 years. Because it was on a diffusion pumped system
it was necessary to clean the window periodically. Given our usage,
relatively low hours, I found it necessary to clean the window about every
four to six months. I did it when the copper L lines decreased in height to
approach the Kalpha line height. I consulted PGT and found that it is
important to 1). Clean it after warming up the system, 2) use a solvent that
is compatible with the adhesive used on the window, 3) don't touch the
window. It would take about 8 to 9 days for our dewar to warm after a
fill. I did not remove the detector from the SEM. I used an eye dropper to
drip a few drops of solvent on to the end of the detector. I was also able
to "squirt" a few drops onto the window directly. I had occasion to employ
this procedure probably 20 times or more. We retired the system, working
very well because we acquired a new SEM that, incidentally has a silicon
drift detector, LN2-free, mounted on it. I would recommend that before you
do any cleaning contact PGT about your detector to get their advice as to
which solvent is best for the window on your detector.

Vern Griffiths, Montana Tech, Emeritus Prof.

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 11:18:07 2004

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hello,

I am currently loocking at liquid polymers in which DNA has been
incorporated. In order to look at the resulting structures, I have tried
several negative stains such as PTA, uranyl acetate, ammonium molybdate
with different results and none of which really satisfy me.

For exemple, I have difficulties getting the sample to actually stay on
the formvar grid, most of it seems to slip away...
The method I use is the following;
sample sitting on the formvar grid for 1-2 minutes
drain the excess with a filter paper
appl the stain for 1 minute
drain the excess with a filter paper

I do not have access to a high vacuum evaporator (shadowing technique)
but someone told me about using colloidal carbon mix with the liquid
polymer sample, similar to negative staining.
Has anyone heard about that technique and, if it is the case, what are
the propotion of carbon, the best way to get good results..etc..

Other ideas are also welcome!!

thank you,

Diane

Diane Montpetit
Microscopie électronique/Electron microscopy
Centre de Recherche et de Développement sur les Aliments/Food and
Development Research Center
Agriculture et Agroalimentaire Canada/Agriculture and Agri-Food Canada
téléphone/telephone 450-778-3024 (196)
télécopieur/facsimile 450-773-8461
3600 Boul. Casavant Ouest/3600 Casavant West boul.
St-Hyacinthe (Québec) J2S 8E3
montpetitd-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 11:48:56 2004

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Elmer wrote:

I am looking for ASTM E112 (Order #PCN 12-501122-28)
or equivalent to determine average grain size. Does
anyone have any information where I can buy or get a
copy? This item is no longer available from ASTM.
Anyone that can provide information for this item is
greatly appreciated. Thank you in advance.

Email: EPablo-at-Polese.com
Name: Elmer Pablo
Organization: Polese Company Inc.

Elmer Pablo
Materials Lab. Tech
Polese Co.
San Diego, Ca
858-348-1202 (Phone)

Elmer, I have a copy of ASTM E 112-96. Check your
e-mail and send me an address.

Stu Smalinskas
Metallurgist
SKF USA
Plymouth, Michigan

__________________________________
Do you Yahoo!?
Yahoo! Mail SpamGuard - Read only the mail you want.
http://antispam.yahoo.com/tools

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 12:46:24 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tgreco-at-seas.marine.usf.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, February 19, 2004 at 12:14:55
---------------------------------------------------------------------------

Email: tgreco-at-seas.marine.usf.edu
Name: Tony Greco

Organization: University of South Florida

Title-Subject: [Microscopy] [Filtered] MListserver:Variable pressure SEM

Question: I purchased a variable pressure SEM with diffusion pump
about 3 years ago and was told that by setting the
sample chamber pressure to between 30-40Pa over the
weekend, I could effectively scrub the inside of the
chamber including any oil that had accumulated on the
x-ray window. Sadly this has not been the case as chamber
and especially the x-ray window regularly becomes
contaminated with rotary pump oil. All efforts to combat
this problem have failed including a foreline trap in the
RP line. Any suggestions?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 13:29:23 2004

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}
} Title-Subject: [Microscopy] [Filtered] Faraday cup
}
} Question: I am using a JEOL 6300F SEM for e-beam lithography using
} Nabity's Nano-Pattern Generation System (NPGS). I need to use a
} Faraday cup to check the beam current. Apparently there is a Faraday
} cup attachment (on a movable arm) in our SEM that was purchased from
} Oxford Instruments. Unfortunately no-one here or at Oxford has any
} memory of where the attachment is placed or how to use it. We have
} found a BNC connector coming out of the specimen exchange chamber that
} may be the connection for an ammeter. Does anyone else have such an
} attachment and know where it may be located within the SEM and how it
} works? Any information will be gratefully received!
}
}

I suggest you contact JEOL in Sydney.

JEOL probably have a PCD accessory for the 6300, which will fit to the scope better
than will any third-party one, and Vitaly Lozbin will no doubt be able to identify your BNC
connector over the phone.

They were even able to make me one for my 840, even though it was not in their
current catalogue. At a very reasonable price.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 13:46:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (JAHMIT-at-aol.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Thursday, February 19, 2004 at 13:41:24
---------------------------------------------------------------------------

Email: JAHMIT-at-aol.com
Name: Natalie Heltman

Organization: E.H. Greene

Education: K-8 Grade Grammar School

Location: Cincinnati, OH 45242

Question: Hello, I'm doing a research paper on John William
Coleman and I cannot find any information on him.
I was in need of any info. you can provide. I know that he was a member of Electron Microscopy
Society? What was his role in the development of the electron microscope with RCA Labs?

Any info. would help I'm sending this message form my Dad's work place. Thanks, Natalie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 14:45:14 2004

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Natalie,

This website...

http://www.princeton.edu/~mcbrown/display/john_coleman.html

..has some information about John William Coleman.

Here is another little bio I found:

JOHN WILLIAM COLEMAN (1929- ) was born in New York City, earning a Ph.D. in
Biophysics from the University of Pennsylvania in 1963. From 1951 to 1953,
John Coleman served as a Physicist for the National Bureau of Standards. He
was an Instructor in Physics at Howard University from 1957-58, later
becoming an Engineer for RCA in 1958. His research involved the physics of
electrons, and he assisted in the development of the American electron
microscope developed at RCA.

The above Princeton website also has a bibliography:

American Men of Science. 11th edition, Supplement 2 (New York:
McGraw-Hill), p. 158.

Blacks in Science and Education. Vivian O. Sammons. (Washington, D.C.:
Hemisphere Publishers), 1989. p.158.

Encyclopedia of Black America. Agustus Low and Virgil A. Clift, editors.
(New York, NY: McGraw-Hill), 1981. p. 744.

Who's Who in the East. 17th edition, 1979-1980. (Wilmette, IL: Marquis
Who's Who), 1979.

Who's Who in the East. 16th edition, 1977-1978. (Wilmette, IL: Marquis
Who's Who), 1977.

Hope this helps,

Ellery

---------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
Department of Geology & Geophysics
University of Minnesota - Twin Cities
Lab Website: http://probelab.geo.umn.edu

On 19 Feb 2004, by way of Ask-A-Microscopist wrote:
}
} Email: JAHMIT-at-aol.com
} Name: Natalie Heltman
}
} Organization: E.H. Greene
}
} Education: K-8 Grade Grammar School
}
} Location: Cincinnati, OH 45242
}
} Question: Hello, I'm doing a research paper on John William
} Coleman and I cannot find any information on him.
} I was in need of any info. you can provide. I know that he was a member
of
} Electron Microscopy
} Society? What was his role in the development of the electron microscope
with
} RCA Labs?
}
} Any info. would help I'm sending this message form my Dad's work place.
} Thanks, Natalie

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 14:50:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Natalie;

You may want to contact SRI [Sarnoff Research International] in Princeton, New Jersey. This was formerly Sarnoff Research, a division of RCA Corp. which I am an alumni of.

Peter Tomic
Agere Systems, formerly Lucent Technologies, Att etc.

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:JAHMIT-at-aol.com]
Sent: Thursday, February 19, 2004 2:57 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (JAHMIT-at-aol.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Thursday, February 19, 2004 at 13:41:24
---------------------------------------------------------------------------

Email: JAHMIT-at-aol.com
Name: Natalie Heltman

Organization: E.H. Greene

Education: K-8 Grade Grammar School

Location: Cincinnati, OH 45242

Question: Hello, I'm doing a research paper on John William
Coleman and I cannot find any information on him.
I was in need of any info. you can provide. I know that he was a member of Electron Microscopy
Society? What was his role in the development of the electron microscope with RCA Labs?

Any info. would help I'm sending this message form my Dad's work place. Thanks, Natalie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 14:55:43 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

Does anyone have an extra 3-1/4 x 4" plate holder insert
that they wouldn't mind getting rid of? We only need the
insert (from a two-piece holder) from a Philips EM 410. I
believe the design hasn't changed in many years and that
it is the same for any CM or 400 series. I can email a
jpg image to anyone who might want to compare what I have
with what they have.

Thank you in advance,

Doug

----------------------
Douglas R. Keene
Associate Investigator
Micro-Imaging Center
Shriners Hospital for Children
3101 S.W. Sam Jackson Park Road
Portland, Oregon 97239-3009
phone: 503-221-3434
FAX: 503-412-6894

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 15:27:56 2004

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On Feb 19, 2004, at 6:43 AM, by way of MicroscopyListserver wrote:

} Name: Jessica deryk
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Confusing
} calculations
}
} Question: Hi,
} I was hoping someone could help me find, what I thought would be
} fundamental relationships for microscopy but are proving to be
} difficult to determine.
} I have a LeicaMz16a steromicroscope with;
} 7.11x to 155x mag
} FOV range: 29.5mm to 1.82mm
}
} This is coupled to a CCD camera with;
} 1300x1030 pixel array
} pixel spacing: 6.7microns
} FOW: 8.7 x 6.9 mm
}
} I'm wondering how I can accurately calculate the effective FOV as seen
} by the rectangular CCD. Also the relationship between magnification in
} the microscope and resulting pixel spacing of my digital images??
}
} I would appreciate any advice in these calculations or references to
} texts which may contain information regarding interaction between CCD
} cameras and microscopes.
}
Dear Jess,
If the FOV of the magnified image (mFOV) was the same at all mags,
then mag x mFOV = FOV. Since that is not true for the two mags you
list, there must be an additional constraint within the scope that does
not let you see as big an area at low mag; that could be a source of
math confusion. In contrast, the size of the FOV of the CCD is
consistent with the number of pixels and the pixel size, and that size
is smaller than the FOVs for each mag, so the CCD should see a
rectangular area within the FOV at any mag. The FOV on the object that
can be seen by the CCD is just the CCD area divided by the mag, so for
the two mags listed, the CCD FOVs would be 1.22 mm x 0.97 mm for 7.11x
and 0.056 mm x 0.044 mm for 155x.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 15:35:40 2004

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We have a Balzer's 301 Freeze Fracture Apparatus available to anyone who can
take it away. The system was modified by Wiltek and equipped with a digital
vacuum control system, a Mass Spec and Cryopump (there are two cryopumps
both currently non-operational). A brief description and pictures will be
available at http://www.cscn.com/gsis/prod01.htm .
If you're interested please contact me, Richard Harris by phone 519-661-2111
ext 86780 or e-mail rjharris-at-uwo.ca.
Thanks

Richard Harris
Laboratory Supervisor
Department of Biology
University of Western Ontario
London Ontario CANADA
Ph. 519-661-2111 ext. 86780
Fax 519-661-3935

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 15:47:30 2004

Contents Retrieved from Microscopy Listserver Archives
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Great subject, Natalie!

http://www.princeton.edu/~mcbrown/display/john_coleman.html

http://www2.sis.pitt.edu/resources/diversity/naa/physics2.html

Good Luck -

Marc Helvey

VLSI Standards, Inc.
Strategic Accounts Manager
3087 North First Street
San Jose, CA 95134-2006
Phone: (408) 428-1800, ext. 108
Fax: (408) 428-9555
E-mail: marc.helvey-at-vlsistd.com
Internet: http://www.vlsistandards.com

-----Original Message-----
} From: JAHMIT-at-aol.com [mailto:JAHMIT-at-aol.com]
Sent: Thursday, February 19, 2004 11:57 AM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (JAHMIT-at-aol.com) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Thursday, February
19, 2004 at 13:41:24
---------------------------------------------------------------------------

Email: JAHMIT-at-aol.com
Name: Natalie Heltman

Organization: E.H. Greene

Education: K-8 Grade Grammar School

Location: Cincinnati, OH 45242

Question: Hello, I'm doing a research paper on John William
Coleman and I cannot find any information on him.
I was in need of any info. you can provide. I know that he was a member of
Electron Microscopy
Society? What was his role in the development of the electron microscope
with RCA Labs?

Any info. would help I'm sending this message form my Dad's work place.
Thanks, Natalie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 16:15:51 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Diane
I know nothing about "colloidal carbon" - does it exist in this
world? From another hand I very doubt that even "colloidal carbon" could
help you. I suppose you want to see the fine details of your sample if
were trying to use negative staining. DNA is 2.4-3 nm in diameter, even
naked DNA may not be visualized well using negative staining. You may see
DNA using "positive staining" but it's quite difficult and you need to use
high-res. STEM and probably Z-contrast (and NEVER Formvar support
film!!!!!). To see any DNA on polymer's background is a big problem because
your polymer will scatter most electrons... Trying to see one polymer
(yours) on another polymer (Formvar) is seems to me even more challenged. I
would suggest, you need to try freeze-fracture in combination with good
SEM. It will give you idea of 3D structure of polymer and you probably
will be able to see some DNA conglomerates (not DNA strands). Sometime
DNA created sort of periodic structure, which you also could see. I know
that some people froze polymer and do ultrathin sections from it, stain
with OsO4 or UA and analyzed it under TEM. Good luck, Sergey.

P.S. In general, you may not use any plastic support film for high
resolution TEM. You need to use thin carbon support film for precise work.

At 09:27 AM 2/19/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 17:20:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi Diane
I know nothing about "colloidal carbon" - does it exist in this
world? From another hand I very doubt that even "colloidal carbon" could
help you. I suppose you want to see the fine details of your sample if
were trying to use negative staining. DNA is 2.4-3 nm in diameter, even
naked DNA may not be visualized well using negative staining. You may see
DNA using "positive staining" but it's quite difficult and you need to use
high-res. STEM and probably Z-contrast (and NEVER Formvar support
film!!!!!). To see any DNA on polymer's background is a big problem because
your polymer will scatter most electrons... Trying to see one polymer
(yours) on another polymer (Formvar) is seems to me even more challenged. I
would suggest, you need to try freeze-fracture in combination with good
SEM. It will give you idea of 3D structure of polymer and you probably
will be able to see some DNA conglomerates (not DNA strands). Sometime
DNA created sort of periodic structure, which you also could see. I know
that some people froze polymer and do ultrathin sections from it, stain
with OsO4 or UA and analyzed it under TEM. Good luck, Sergey.

P.S. In general, you may not use any plastic support film for high
resolution TEM. You need to use thin carbon support film for precise work.

At 09:27 AM 2/19/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 17:23:14 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi Diane
I know nothing about "colloidal carbon" - does it exist in this
world? From another hand I very doubt that even "colloidal carbon" could
help you. I suppose you want to see the fine details of your sample if
were trying to use negative staining. DNA is 2.4-3 nm in diameter, even
naked DNA may not be visualized well using negative staining. You may see
DNA using "positive staining" but it's quite difficult and you need to use
high-res. STEM and probably Z-contrast (and NEVER Formvar support
film!!!!!). To see any DNA on polymer's background is a big problem because
your polymer will scatter most electrons... Trying to see one polymer
(yours) on another polymer (Formvar) is seems to me even more challenged. I
would suggest, you need to try freeze-fracture in combination with good
SEM. It will give you idea of 3D structure of polymer and you probably
will be able to see some DNA conglomerates (not DNA strands). Sometime
DNA created sort of periodic structure, which you also could see. I know
that some people froze polymer and do ultrathin sections from it, stain
with OsO4 or UA and analyzed it under TEM. Good luck, Sergey.

P.S. In general, you may not use any plastic support film for high
resolution TEM. You need to use thin carbon support film for precise work.

At 09:27 AM 2/19/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 17:54:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Chris,
If no one else has given you a perchloric acid-free electrolyte for Ti alloys,
look in "Metallography Principles and Practices" by Vander Voort. He lists
several electrolytes for Ti and Ti alloys in Appendix H that do not contain
perchloric acid.
If you cannot find a Vander Voort book (which you should definitely have before
you start electropolishing Ti), write back to me and I will give you a couple of
recipes out of my copy. I have no experience with using them myself.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "by way of MicroscopyListServer" {cmeyer911-at-yahoo.com}
To: "MicroscopyListserver" {microscopy-at-msa.microscopy.com}
Sent: Wednesday, February 11, 2004 2:23 PM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (richard-at-polymer.kth.se) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, February 19, 2004 at 15:44:28
---------------------------------------------------------------------------

Email: richard-at-polymer.kth.se
Name: Richard Olsson

Organization: Royal Institute of technology

Title-Subject: [Microscopy] [Filtered] MListserver: Epoxy matrix for nanoparticles

Question: Dear listeners,
Can anyone suggest a good curing agent for a regular Bisphenol-A- epichlorohydrin resin (Epon 828 or sililair). I am using magnetic ferrite nanoparticles (20-100nm) and I want to lock them in their positions very quickly after dispersing them with an ultrasonic probe in the epoxy. At the moment I am playing with viscosity to keep them separated in the "pure epoxy" but I also want to cure my epoxy and shorten the curing time to as short as possible so that I can keep them separated in the cured sample.

Thank you all for listening.

Regards from Sweden
Richard Olsson

Ps. I wish to avoid to high exotherms because my sample is 30 millimeters thick and I want to avoid degradation of my matrix.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 21:31:13 2004

Contents Retrieved from Microscopy Listserver Archives
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} Date: Thu, 19 Feb 2004 13:04:49 -0800
} To: Julie.Glasscock-at-csiro.au (by way of MicroscopyListserver)
} From: Gary Gaugler {gary-at-gaugler.com}
} Subject: [Microscopy] Re: viaWWW: Faraday cup
}
} To make a specimen current reading, the stage
} must be isolated such that the Faraday cup
} is electrically brought out of the chamber.
} The BNC connector should do this. However, if
} the BNC connector is not currently shorted via
} a shorting plug, chances are that the stage is
} not isolated. If it were isolated and not
} grounded, the specimens would charge up. You can
} verify continuity by measuring resistance from
} the stage (specimen holder) to door frame ground--
} this should read infinity (no continuity). Then
} read from stage (holder) to center pin of BNC--this
} should read zero Ohms (closed circuit).
}
} If the above checks out, you need a Faraday cup.
} If there is not one in your system, you can buy
} one from SEM supply houses like MSA, et. al. or
} make one. A Faraday cup is a hole in a piece of
} metal or Carbon with a small hole at the top. The
} easiest way to do this is to mount a 100u aperture
} on top of a pin stub that has a hole drilled in it.
}
} Then take a DVM and plug it into the BNC connector.
} Put the DVM on the lowest voltage range and read the
} voltage. Current will be voltage divided by 10^6.
} I=E/R where I is the current, E is the voltage reading
} and R is the ten meg Ohms input resistance of the DVM.
} The jazzy way to do this is to use a picoampmeter.
} But these cost about $1,000 vs. about $100 for a DVM.
}
} gary g.
}
}
} At 06:43 AM 2/19/2004, you wrote:
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 19 22:06:54 2004

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Colleagues

Looks like there was a spam attack while I was on my way back
from across the Pacific. Unfortunately, the long flight mean't
I was off-line for nearly 2 days and a number (but not all) of you appeared
to have been hit by a forged from address during the last 2 days.

Please remember any Email that does not have the phrase

as the begining of the SUBJECT line did not go through the
Listserver Email filters. You should immediately suspect
that message as junk mail, even if it appears to come from
"MICROSCOPY.COM".

I think I have found and plugged the hole that could have allowed the
junk mail to get to some of you. However, remember
the spoofing/faking of Email addresses now abounds and
it is very difficult to track.

Don't be afraid to report suspect Email . I try to
look into everything, to try to minimize problems.

My apologies...

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 00:56:48 2004

Contents Retrieved from Microscopy Listserver Archives
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Nestor,
I think we all know how problematic SPAM gets and how difficult it is to get
rid of it. To be honnest, I'm already surprised that not more gets through,
I guess you must already block a lot of messages! For those who are still
receiving SPAM-messages, it might be interesting to install an extra
SPAM-filter on your email, so it gets double-checked and will decrease the
number even more. Just look around the net, there are a few very good,
cheap or even free anti-SPAM-programs available. We have one here on at the
university and still I get about 15 mails per day on average which were not
blocked. Those senders are really abusing their knowledge I think!
Good luck & best regards,
Sven

-----Original Message-----
} From: Nestor J. Zaluzec [mailto:zaluzec-at-microscopy.com]
Sent: vrijdag 20 februari 2004 05:17
To: microscopy-at-ns.microscopy.com

Colleagues

Looks like there was a spam attack while I was on my way back
from across the Pacific. Unfortunately, the long flight mean't
I was off-line for nearly 2 days and a number (but not all) of you appeared
to have been hit by a forged from address during the last 2 days.

Please remember any Email that does not have the phrase

as the begining of the SUBJECT line did not go through the
Listserver Email filters. You should immediately suspect
that message as junk mail, even if it appears to come from
"MICROSCOPY.COM".

I think I have found and plugged the hole that could have allowed the
junk mail to get to some of you. However, remember
the spoofing/faking of Email addresses now abounds and
it is very difficult to track.

Don't be afraid to report suspect Email . I try to
look into everything, to try to minimize problems.

My apologies...

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 10:38:18 2004

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Listers:

I had asked the list a while ago regards to replacement lamps for a
Microtek 2500F scanner.

A number of folks asked for the outcome, and I also feel it is my
responsibility to inform the scientific community of serious issues with one of
the top recommended scanners.

It seems that for whatever reason microtek will NOT sell or ship
replacement lamps for this scanner. YOU MUST ship the scanner back to
microtek ITSELF. There are no authorized repair facilities (in North America)
other than the single office center in California. Now please folks realize, we
are talking about shiiping a 70 pound, delicate scanner that costs ~ $3K USD,
and that comes in a box as big as a desk across a continent. For a lamp
assembly that is replaced with 6 screws total, and should have a cost of less
than $20.

For anyone out there who has replaced a flat bed scanner lamp you know
exactly how absurd this is.

Please, I urge you DO NOT BUY MICROTEK SCANNERS.

(Anyone want to buy a Scanner? Needs a new lamp.)

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 10:47:00 2004

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I apologize for this double posting made an error in the Web page address -
use the address in this e-mail thank you.

We have a Balzer's 301 Freeze Fracture Apparatus available to anyone who can
take it away. The system was modified by Wiltek and equipped with a digital
vacuum control system, a Mass Spec and Cryopump (there are two cryopumps
both currently non-operational). A brief description and pictures will be
available at http://www.gsisinc.com
If you're interested please contact me, Richard Harris by phone 519-661-2111
ext 86780 or e-mail rjharris-at-uwo.ca.
Thanks

Richard Harris
Laboratory Supervisor
Department of Biology
University of Western Ontario
London Ontario CANADA
Ph. 519-661-2111 ext. 86780
Fax 519-661-3935

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 10:56:02 2004

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Has anyone come up with a way to QC these grids "on the fly"? We've
started using them for IEM and have had a few that weren't totally coated
with Au; the Cu etched in my Tris buffer (yes, I know I can use phosphate
instead). Sometimes it is obvious, but I came in this morning to find 4
blue antibody drops....I was sure these 4 grids were well-coated.

Any ideas? Current thinking is to give up and use these as expensive Cu
grids and go back to annoying Ni for IEM (plain Au is a bit pricey and the
students tend to turn them into tacos).

Thanks!

Tamara

|--------------------------------------------------|
Tamara Howard
Department of Cell Biology and Physiology
University of New Mexico - Health Sciences Center
Albuquerque, NM 87131
thoward-at-unm.edu
|--------------------------------------------------|

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 11:36:46 2004

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Richard,

Have you considered procuring a replacement lamp from another source based on the
identification on the lamp itself? Chances are that Microtek doesn't make it
anyway, they buy it from someone else. It's often the case that the same
replacement part is marked up 100% by the equipment manufacturer if they have to
stock it as a replacement item. You might contact Aristo, Gilway Technical Lamp,
BulbDirect.com or similar. It might be less trouble than packing and shipping the
scanner anywhere and cheaper as well.

John Twilley

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 12:20:26 2004

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Try Pureland Supply as well: www.purelandsupply.com
Randy

-----Original Message-----
} From: John Twilley [mailto:jtwilley-at-sprynet.com]
Sent: Friday, February 20, 2004 12:13 PM
To: edelmare-at-MUOHIO.EDU
Cc: microscopy-at-msa.microscopy.com

Tony,

XEI Scientific makes the Evactron Anti-contaminator for removing oil from
SEM Chambers and X-ray windows. Full details about the Evactron system can
be found at our web site: Evactron.com.

We have just submitted two abstracts to M&M 2004 meeting about this subject:
"A Study of the Effects of Evactron® Plasma Cleaning on X-ray Windows" by
R.Vane, C.Roberts, and V.L. Carlino and "Improved Carbon Analysis with
Evactron Plasma Cleaning" by Pierre Rolland, Vince Carlino, and Ronald Vane

We would be happy to send you preprints. Please e-mail Sales-at-Evactron.com
and request X-ray papers.

Ronald Vane
XEI Scientific

----- Original Message -----
} From: "by way of MicroscopyListserver" {tgreco-at-seas.marine.usf.edu}
To: {microscopy-at-ns.microscopy.com}
Sent: Thursday, February 19, 2004 10:56 AM

} -Diane-

DNA won't stick to formvar. One must use colloidin which is (I
think) some form of nitrocellulose. It is also barely possible to
visualize it by staining. The 1.5 nm diameter limits this technique,
not because it is below the resolving power of the EM, but because
one cannot get enough stain on the double helix to distinguish it
from background by conventional imaging techniques.

} -----------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
__
Carol A. Heckman, Ph.D.
Professor of Biological Sciences
Director, Center for Microscopy & Microanalysis
Bowling Green State University, Bowling Green, OH 43403
fax: (419) 372-2024 email: heckman-at-bgnet.bgsu.edu
___________________________________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 14:56:40 2004

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Jessica,
I guess I will address your question even though you are a Hawkeye.

I would do way with most of the numbers your gave. I would roll most
everything together into a black box and start from scratch. There is
usually a variety of unknown optics in the path so that the
magnification/field of view/pixel spacing is not a straightforward
calculation. There is also the issue that the CCD size is not always
well-matched to the microscope so that the field of view at the camera is
typically not quite the same as through the eyepieces. I simply take an
object of known size and take images of it at various magnifications and
calculate the desired parameters. You could then do a follow-up exercise to
calculate the cumulative effect of the intermediate parts.

Warren, a Cyclone

At 08:43 AM 2/19/2004, you wrote:
} -------------------------------------------------------------------------------
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (jderyk-at-dpi.radiology.uiowa.edu) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Wednesday, February 18, 2004 at 15:32:49
} ---------------------------------------------------------------------------
}
} Email: jderyk-at-dpi.radiology.uiowa.edu
} Name: Jessica deryk
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Confusing calculations
}
} Question: Hi,
} I was hoping someone could help me find, what I thought would be
} fundamental relationships for microscopy but are proving to be difficult
} to determine.
} I have a LeicaMz16a steromicroscope with;
} 7.11x to 155x mag
} FOV range: 29.5mm to 1.82mm
}
} This is coupled to a CCD camera with;
} 1300x1030 pixel array
} pixel spacing: 6.7microns
} FOW: 8.7 x 6.9 mm
}
} I'm wondering how I can accurately calculate the effective FOV as seen by
} the rectangular CCD. Also the relationship between magnification in the
} microscope and resulting pixel spacing of my digital images??
}
} I would appreciate any advice in these calculations or references to texts
} which may contain information regarding interaction between CCD cameras
} and microscopes.
} Thanks
} Jess

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 15:15:01 2004

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We have a Hitachi S2460N that we have been leaving at 40 Pa when idle
(nights and weekends). It has remained clean for almost 10 years now. Our
JEOL 840A could benefit from an XEI system. Since it remains at high
vacuum, we build up oil contamination on the EDS detector as it acts as a
cold finger.

I have been told that some time at 40 Pa would remove contamination after
it built up. I do not know. I suppose it could work, but I don't think the
vapor pressure of the pump oil would be so high as to make it a very fast
process. I think a system such as XEI's which uses an activated species
would do better at removing accumulated contamination. Of course, you still
might want to CAREFULLY clean your dirty x-ray detector first.

You say that even your chamber is dirty. That sounds like an extreme
problem to me. We accumulate oil on the x-ray detector, but I have yet to
see oily surface elsewhere inside our scopes. Maybe there is some other
problem with the vacuum system that a service engineer should examine.

Warren

At 12:56 PM 2/19/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 17:04:23 2004

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I know how to make a composite DAPI, FITC, Rhodamine (i.e., Blue, Green,
Red) color image by pasting the grey scale digital fluorescence images into
the RGB channels but how do you get a 4th color (e.g., Far Red 647) into
the image. I know there must be a simple way that my tired old mind is
forgetting. Could some Photoshop maven help me out? Thanks, Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 20 17:57:11 2004

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Sorry, Tom, you can't do that. Human eyes have three kinds of cones, and
consequently computer displays have three kinds of phosphors. You can generate a
wide range of color combinations with those three phosphors, and so there is no
fourth color available that doesn't occur when the right proportions of the
three are present. Now, if you were a pigeon, you'd have 5 kinds of cones, and
you would have designed monitors with more phosphors, and been able to handle
more independent signals at the same time.

John Russ
========
In a message dated 2/20/04 6:19:40 PM, phillipst-at-missouri.edu writes:

} I know how to make a composite DAPI, FITC, Rhodamine (i.e., Blue, Green,
}
} Red) color image by pasting the grey scale digital fluorescence images
} into
} the RGB channels but how do you get a 4th color (e.g., Far Red 647) into
}
} the image. I know there must be a simple way that my tired old mind is
}
} forgetting. Could some Photoshop maven help me out? Thanks, Tom

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 21 07:08:53 2004

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Tom Phillips writes ...

} I know how to make a composite DAPI, FITC, Rhodamine (i.e.,
} Blue, Green, Red) color image by pasting the grey scale
} digital fluorescence images into the RGB channels but how
} do you get a 4th color (e.g., Far Red 647) into the image.
} ...

Making a composite given R,G & B is straightforward, i.e., all channels
contribute equally to the presentation (if not the aesthetics).
Possibilities for adding a 4th channel are possible, but now you are
confronted with non-equal contributions to the presentation, and with what
channels, for what influence. An example would be to create a CMYK file and
put the grayscales into the 4 channels as you would with 3 into RGB ... but
which channel do you put into the 'K' channel, which might do nothing, or
something strange, with what you're trying to present.

Another possibility is to pick 3 for the RGB channels, and put a yellow
layer on top, and use the 4th channel as a "layer mask". Again it depends
on what you want this 4th channel to present, but this method offers more
flexibility (e.g., use different color layers ... use the mask as 'show' or
'hide' modes ... and you can "blend" the additional layer in any number of
ways, e.g., difference, multiply, etc)

Alas ... in the end, what have you got? Does the image present well? Will
your colleagues understand the presentation? I have this nagging feeling
you're asking "what does everyone else do?" towards creating a presentation
everyone can redily understand. I am not familiar with these channels of
information, but the last possibility is to blend 2 channels into 1, and
your colleagues may need to come to agreement on which channels. For
example, if the channels were elemental spatial maps, you may blend Fe and
Mg because they substitute for each other (usually). At my wwwsite, there
is an example of where I blended Na & Ca for the same reason (plagioclase
feldspar).

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 21 08:30:29 2004

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This is certainly an interesting problem. Of course, the astronomers
deal with similar ones all the time, as they try to assign different
non-visible wavelengths to color images. I would think that you
might be able to assign different combinations of color to each
channel instead of limiting yourself to RGB. One way to think of
this might be to construct specific color look-up-tables for each of
the gray scale images using a program like ImageJ so that each
channel would have its own color structure. Then, you could convert
each of the images to RGB (which would calculate the ratios
automatically) and use Photoshop to overlay one on the other. Areas
of colocalization will appear in interesting combinations, but the
unique areas should show through in the colors that you have
assigned.

Joel

} From: "michael shaffer" {michael-at-shaffer.net}
To: "Tom Phillips" {phillipst-at-missouri.edu} , {Microscopy-at-msa.microscopy.com}

Of course John is right that there are only 3 types of color receptors in
the human eye, and the same number of different phosphors in a CRT, but I
disagree with John that you cannot have more than 3 colors for different
fluorochromes. Unfortunately I cannot speak for Photoshop, as I don't know
enough about that software, but we do that routinely in our mFIP module
(Multiple Fluorescence Image Processing). Instead of assigning just red,
green, and blue, you can also assign other colors, such as, for example,
yellow or magenta and thus create color images with more than 3
fluorochromes.

I don't know how you would do this in Photoshop, but you could, for example,
assign only red to one fluorochrome, green to another, blue to the third,
and blue and red in equal proportions to the fourth.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Friday, February 20, 2004 17:08
To: phillipst-at-missouri.edu; Microscopy-at-msa.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (R.H.Olley-at-reading.ac.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, February 21, 2004 at 10:28:29
---------------------------------------------------------------------------

Email: R.H.Olley-at-reading.ac.uk
Name: Robert H. Olley

Organization: University of Reading

Title-Subject: [Microscopy] [Filtered] MListserver: OM: Phyiscs Experiments

Question: We are finding that computer controlled 'experiments' do not inspire our undergraduates. Does anyone know of suitable physics experiments for students that would use an optical microscope?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 21 11:41:58 2004

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Of course, you can assign another signal to the yellow channel, or the
magenta channel, but it cannot show uniquely that signal, because the colocalization
of red and green will produce an indistinguishable yellow from the one you've
assigned to the additional channel, etc. Doing it in Photoshop is simple -
just convert the RGB image to CMYK and paste into the C M or Y channel (don't
mess with the black channel - you will get some unexpected and unwelcome effects
when you go back to RGB). The problem is that the color channels have become
garbled and may not communicate the intended information. It is usually better
to try to overlay textures on regions to try to illustrate more signal
channels. Or, as someone else has already suggested, try to create derived
combinations of your "pure channel" signals to identify structural regions of interest.
PCA is a good way to pursue getting the three "best" combinations of signals
to put into RGB. To learn more, check out the (rich) literature on satellite
imagery, where the problems of more than 3 channels are old news.

John Russ
=====
In a message dated 2/21/04 11:20:34 AM, mb-at-soft-imaging.com writes:

} Of course John is right that there are only 3 types of color receptors
} in
} the human eye, and the same number of different phosphors in a CRT, but
} I
} disagree with John that you cannot have more than 3 colors for different
} fluorochromes. Unfortunately I cannot speak for Photoshop, as I don't know
} enough about that software, but we do that routinely in our mFIP module
} (Multiple Fluorescence Image Processing). Instead of assigning just red,
} green, and blue, you can also assign other colors, such as, for example,
} yellow or magenta and thus create color images with more than 3
} fluorochromes.
}
} I don't know how you would do this in Photoshop, but you could, for example,
} assign only red to one fluorochrome, green to another, blue to the third,
} and blue and red in equal proportions to the fourth.
}

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 21 12:25:51 2004

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Hank,

These pumps were made by Edwards Vacuum for Philips, as a special order. EP-100, 100 l/s. I doubt you can get a brand new
replacement. You may, however, rebuild this pump at Duniway Stockroom, they do a good job. (650)969-8811 or www.duniway.com

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "Hank Beebe (by way of MicroscopyListServer)" {hbeebe-at-rjlg.com}
To: "MicroscopyListserver" {microscopy-at-msa.microscopy.com}
Sent: Saturday, February 14, 2004 8:03 PM

Robert,

Many years ago, one could use uranium block glass to demonstrate the exit
pupil of the condenser lens, thus showing the affects of changing substage
condenser aperture in brightfield, the hollow cone of darkfield and
Rheinberg, and single azimuth or oblique angle illumination. Furthermore,
students could visually see the affect of changing for instance, the
aperture or condenser height and how these parameters related to numerical
aperture.

However, I do not have access to block glass. Therefore, I use a single
sheet of white notecard stock, approximately 4cm x 4cm, folded 90 degrees.
One portion of the card rests on the stage while the other portion extends
upward toward the objective. You will need to lower your stage or raise
your objective to fit the card into position. The card is then moved just
into position so as to reveal the illumination of the exit pupil and cast in
effect the angular aperture angle on the card.

This is a very simple demonstration and one can 'experiment' with the
condenser optics to understand the relationship of angular aperture, working
distance, and numerical aperture.

I have other suggestions, but this is one of the most simple and
fundamentally important. Good Luck!

Sincerely,
Ken

_______________________________________
Kenneth L. Tiekotter, Adjunct Professor
The University of Portland
Department of Biology
5000 N Willamette Blvd.
Portland, OR 97203 USA

Director, MicroImaging Dx Center
Legacy Portland Hospitals
Legacy Holladay Park Medical Center
1225 NE 2nd Avenue
Portland, OR 97232 USA

Tel.: 503.413.5391

On 2/21/04 8:50 AM, "by way of MicroscopyListserver"
{R.H.Olley-at-reading.ac.uk} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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-
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted
} by (R.H.Olley-at-reading.ac.uk) from
} http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday,
} February 21, 2004 at 10:28:29
} ---------------------------------------------------------------------------
}
} Email: R.H.Olley-at-reading.ac.uk
} Name: Robert H. Olley
}
} Organization: University of Reading
}
} Title-Subject: [Microscopy] [Filtered] MListserver: OM: Phyiscs Experiments
}
} Question: We are finding that computer controlled 'experiments' do not inspire
} our undergraduates. Does anyone know of suitable physics experiments for
} students that would use an optical microscope?
}
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 21 12:58:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jcma01-at-students.stir.ac.uk) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, February 21, 2004 at 12:35:51
---------------------------------------------------------------------------

Email: jcma01-at-students.stir.ac.uk
Name: Jafet

Organization: University of Stirling

Education: Undergraduate College

Location: Stirling, Scotland, Great Britaion

Question: Hi!

I'm a relatively new ligth microscope user. I've been working with a compound microscope full time for a week now. After a few hours of use, my eyes (especially one eye) get sore and eventually I get a headace. Is this normal? Can prolonged use lead to eye damage? Can anything be done to avoid it?

Thanks alot!

/Jafet

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Feb 22 12:11:35 2004

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Hi folks,

I continue to have problems getting uranyl acetate into solution
(aqueous or acetone) so that it not only goes in but stays in for a
reasonable period of time (weeks preferably). Concentrations can vary from
0.5% to 2% but the problem remains. I have tried uranyl acetate from a
number of different sources and still have minimal luck.

What we do now is put the required amount into the solvent and then let
stir on a magnetic stirrer, often for hours. Then we filter out what does
not dissolve. Of course this leaves an unknown concentration in the final
solution.

Does anyone have a brand to recommend that dissolves well or any special
tricks?

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 03:22:06 2004

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Dear Debby
Uranyl Acetate is quite soluble in the water. 1-2% (w/v) aqueous solutions
are stable in the dark at +4oC for a few months. Usually I dissolve UA in
plastic tube with gentle shaking. It's completely dissolved in about 40
min at RT. If your "uranyl acetate" is not dissolved in water, it means,
it's not UA from chemical point of view. Perhaps, it's uranyl nitrate,
which is less dissolvable in water... I would think EVERY EM supplier will
be happy to supply you with fresh real uranyl acetate which SHOULD be
dissolvable in the water by Merck Index... Sergey

At 01:25 PM 2/22/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 07:10:10 2004

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Jafet;

You'll want to make sure that both eyepieces are adjusted correctly. That is, one or both will have an adjustment that can compensate for the difference in vision between the eyes. If these are significantly out of focus you may have the symptoms you describe. It also helps to keep lenses and mirrors clean. In the end, see your eye care physician to make sure you don't have any issues with your eyes themselves.

Hope that's of some help.

Peter

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:jcma01-at-students.stir.ac.uk]
Sent: Saturday, February 21, 2004 2:09 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jcma01-at-students.stir.ac.uk) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, February 21, 2004 at 12:35:51
---------------------------------------------------------------------------

Email: jcma01-at-students.stir.ac.uk
Name: Jafet

Organization: University of Stirling

Education: Undergraduate College

Location: Stirling, Scotland, Great Britaion

Question: Hi!

I'm a relatively new ligth microscope user. I've been working with a compound microscope full time for a week now. After a few hours of use, my eyes (especially one eye) get sore and eventually I get a headace. Is this normal? Can prolonged use lead to eye damage? Can anything be done to avoid it?

Thanks alot!

/Jafet

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 07:43:42 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

As it was explained to me, (I'm blind in one eye so cannot say that it
works, but it should) -

One of the two eyepieces on the compound microscope should have a focusing
ring on it. The other should not. Look with one eye through the eyepiece
that does not, and focus it with the microscope's focusing knob(s).

Look with the other eye through the eyepiece that has its own focusing ring
and, use only that ring to focus the image in that eye. Finally, adjust the
eyepieces sideways to match your interpupilar distance by moving the
eyepieces either closer together or further apart.

Ron L

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Jafet;

You'll want to make sure that both eyepieces are adjusted correctly. That
is, one or both will have an adjustment that can compensate for the
difference in vision between the eyes. If these are significantly out of
focus you may have the symptoms you describe. It also helps to keep lenses
and mirrors clean. In the end, see your eye care physician to make sure you
don't have any issues with your eyes themselves.

Hope that's of some help.

Peter

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:jcma01-at-students.stir.ac.uk]

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (jcma01-at-students.stir.ac.uk) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, February
21, 2004 at 12:35:51
---------------------------------------------------------------------------

Email: jcma01-at-students.stir.ac.uk
Name: Jafet

Organization: University of Stirling

Education: Undergraduate College

Location: Stirling, Scotland, Great Britaion

Question: Hi!

I'm a relatively new ligth microscope user. I've been working with a
compound microscope full time for a week now. After a few hours of use, my
eyes (especially one eye) get sore and eventually I get a headace. Is this
normal? Can prolonged use lead to eye damage? Can anything be done to avoid
it?

Thanks alot!

/Jafet

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 07:47:49 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Peter writes ...

} You'll want to make sure that both eyepieces are adjusted
} correctly. That is, one or both will have an adjustment that can
} compensate for the difference in vision between the eyes. If
} these are significantly out of focus you may have the symptoms
} you describe. It also helps to keep lenses and mirrors clean.
} In the end, see your eye care physician to make sure you don't
} have any issues with your eyes themselves.

I would only add, ... my experience with my users having eye strain problems
usually finds that they haven't yet found a way to relax and focus their
eyes at infinity ... and then make the ocular and eyepiece adjustments.
I've also not yet found a way for them to take a systematic approach
(suggestions?) ... but what can help is to gaze out the window at infinity
for a short period, and then switch to the m'scope and make adjustments
while similarly relaxed.

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

Jafet asks ...

} I'm a relatively new ligth microscope user. I've been working
} with a compound microscope full time for a week now. After a few
} hours of use, my eyes (especially one eye) get sore and
} eventually I get a headace. Is this normal? Can prolonged use
} lead to eye damage? Can anything be done to avoid it?

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 07:57:03 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Sergey,
I am using uranyl acetate not uranyl nitrate. At least I believe the
label on the bottles. I have gotten it from leading supply houses recently
and also have some older bottles from a variety of supply houses. This is
not a new problem...one I have had over many years. Apparently from the
response to my E-mail lots of others have the same problem.

Keeping the solution dark does help slow down precipitation but it still
occurs and this does not help with the initial dissolving of the reagent.

One solution seems to be to add acetic acid to the water to lower pH. The pH
of water, although usually acidic, does vary depending on the purification
method. Does anyone know the optimum pH for dissolving UA? This solution
however will not work with acetone when you want to add UA for freeze
substitution.

Perhaps we need to forget the percentages listed in all the methods and
just admit that we are using "saturated" solutions of UA or report the pH
just like you do with other solutions.

Debby

On 2/23/04 4:40 AM, "Sergey Ryazantsev" {sryazant-at-ucla.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Dear Debby
} Uranyl Acetate is quite soluble in the water. 1-2% (w/v) aqueous solutions
} are stable in the dark at +4oC for a few months. Usually I dissolve UA in
} plastic tube with gentle shaking. It's completely dissolved in about 40
} min at RT. If your "uranyl acetate" is not dissolved in water, it means,
} it's not UA from chemical point of view. Perhaps, it's uranyl nitrate,
} which is less dissolvable in water... I would think EVERY EM supplier will
} be happy to supply you with fresh real uranyl acetate which SHOULD be
} dissolvable in the water by Merck Index... Sergey
}
} At 01:25 PM 2/22/2004 -0500, you wrote:
}
}
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } Hi folks,
} }
} } I continue to have problems getting uranyl acetate into solution
} } (aqueous or acetone) so that it not only goes in but stays in for a
} } reasonable period of time (weeks preferably). Concentrations can vary from
} } 0.5% to 2% but the problem remains. I have tried uranyl acetate from a
} } number of different sources and still have minimal luck.
} }
} } What we do now is put the required amount into the solvent and then let
} } stir on a magnetic stirrer, often for hours. Then we filter out what does
} } not dissolve. Of course this leaves an unknown concentration in the final
} } solution.
} }
} } Does anyone have a brand to recommend that dissolves well or any special
} } tricks?
} }
} } Debby
} }
} } Debby Sherman, Manager Phone: 765-494-6666
} } Life Science Microscopy Facility FAX: 765-494-5896
} } Purdue University E-mail: dsherman-at-purdue.edu
} } S-052 Whistler Building
} } 170 S. University Street
} } West Lafayette, IN 47907
} } http://www3.agriculture.purdue.edu/microscopy
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 07:58:49 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

As it was explained to me, (I'm blind in one eye so cannot say that it
works, but it should) -

One of the two eyepieces on the compound microscope should have a focusing
ring on it. The other should not. Look with one eye through the eyepiece
that does not, and focus it with the microscope's focusing knob(s).

Look with the other eye through the eyepiece that has its own focusing ring
and, use only that ring to focus the image in that eye. Finally, adjust the
eyepieces sideways to match your interpupilar distance by moving the
eyepieces either closer together or further apart.

Ron L

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Jafet;

You'll want to make sure that both eyepieces are adjusted correctly. That
is, one or both will have an adjustment that can compensate for the
difference in vision between the eyes. If these are significantly out of
focus you may have the symptoms you describe. It also helps to keep lenses
and mirrors clean. In the end, see your eye care physician to make sure you
don't have any issues with your eyes themselves.

Hope that's of some help.

Peter

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:jcma01-at-students.stir.ac.uk]

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (jcma01-at-students.stir.ac.uk) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, February
21, 2004 at 12:35:51
---------------------------------------------------------------------------

Email: jcma01-at-students.stir.ac.uk
Name: Jafet

Organization: University of Stirling

Education: Undergraduate College

Location: Stirling, Scotland, Great Britaion

Question: Hi!

I'm a relatively new ligth microscope user. I've been working with a
compound microscope full time for a week now. After a few hours of use, my
eyes (especially one eye) get sore and eventually I get a headace. Is this
normal? Can prolonged use lead to eye damage? Can anything be done to avoid
it?

Thanks alot!

/Jafet

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 09:39:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Debby,

We have always used a saturated soltn of uranyl acetate in water for staining
grids; when we make it up, we stir overnight, then once it settles, we use the
"clear" stain. For use, we dilute the saturated UA 1:1 with 100% methanol and
then filter through a 0.4 micron syringe filter into the Hiroaka staining
trough. We have never had bad results.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Debby Sherman [mailto:dsherman-at-purdue.edu]
Sent: Monday, February 23, 2004 9:11 AM
To: Sergey Ryazantsev; message to: MSA list

Sergey,
I am using uranyl acetate not uranyl nitrate. At least I believe the
label on the bottles. I have gotten it from leading supply houses recently
and also have some older bottles from a variety of supply houses. This is
not a new problem...one I have had over many years. Apparently from the
response to my E-mail lots of others have the same problem.

Keeping the solution dark does help slow down precipitation but it still
occurs and this does not help with the initial dissolving of the reagent.

One solution seems to be to add acetic acid to the water to lower pH. The pH
of water, although usually acidic, does vary depending on the purification
method. Does anyone know the optimum pH for dissolving UA? This solution
however will not work with acetone when you want to add UA for freeze
substitution.

Perhaps we need to forget the percentages listed in all the methods and
just admit that we are using "saturated" solutions of UA or report the pH
just like you do with other solutions.

Debby

On 2/23/04 4:40 AM, "Sergey Ryazantsev" {sryazant-at-ucla.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Dear Debby
} Uranyl Acetate is quite soluble in the water. 1-2% (w/v) aqueous solutions
} are stable in the dark at +4oC for a few months. Usually I dissolve UA in
} plastic tube with gentle shaking. It's completely dissolved in about 40
} min at RT. If your "uranyl acetate" is not dissolved in water, it means,
} it's not UA from chemical point of view. Perhaps, it's uranyl nitrate,
} which is less dissolvable in water... I would think EVERY EM supplier will
} be happy to supply you with fresh real uranyl acetate which SHOULD be
} dissolvable in the water by Merck Index... Sergey
}
} At 01:25 PM 2/22/2004 -0500, you wrote:
}
}
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } Hi folks,
} }
} } I continue to have problems getting uranyl acetate into solution
} } (aqueous or acetone) so that it not only goes in but stays in for a
} } reasonable period of time (weeks preferably). Concentrations can vary from
} } 0.5% to 2% but the problem remains. I have tried uranyl acetate from a
} } number of different sources and still have minimal luck.
} }
} } What we do now is put the required amount into the solvent and then let
} } stir on a magnetic stirrer, often for hours. Then we filter out what does
} } not dissolve. Of course this leaves an unknown concentration in the final
} } solution.
} }
} } Does anyone have a brand to recommend that dissolves well or any special
} } tricks?
} }
} } Debby
} }
} } Debby Sherman, Manager Phone: 765-494-6666
} } Life Science Microscopy Facility FAX: 765-494-5896
} } Purdue University E-mail: dsherman-at-purdue.edu
} } S-052 Whistler Building
} } 170 S. University Street
} } West Lafayette, IN 47907
} } http://www3.agriculture.purdue.edu/microscopy
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 09:57:26 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Michael (and all)

} I would only add, ... my experience with my users having eye strain problems
} usually finds that they haven't yet found a way to relax and focus their
} eyes at infinity ... and then make the ocular and eyepiece adjustments.
} I've also not yet found a way for them to take a systematic approach
} (suggestions?)

Having in the beginnig the same problem, I found very much help in an old
booklet from Zeiss, were they wrote :
"don't look IN the microscope, but TROUGH the microscope"

It's only psychology, but it helps. You must look "at the object" and not
"in the microscope", and when you have forgotten the microscope, it's OK.
It's the same thing looking a deer or a rabbit trough glasses.

Jacques Faerber
IPCMS

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 10:02:04 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Fellow List Members,

Members in the Greater Baltimore-Washingon, D.C. area are cordially invited to "Cryoultramicrotomy Techniques for The Biomedical and Biological Sciences."

There is no charge for this workshop, and refreshments will be served!

When:
Thursday, March 4, 9:30am - 5:00pm
Friday, March 5, 9:30am - 2:00pm

Where:
Johns Hopkins University Medical School
Ross Bldg., #529
720 Rutland
Baltimore, MD 21205

What:
A two-day "mini-workshop" with lectures, presentations, demonstrations and hands-on sessions for cryoultramicrotomy and associated techniques (cryo tool making, glass knife making, evaluation of glass knives, care and cleaning of diamond knives, operation of the ultramicrotome and immunoelectron microscopy).

Important Info:
Attendance is open (but space is limited) for all of the presentations and demonstrations on Thursday, March 4th. The lecture room can accommodate approximately 15 people.

Also due to space requirements, attendance is limited to 12 people for the cryoultramicrotomy hands-on sessions on Friday, March 5th.

Contact:
For additional details, to RSVP or to reserve a spot for the hands-on sessions, please contact Kim Megaw at Boeckeler Instruments, Inc. ( {Kim-at-boeckeler.com} , 800.552.2262).

Sponsors and Organizers:
RMC Products Group, Boeckeler Instruments, Inc.

Dr. David Ryugo's Laboratory
Department of Neuroscience
Johns Hopkins School of Medicine

Hope to see you there!

Bob Chiovetti
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 13:54:13 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Fellow ListServer Users:

I am in the process of repairing a JEOL JSM T200 SEM. One of the scan circuits in the electron optic system is not operational. The problem seems to be related to the "Operation Board".

The PK00023 EF version of the Operation Board schematics I have on hand do not quite match the the circuit board that is installed in the SEM, they are a different revision level. I have contacted JEOL and they no longer seem to have the one I need.

I am looking for a schematic for the PH00023 EF version of the Operation Board.

Any assistance or direction, will be much appreciated.

Best Regards,

Grant Baumgardner

Arizona State University
Center for High Resolution Microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 15:00:11 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Debby
Yes, I think it's a water problem.
I usually use 20 Mohm/cm2 "cell culture" grade water from Milli-Q
(Millipore). pH of water depends from CO2 presence and are not
characteristic. Usually, at the normal circumstances, water exposures to
the air has pH 5-5.5. Basic water pH usually indicates germ contamination
(on the filter, lines etc). In Russia we used to use double-distilled in
quartz water without any problems. According Merck Index, UA is soluble in
10 parts of water, which means 10%.
Try Ted Pella UA Cat # 19481 - it works fine to me - no special preference
is given to Ted Pella.
The bottom line, perhaps, (I never think about it) water should be acidic,
not basic. Sergey

At 06:10 AM 2/23/2004, you wrote:
} Sergey,
} I am using uranyl acetate not uranyl nitrate. At least I believe the
} label on the bottles. I have gotten it from leading supply houses recently
} and also have some older bottles from a variety of supply houses. This is
} not a new problem...one I have had over many years. Apparently from the
} response to my E-mail lots of others have the same problem.
}
} Keeping the solution dark does help slow down precipitation but it still
} occurs and this does not help with the initial dissolving of the reagent.
}
} One solution seems to be to add acetic acid to the water to lower pH. The pH
} of water, although usually acidic, does vary depending on the purification
} method. Does anyone know the optimum pH for dissolving UA? This solution
} however will not work with acetone when you want to add UA for freeze
} substitution.
}
} Perhaps we need to forget the percentages listed in all the methods and
} just admit that we are using "saturated" solutions of UA or report the pH
} just like you do with other solutions.
}
} Debby
}
}
}
} On 2/23/04 4:40 AM, "Sergey Ryazantsev" {sryazant-at-ucla.edu} wrote:
}
} }
} }
} }
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ------------------------------------------------------------------------------}
} -
} }
} } Dear Debby
} } Uranyl Acetate is quite soluble in the water. 1-2% (w/v) aqueous solutions
} } are stable in the dark at +4oC for a few months. Usually I dissolve UA in
} } plastic tube with gentle shaking. It's completely dissolved in about 40
} } min at RT. If your "uranyl acetate" is not dissolved in water, it means,
} } it's not UA from chemical point of view. Perhaps, it's uranyl nitrate,
} } which is less dissolvable in water... I would think EVERY EM supplier will
} } be happy to supply you with fresh real uranyl acetate which SHOULD be
} } dissolvable in the water by Merck Index... Sergey
} }
} } At 01:25 PM 2/22/2004 -0500, you wrote:
} }
} }
} } }
} -----------------------------------------------------------------------------} }
} -
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} -----------------------------------------------------------------------------
} } } --
} } }
} } } Hi folks,
} } }
} } } I continue to have problems getting uranyl acetate into solution
} } } (aqueous or acetone) so that it not only goes in but stays in for a
} } } reasonable period of time (weeks preferably). Concentrations can vary
} from
} } } 0.5% to 2% but the problem remains. I have tried uranyl acetate from a
} } } number of different sources and still have minimal luck.
} } }
} } } What we do now is put the required amount into the solvent and
} then let
} } } stir on a magnetic stirrer, often for hours. Then we filter out what does
} } } not dissolve. Of course this leaves an unknown concentration in the final
} } } solution.
} } }
} } } Does anyone have a brand to recommend that dissolves well or any special
} } } tricks?
} } }
} } } Debby
} } }
} } } Debby Sherman, Manager Phone: 765-494-6666
} } } Life Science Microscopy Facility FAX: 765-494-5896
} } } Purdue University E-mail: dsherman-at-purdue.edu
} } } S-052 Whistler Building
} } } 170 S. University Street
} } } West Lafayette, IN 47907
} } } http://www3.agriculture.purdue.edu/microscopy
} }
} }
} }

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 15:28:57 2004

Contents Retrieved from Microscopy Listserver Archives
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Debby,

In the UA that is commercially available (radioactively "depleted", but
probably irrelevant to this discussion on solubility) there is always a
small amount of totally insoluable (in water) "contaminant" - that according
to my vendor whom I discussed this with about 5 years ago.

So when I mix up 3% UA in distilled water, I stir it on magnetic mixer for
an hour, add 1 drop of concentrated glacial acetic acid per 10.0 ml of stain
to reduce long term U ppt formation (it works, I've kept small vials of
stain from same batch with and without the GAA and is less ppt in the GAA
treated stain), then let it stand overnight, and carefully pipet off the
clear UA into a clean, clear glass bottle, store inside a dark box. It will
stay clear with no ppt gathering on the bottom of the bottle for about 1-2
months, then maybe a real fine layer may be discerned on the bottle bottom,
at which point we filter it through 0.2 micron filters as we use it.

By the way, I collected some of that insoluble component that settled out
during the night after dissolving the UA, washed those crystals with
distilled water to get off any residual UA, and did EDS on them in my
SEM/EDS machine. All crystals examined had high to medium amounts of
titanium, Silicon and uranium in them, medium amounts of oxygen, low amounts
of iron and aluminum, some with low phosphorous. So the crystals are
probably a mix of 2-3 types of an insoluable uranium compound.

As for ending up with unknown concentration from filtering, you're probably
still pretty close to the 2% target you use, and if you mix up same
way/amount each time and stain for some empirically determined time, at
least you'll be consistent.

In sum, there will always be some insoluable crystals left when dissolving
UA, so handle as above to minimize or eliminate ppt from that source on
sections.

Gib
--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra

} Hi folks,
}
} I continue to have problems getting uranyl acetate into solution
} (aqueous or acetone) so that it not only goes in but stays in for a
} reasonable period of time (weeks preferably). Concentrations can vary from
} 0.5% to 2% but the problem remains. I have tried uranyl acetate from a
} number of different sources and still have minimal luck.
}
} What we do now is put the required amount into the solvent and then let
} stir on a magnetic stirrer, often for hours. Then we filter out what does
} not dissolve. Of course this leaves an unknown concentration in the final
} solution.
}
} Does anyone have a brand to recommend that dissolves well or any special
} tricks?
}
} Debby
}
} Debby Sherman, Manager Phone: 765-494-6666
} Life Science Microscopy Facility FAX: 765-494-5896
} Purdue University E-mail: dsherman-at-purdue.edu
} S-052 Whistler Building
} 170 S. University Street
} West Lafayette, IN 47907
} http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 15:31:16 2004

Contents Retrieved from Microscopy Listserver Archives
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I think, the problem here what you want from the final image. If you just
want to have "map" with sort of color table for each stain (like one area
is green, another -pink etc), in this case you could not owerlap areas. Or
you need to represent amount of stain (let say brighter red means more your
rhodamine stain)- if so, you may not introduce other than RGB channels as
John Russ absolutely correctly pointed out. If you will introduce other
than RGB colors - you may not quantitate anymore because yellow may be your
"4th color" or just superposition of "red" and "green" from other
stains... the same for any other colors because all of them are
superposition of RGB by definition. I think, more scientific way to
represent such data is to present gray (or real color) images for all your
stains and show separately superposition of RGB for 3 stains, so you need
more than one superimposed color picture for more than 3 stains. It's also
make sence, because in real you have red, green and blue fluorescence. Sergey

At 08:02 AM 2/21/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 17:55:28 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Grant.Baumgardner-at-asu.edu) from on Monday, February 23, 2004 at 11:12:14
---------------------------------------------------------------------------

Email: Grant.Baumgardner-at-asu.edu
Name: Grant Baumgardner

Organization: Arizona State University Center for High Resolution Microscopy

Title-Subject: [Microscopy] [Filtered] MListserver: Correct Schematics for JEOL JSM T200

Question: Dear Fellow ListServer Users:

I am in the process of repairing a JEOL JSM T200 SEM. One of the scan circuits in the electron optic system is not operational. The problem seems to be related to the "Operation Board".

The PK00023 EF version of the Operation Board schematics I have on hand do not quite match the the circuit board that is installed in the SEM, they are a different revision level. I have contacted JEOL and they no longer seem to have the one I need.

I am looking for a schematic for the PH00023 EF version of the Operation Board.

Any assistance or direction, will be much appreciated.

Best Regards,

Grant Baumgardner

Arizona State University
Center for High Resolution Microscopy

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Feb 23 20:56:38 2004

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All arc lamps require a warmup period. 40 min is about the minimum.
How long do you leave the burner running? They do not like being switched
off and on a few times a day. It leads to a short life.

New burners require a burn in period before they are stable, IIRC it is a
period of several hours.

I haven't seen a comparison study of stability between mercury and Xenon
arc lamps. I do know that the DC mercury burners produce a more stable
arc with less flicker than the AC varieties.

Neither is an inexpensive upgrade, usually requiring a new power supply,
socket and maybe a new lamp house as well to obtain the proper optics for
the new bulb.

Bob

On 12 Feb 2004, at 19:23, Marie-Claude Bélanger wrote:
}
} Dear all,
}
} I have a couple questions regarding the illumination stability of mercury
} burners:
}
} 1- When a new burner is installed, is there a period of time (within a few
} hours) where the intensity increases to a plateau? With an older lamp,
} everytime we turn the lamp on, we have observed that it takes about 40 minutes
} to reach a plateau. We installed a new burner recently, and images have been
} brighter from day to day for the first 3 days and remained stable afterwards.
} Is it just a coincidence?
}
} 2- To solve the stability problems we have with the mercury burners, we’re
} considering the use of xenon lamps. Is there somewhere a comparative stability
} study of the 2 types of burners?
}
} Thank you.
}
}
}
} Marie-Claude Belanger
}
} _________________________________________________________________
} MSN Messenger : discutez en direct avec vos amis !
} http://messenger.fr.msn.ca/
}

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 09:06:45 2004

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Thank you Bob, for this valuable information.

As an addendum, I received another information from Sylvania-Osram, stating
that the burn in period for a new lamp is 24 hours.

Marie-Claude Belanger

On 23 Feb 2004, at 21:03, Bob Sunley wrote:

}
} All arc lamps require a warmup period. 40 min is about the minimum.
} How long do you leave the burner running? They do not like being switched
} off and on a few times a day. It leads to a short life.
}
} New burners require a burn in period before they are stable, IIRC it is a
} period of several hours.
}
} I haven't seen a comparison study of stability between mercury and Xenon
} arc lamps. I do know that the DC mercury burners produce a more stable
} arc with less flicker than the AC varieties.
}
} Neither is an inexpensive upgrade, usually requiring a new power supply,
} socket and maybe a new lamp house as well to obtain the proper optics for
} the new bulb.
}
} Bob
}
} On 12 Feb 2004, at 19:23, Marie-Claude Bélanger wrote:
} }
} } Dear all,
} }
} } I have a couple questions regarding the illumination stability of
} mercury
} } burners:
} }
} } 1- When a new burner is installed, is there a period of time (within a
} few
} } hours) where the intensity increases to a plateau? With an older lamp,
} } everytime we turn the lamp on, we have observed that it takes about 40
} minutes
} } to reach a plateau. We installed a new burner recently, and images have
} been
} } brighter from day to day for the first 3 days and remained stable
} afterwards.
} } Is it just a coincidence?
} }
} } 2- To solve the stability problems we have with the mercury burners,
} we’re
} } considering the use of xenon lamps. Is there somewhere a comparative
} stability
} } study of the 2 types of burners?
} }
} } Thank you.
} }
} }
} }
} } Marie-Claude Belanger
} }
} } _________________________________________________________________
} } MSN Messenger : discutez en direct avec vos amis !
} } http://messenger.fr.msn.ca/
} }
}
}

_________________________________________________________________
MSN Search, le moteur de recherche qui pense comme vous !
http://fr.ca.search.msn.com/

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 10:28:39 2004

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Nestor:

I think you do a great job! Many thanks.
Gail

} I think I have found and plugged the hole that could have allowed the
} junk mail to get to some of you. However, remember
} the spoofing/faking of Email addresses now abounds and
} it is very difficult to track.
}
} Don't be afraid to report suspect Email . I try to
} look into everything, to try to minimize problems.
}
}
} My apologies...
}
} Nestor
} Your Friendly Neighborhood SysOp
}
}

Gail S. Kenner
Department of Botany
University of British Columbia
3529-6270 University Blvd.
Vancouver, British Columbia V6T 1Z4
Canada

tel: (604) 822-5223
FAX: (604) 822-6089

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 12:38:32 2004

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I searching for information on the Olympus Video archiving system (VAS)
II. I have one, and I have been asked to determine if we can network the
system to down load images to other work stations. There are ports on the
back of the unit, but I can find no reference to what they are for, nor can
I find any software for the darn thing. Any help would be appreciated!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 14:14:31 2004

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A colleague asked for any information on the following:

Plastic coverslips. They used to be made by a company
called Oncor
Cat # S1370-14. The company doesn't make them anymore and
web searches for them using google only turns up the
thermanox
coverlips. If anyone knows anything about them, such as
what type of plastic it is or any other plastic companies
that make something like this.

If any one knows any thing about this product she would be
most grateful. I will pass along any information that
anyone has.

Thanks.

ML

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 14:39:51 2004

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Hi,
We used the Thermonox coverslips since the 70's for SEM preps of tissue
cultures, bacteria, bacterial spores, etc. At least then, the coverslips
withstood the solutions normally used for SEM i.e. G-Os,EtOH, then
either CPD or Freeze Drying. They certainly withstood metal coatings
and evaporator heat as well.
Hope that is helpful.

Judy M.

Judy Murphy, PhD
San Joaquin Delta College
Microscopy Technology
5151 Pacific Ave
Stockton, CA 95207
209-954-5284
FAX 209-954-5600
jmurphy-at-deltacollege.edu
http://www.sjdccd.cc.ca.us/dept/electmicro/index.html

Mei Lie Wong wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} A colleague asked for any information on the following:
}
} Plastic coverslips. They used to be made by a company
} called Oncor
} Cat # S1370-14. The company doesn't make them anymore and
} web searches for them using google only turns up the
} thermanox
} coverlips. If anyone knows anything about them, such as
} what type of plastic it is or any other plastic companies
} that make something like this.
}
} If any one knows any thing about this product she would be
} most grateful. I will pass along any information that
} anyone has.
}
} Thanks.
}
} ML

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 14:43:04 2004

Contents Retrieved from Microscopy Listserver Archives
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Try Fisher Scientific's unbreakable cover slips (catolog number 12-547). I
don't know if they will meet your needs, but I use them for making
impressions of hair scales and they work quite nicely.

Best wishes.........

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 15:12:22 2004

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Hi,

What is a good embedding media for bone ultramicrotomy?
I use Epon 812 and Spurr resin, but penetration is not really
good enough.

Thanks,

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 15:13:20 2004

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Dear colleagues,
how do you archive pictures taken by digital camera?
There is some problems with images and data stored on the CD.

Keep care and be of good cheer

Regards

(name) Vratislav Richard Eugene Maria John Baptist
(surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

Tenebrionidae of the World, incl. Alleculinae and Lagriinae,
higher taxonomy, Australian beetles.
websites:
http://www.coleoptera.org. and
http://www.egroups.com/group/coleoptera

University of Sydney
The Wentworth Bldg., B 62
NSW 2006
AUSTRALIA
phone : +61 414 540 465
email: ricardo-at-ans.com.au
vratislav-at-bigfoot.com
ICQ: 13610107

Only after the last tree has been cut down,
only after the last river has been poisoned,
only after the last fish has been caught,
only then will you find that money can not be eaten.'
CREE INDIAN PROPHECY.

Incoming mail is certified Virus Free.
Checked by AVG anti-virus system (http://www.grisoft.com).

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 17:19:29 2004

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There can be problems archiving files to cheap
CDs. Same for DVDs. A good approach is to use
Mitsui CDs and DVDs. Never had a problem. A
bit more expensive but well worth the non-loss
of precious data. Be sure that your burning
software performs a verify after burn.

gary g.

At 01:27 PM 2/24/2004, you wrote:

} Dear colleagues,
} how do you archive pictures taken by digital camera?
} There is some problems with images and data stored on the CD.
}
} Keep care and be of good cheer
}
} Regards
}
} (name) Vratislav Richard Eugene Maria John Baptist
} (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 21:14:30 2004

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As a computer network admin type, I can't emphasize enough to burn 3
copies on good media. CDR's are not really archival media yet. They do
last a good while, but they are easily damaged and they do die a natural
death.

Bob

On 24 Feb 2004, at 15:32, Gary Gaugler wrote:

}
} There can be problems archiving files to cheap
} CDs. Same for DVDs. A good approach is to use
} Mitsui CDs and DVDs. Never had a problem. A
} bit more expensive but well worth the non-loss
} of precious data. Be sure that your burning
} software performs a verify after burn.
}
} gary g.
}
}
} At 01:27 PM 2/24/2004, you wrote:
}
} } Dear colleagues,
} } how do you archive pictures taken by digital camera?
} } There is some problems with images and data stored on the CD.
} }
} } Keep care and be of good cheer
} }
} } Regards
} }
} } (name) Vratislav Richard Eugene Maria John Baptist
} } (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 21:46:33 2004

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This topic has been discussed before. The bottom line
is to backup to quality CD/DVD media and to redundantly
backup to tape. I use Ultrium 2 LTO. Yes, the CDs and
DVDs are duplicated (just 2) but only one LTO tape.
I have never lost a file. However, having said that,
I do keep copies on Dell NAS servers.

gary g.

At 07:28 PM 2/24/2004, you wrote:

} As a computer network admin type, I can't emphasize enough to burn 3
} copies on good media. CDR's are not really archival media yet. They do
} last a good while, but they are easily damaged and they do die a natural
} death.
}
} Bob
}
}
} On 24 Feb 2004, at 15:32, Gary Gaugler wrote:
}
} }
} } There can be problems archiving files to cheap
} } CDs. Same for DVDs. A good approach is to use
} } Mitsui CDs and DVDs. Never had a problem. A
} } bit more expensive but well worth the non-loss
} } of precious data. Be sure that your burning
} } software performs a verify after burn.
} }
} } gary g.
} }
} }
} } At 01:27 PM 2/24/2004, you wrote:
} }
} } } Dear colleagues,
} } } how do you archive pictures taken by digital camera?
} } } There is some problems with images and data stored on the CD.
} } }
} } } Keep care and be of good cheer
} } }
} } } Regards
} } }
} } } (name) Vratislav Richard Eugene Maria John Baptist
} } } (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Tue Feb 24 23:46:48 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1a ] --

Vladimir Dusevich wrote:
================================================================
What is a good embedding media for bone ultramicrotomy?
I use Epon 812 and Spurr resin, but penetration is not really
good enough.
===============================================================\
I would refer you to the publications of M. Cole, a few of which are listed
below:

Cole, M. B., Jr., Gylcol methacrylate embedding of bone and
cartilage for light microscopic staining,
J. Microsc. (Oxf), 127, 139-148 (1982).

This was taken from a longer list of publications on URL
http://www.2spi.com/catalog/chem/rep-references.html

The SPI-Chem™ Brand Low Acid GMA is based on the work of Dr. Cole. See URL
http://www.2spi.com/catalog/chem/embed4.shtml

The GMA monomer is perhaps the most "infiltrateable" resin of all, since it
has a viscosity slightly less than that of water. Another advantage of the
GMA system is that dehydration is not necessary since some water is needed
to make the polymerization occur. It has been used widely on both bone,
cartilage, and teeth.

Chuck

Disclaimer: SPI Supplies is the supplier of the SPI-Chem brand Low Acid GMA

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 05:05:01 2004

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Vladimir Dusevich wrote:
================================================================
What is a good embedding media for bone ultramicrotomy?
I use Epon 812 and Spurr resin, but penetration is not really
good enough.

I asked my colleque Saddha Cuijpers and she wrote me this answer:

Working with archaeological bone and especially with cremated remains the
embedding agent Biodur E12 in combination with E1 (Dr. G. von Hagens,
Heidelberg) works very good and is easy to apply.
This two-component resin infiltrates unburnt bone without trouble and gives
a good clear histological picture under the microscope.
When dealing with burnt bone fragments, however, a cover glass is glued on
the top before cutting to keep this material together, because cremated
bone is not easily infiltrated.
Reference:
Herrmann, B., G. Grupe, S. Hummel, H. Piepenbrink & H. Schutkowski (1990).
Prähistorische Anthropologie. Berlin: Springer Verlag, pp. 186-207.
van der Lubbe e.a., 1988. A simple method fo preparing thin histological
sections of undecalcified plastic embedded bone with implants.in Stain
Technology 63, 171-176.

Ineke

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 08:08:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mccaulak-at-wfu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 25, 2004 at 07:15:27
---------------------------------------------------------------------------

Email: mccaulak-at-wfu.edu
Name: Anita McCauley

Organization: Wake Forest University

Title-Subject: [Microscopy] [Filtered] MListserver: capture board for an SEM

Question: I am looking to upgrade the image capture board for our Amray 1810 SEM. I am trying to find a board that will capture NTSC composite video at 640x480 pixels using TWAIN or WDM capture and is compatible with Windows XP. We have found a couple of possibilities: Flashpoint 4XL Lite, Flashbus Spectrum Lite framegrabber, Data Translation DT3120.

Any suggestions for boards that would work or any feedback regarding the boards I mentioned would be greatly appreciated.

Thanks

Anita K. McCauley, PhD
Director of Microscopy
Adjunct Asst. Professor
Biology Department
Wake Forest University
Winston-Salem, NC 27109

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From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 08:32:31 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tgardiner-at-mmtinc.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 25, 2004 at 08:21:13
---------------------------------------------------------------------------

Email: tgardiner-at-mmtinc.com
Name: Tammy

Title-Subject: [Microscopy] [Filtered] NiChrome etchant

Question: Does anyone know how to etch 80% Nickle 20% Chrome to see the microstructure.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 08:37:30 2004

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Focus on Microscopy 2004, Philadelphia, April 4-8

Dear Colleagues,

The draft program of the international conference Focus on Microscopy
2004 is now available,
please review under http://www.focusonmicroscopy.org .
Abstracts for the poster session may be still submitted, but may not
be included in the printed conference material.

Plenary speakers include:

S. Hell: Fluorescence nanoscopy through reversible optically
saturable transitions
Z. Galis: Exploring revascularization using fluorescence angiography:
going with the flow
S.M. Hewitt: Confocal imaging meets tissue microarrays: high
throughput biology moves to the next level
E. Manders, Controlled light exposure microscopy (clem): an effective
reduction of phototoxicity.
R.F. Murphy, R.F.: Automated interpretation of images for location proteomics
B. Parvin: Convergence of microscopy and imaging bioinformatics
A. Periasamy: Protein localization in cells and tissues: Flim-Fret microscopy
K. Pourezzaei:Application of nano optical tools to single cell imaging
A. Waggoner: Quantum dots for in-vivo imaging in mice
W. Zipfel: Applications of multiphoton microscopy and nonlinear excitation

Sessions are dedicated to the following topics:
Optical theory, multidimensional image processing, 3D/4D in-vivo imaging,
non-linear biological imaging, Raman/Cars microscopy, tuning the
microscope resolution,
image restoration, new instrumentation, high-througput microscopy and
human cytome project

Also included:
Pre-conference workshops, trade show, poster session

Looking forward seeing you in Philadelphia,

Andres Kriete, Philadelphia
Fred Brakenhoff, Amsterdam
--
+-----------------------------------------+
Prof. Dr. G.J. Brakenhoff
University of Amsterdam
Institute for Molecular Cell Biology
Section Molecular Cytology
Kruislaan 316
1098 SM Amsterdam, The Netherlands

Tel. : 31-20-5255189
Fax. : 31-20-5256271
Email: brakenhoff-at-science.uva.nl
+-----------------------------------------+

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 09:14:09 2004

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You can display as many colors as you like, with the caveat that you
won't be able to separate them again if they're mixed.

In our software (Image-Pro, using the Colro Composite) we allow
compositing as many colors as desired; red, green, blue, yellow, cyan,
magenta, etc. We do this by assigning each input a particular color mix
- an input image assigned to yellow contributes equally to red and
green, while orange contributes fully to red and only half as much to
green.

With three colors (RGB) you can separate them out from each other using
only the final 24-bit color composite. With multiple color mixing using
combinations of RGB you cannot. However, you can view these just fine as
long as the objects of different colors do not overlap (and mix) too
much. We even allow white, so that you can overlay DIC and fluorescence
images; this works quite well if you treat the 'white' input as a
background to the others.

-- Kevin Ryan
kryan-at-mediacy.com

Media Cybernetics, Inc.
www.mediacy.com

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Friday, February 20, 2004 17:08
To: phillipst-at-missouri.edu; Microscopy-at-msa.microscopy.com

Sorry, Tom, you can't do that. Human eyes have three kinds of cones, and

consequently computer displays have three kinds of phosphors. You can
generate a
wide range of color combinations with those three phosphors, and so
there is no
fourth color available that doesn't occur when the right proportions of
the
three are present. Now, if you were a pigeon, you'd have 5 kinds of
cones, and
you would have designed monitors with more phosphors, and been able to
handle
more independent signals at the same time.

John Russ
========
In a message dated 2/20/04 6:19:40 PM, phillipst-at-missouri.edu writes:

} I know how to make a composite DAPI, FITC, Rhodamine (i.e., Blue,
} Green,
}
} Red) color image by pasting the grey scale digital fluorescence images
} into the RGB channels but how do you get a 4th color (e.g., Far Red
} 647) into
}
} the image. I know there must be a simple way that my tired old mind is
}
} forgetting. Could some Photoshop maven help me out? Thanks, Tom

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 09:25:00 2004

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Dear list,

During the past month, I have been working on semithick sectioning. The
sections are around green-purple , which translates into thickness of
120-250 micron. To spread the wrinkles , I used Chloroform and it worked
fine. However, it made me very sick, shortness of breath. I am wondering
if any of you have better and safer methods to spread the thick sections.

Thank you,

Long

-----------------------------------------------
Miao, Long
Dept of Biological Science
334 Bio. Unit1
Florida State University
Tallahassee, FL32306-4370
email: lmiao-at-bio.fsu.edu
Voice: (850)644-9817
FAX : (850)644-0481
-----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 10:06:45 2004

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To all:

The March 8th meeting of the New England Society for Microscopy (NESM) will
be held at Worcester Polytechnic Institute (WPI), Worcester, MA. Three
speakers, two from the WPI faculty and one from UMASS will present a "Forum
on Nanotechnology".

Registration is from 5-6pm followed by a reception/dinner from 5:30-7pm.
The registration fee for this meeting is $25.00 (members and non-members
alike). Please visit NESM's website (MSA website-local societies) for
further details. Click on "current newsletter" for directions, a map, and
registration form. To register, print out the registration form, and send
completed form with money to Paul Bain, NESM Treasurer by March 5, 2004.

We hope many of you will attend this most informative meeting!

Peggy Sherwood
Corresponding Secretary, NESM

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 10:08:31 2004

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I bought a heat pen from Ted Pella (I have no financial interests in this
company). It was expensive ($300??) but a lot better than the small
battery operated units (~$40). I liked it so much, I bought two more for
my other ultramicrotomes. We use it on both thin and semi-thin. It is a
lot better and safer than chloroform (long term liver problems can result
from repeated inhalation). good luck

10:37 AM 2/25/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 10:15:39 2004

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You may try this at Acton Technologies, http://www.actontech.com/elec3.htm

Peter Tomic
Agere Systems

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:tgardiner-at-mmtinc.com]
Sent: Wednesday, February 25, 2004 9:46 AM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tgardiner-at-mmtinc.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 25, 2004 at 08:21:13
---------------------------------------------------------------------------

Email: tgardiner-at-mmtinc.com
Name: Tammy

Title-Subject: [Microscopy] [Filtered] NiChrome etchant

Question: Does anyone know how to etch 80% Nickle 20% Chrome to see the microstructure.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 10:19:24 2004

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Have you heard of a heat pen? Theycan be used to get rid of wrinkles. You hold it over the sections like you do the chloroform stick and the wrinkles should go away. I don't know which EM vendor has them, but it used to be tha all of the EM vendors sold them.

Good luck and please get some fresh air,

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax
} } } "Long Miao" {lmiao-at-bio.fsu.edu} 02/25/04 10:51 AM } } }

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Dear list,

During the past month, I have been working on semithick sectioning. The
sections are around green-purple , which translates into thickness of
120-250 micron. To spread the wrinkles , I used Chloroform and it worked
fine. However, it made me very sick, shortness of breath. I am wondering
if any of you have better and safer methods to spread the thick sections.

Thank you,

Long

-----------------------------------------------
Miao, Long
Dept of Biological Science
334 Bio. Unit1
Florida State University
Tallahassee, FL32306-4370
email: lmiao-at-bio.fsu.edu
Voice: (850)644-9817
FAX : (850)644-0481
-----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 10:21:53 2004

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We are having problems with our Hitachi S-570 and a service technician
is not available until the end of April. Perhaps someone has experienced
a similar problem and can give us some advice.

At low magnifications, everything appears to be okay (perhaps because
the irregularity is too small to see) but around 2500 X the entire image
on the CRT begins to wave. This waviness increases in size when the
magnification is increased. For instance, if a straight line is focused
on, a regular frequency wave appears to travel along the line. Magnify
this image and the wave also magnifies. The problem is accentuated when
moving from aperture 3 to aperture 2.

We don't believe any other equipment is causing an external
disturbance. We have changed the filament, cleaned the Wehnelt, anode,
and movable and fixed apertures. Any ideas on a possible solution?

Shannan

Shannan Little
Research Technician/Technicien de recherche
Electron Microscopy and Image Analysis /
Microscopie électronique et Analyse d'images
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 403-317-3446
Facsimile/Télécopieur: 403-382-3156
P.O. Box 3000 / CP 3000
Lethbridge, Alberta T1J 4B1
littlesm-at-em.agr.ca
http://res2.agr.ca/lethbridge/emia/index_e.htm

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 10:34:22 2004

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Long

stop using chloroform immediately. It's harmful and should have been risk assessed - not only is it an anaesthetic it is harmful over a prolonged exposure by inhalation and a category 3 carcinogen. We only use chloroform in the fume hood these days.

The safest method is to buy a heat pen - available at most e.m suppliers. This uses a hot tungsten wire to soften and spread your sections.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
UK

----- Original Message -----
} From: Long Miao {lmiao-at-bio.fsu.edu}

------------------------------------------------------------------------------
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Focus on Microscopy 2004, Philadelphia, April 4-8

Dear Colleagues,

The draft program of the international conference Focus on Microscopy
2004 is now available,
please review under http://www.focusonmicroscopy.org .
Abstracts for the poster session may be still submitted, but may not
be included in the printed conference material.

Plenary speakers include:

S. Hell: Fluorescence nanoscopy through reversible optically
saturable transitions
Z. Galis: Exploring revascularization using fluorescence angiography:
going with the flow
S.M. Hewitt: Confocal imaging meets tissue microarrays: high
throughput biology moves to the next level
E. Manders, Controlled light exposure microscopy (clem): an effective
reduction of phototoxicity.
R.F. Murphy, R.F.: Automated interpretation of images for location proteomics
B. Parvin: Convergence of microscopy and imaging bioinformatics
A. Periasamy: Protein localization in cells and tissues: Flim-Fret microscopy
K. Pourezzaei:Application of nano optical tools to single cell imaging
A. Waggoner: Quantum dots for in-vivo imaging in mice
W. Zipfel: Applications of multiphoton microscopy and nonlinear excitation

Sessions are dedicated to the following topics:
Optical theory, multidimensional image processing, 3D/4D in-vivo imaging,
non-linear biological imaging, Raman/Cars microscopy, tuning the
microscope resolution,
image restoration, new instrumentation, high-througput microscopy and
human cytome project

Also included:
Pre-conference workshops, trade show, poster session

Looking forward seeing you in Philadelphia,

Andres Kriete, Philadelphia
Fred Brakenhoff, Amsterdam
--
+-----------------------------------------+
Prof. Dr. G.J. Brakenhoff
University of Amsterdam
Institute for Molecular Cell Biology
Section Molecular Cytology
Kruislaan 316
1098 SM Amsterdam, The Netherlands

Tel. : 31-20-5255189
Fax. : 31-20-5256271
Email: brakenhoff-at-science.uva.nl
+-----------------------------------------+

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 11:38:50 2004

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The solutions for immersion etching are typically a
mixture of high concentrations of strong acids which
can be nasty to use and don't store well.

Electrolytic etching is the preferred method. Start
with 2% H2SO4 in water, 3-10 V dc, 5-15 secs with Pt
lead wires. The sufuric acid concentration may be
increased up to 20% for a deeper etch.

Stu Smalinskas
Metallurgist
SKF NATC
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Tammy wrote:

Question: Does anyone know how to etch 80% Nickle 20%
Chrome to see the microstructure.

Email: tgardiner-at-mmtinc.com
Name: Tammy

__________________________________
Do you Yahoo!?
Yahoo! Finance: Get your refund fast by filing online.
http://taxes.yahoo.com/filing.html

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 11:39:44 2004

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Instead of a $300 heat pen how about a soldering iron/gun?

Geoff

Tom Phillips wrote:

} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} I bought a heat pen from Ted Pella (I have no financial interests in
} this company). It was expensive ($300??) but a lot better than the
} small battery operated units (~$40). I liked it so much, I bought two
} more for my other ultramicrotomes. We use it on both thin and
} semi-thin. It is a lot better and safer than chloroform (long term
} liver problems can result from repeated inhalation). good luck
}
}
} 10:37 AM 2/25/2004 -0500, you wrote:
}
}
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } Dear list,
} }
} } During the past month, I have been working on semithick sectioning. The
} } sections are around green-purple , which translates into thickness of
} } 120-250 micron. To spread the wrinkles , I used Chloroform and it
} } worked
} } fine. However, it made me very sick, shortness of breath. I am
} } wondering
} } if any of you have better and safer methods to spread the thick
} } sections.
} }
} } Thank you,
} }
} } Long
} }
} }
} } -----------------------------------------------
} } Miao, Long
} } Dept of Biological Science
} } 334 Bio. Unit1
} } Florida State University
} } Tallahassee, FL32306-4370
} } email: lmiao-at-bio.fsu.edu
} } Voice: (850)644-9817
} } FAX : (850)644-0481
} } -----------------------------------------------
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 11:58:55 2004

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Dear Shannon,
I have two S-570s and the problem you see is almost certainly a magnetic field
affecting the image. Does it translate to 60-cycle from the mains? Does the
problem go away at higher magnifications, when the relays in the back "click"? I
have seen this when the microscope was a bit too close to a circuit-breaker box
or when there was a big instrument that drew a lot of current was "downstream"
on the same electrical feed as the SEM or the SEM was too close to the power
lines in the room.
On the microscope, there are two relays that control magnification at the
back-right corner. You can hear them click when you go up and down in mag. You
can get two more and replace them, if that is the problem. The other thing that
could cause the ripple is a ripple in one of the power supplies. An electronics
technician could put an oscilloscope on the various test points and see if that
is the problem.
Waves and ripples on the image are usually mechanical vibration or mag field,
but yours seems too severe to be vibration.
Good luck,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Shannan Little" {littlesm-at-agr.gc.ca}
To: {Microscopy-at-sparc5.microscopy.com}
Cc: "Byron Lee" {lee-at-agr.gc.ca}
Sent: Wednesday, February 25, 2004 8:34 AM

We are having problems with our Hitachi S-570 and a service technician
is not available until the end of April. Perhaps someone has experienced
a similar problem and can give us some advice.

At low magnifications, everything appears to be okay (perhaps because
the irregularity is too small to see) but around 2500 X the entire image
on the CRT begins to wave. This waviness increases in size when the
magnification is increased. For instance, if a straight line is focused
on, a regular frequency wave appears to travel along the line. Magnify
this image and the wave also magnifies. The problem is accentuated when
moving from aperture 3 to aperture 2.

We don't believe any other equipment is causing an external
disturbance. We have changed the filament, cleaned the Wehnelt, anode,
and movable and fixed apertures. Any ideas on a possible solution?

Shannan

Shannan Little
Research Technician/Technicien de recherche
Electron Microscopy and Image Analysis /
Microscopie électronique et Analyse d'images
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 403-317-3446
Facsimile/Télécopieur: 403-382-3156
P.O. Box 3000 / CP 3000
Lethbridge, Alberta T1J 4B1
littlesm-at-em.agr.ca
http://res2.agr.ca/lethbridge/emia/index_e.htm

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 12:27:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tgardiner-at-mmtinc.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 25, 2004 at 08:21:13
---------------------------------------------------------------------------

Email: tgardiner-at-mmtinc.com
Name: Tammy

Title-Subject: [Microscopy] [Filtered] NiChrome etchant

Question: Does anyone know how to etch 80% Nickle 20% Chrome to see the microstructure.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 13:03:22 2004

Contents Retrieved from Microscopy Listserver Archives
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Shannan, I believe you have a classic case of the
"jiggies". This phenomenon presents itself when you
image a sample that is held loose in the SEM. The
part must be clamped firmly to the base to get rid of
the jiggies. This issue was addressed in a recent
issue of "Microscopy Today".

Stu Smalinskas, P.E.
Metallurgist
SKF NATC
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Shannan wrote:

We are having problems with our Hitachi S-570 and a
service technician is not available until the end of
April. Perhaps someone has experienced a similar
problem and can give us some advice.

At low magnifications, everything appears to be okay
(perhaps because the irregularity is too small to see)
but around 2500 X the entire image on the CRT begins
to wave. This waviness increases in size when the
magnification is increased. For instance, if a
straight line is focused on, a regular frequency wave
appears to travel along the line. Magnify this image
and the wave also magnifies. The problem is
accentuated when moving from aperture 3 to aperture 2.

We don't believe any other equipment is causing an
external disturbance. We have changed the filament,
cleaned the Wehnelt, anode, and movable and fixed
apertures. Any ideas on a possible solution?

Shannan

Shannan Little
Research Technician/Technicien de recherche
Electron Microscopy and Image Analysis /
Microscopie électronique et Analyse d'images
Agriculture and Agri-Food Canada/Agriculture et
Agroalimentaire Canada
Telephone/Téléphone: 403-317-3446
Facsimile/Télécopieur: 403-382-3156
P.O. Box 3000 / CP 3000
Lethbridge, Alberta T1J 4B1
littlesm-at-em.agr.ca
http://res2.agr.ca/lethbridge/emia/index_e.htm

__________________________________
Do you Yahoo!?
Yahoo! Mail SpamGuard - Read only the mail you want.
http://antispam.yahoo.com/tools

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 14:00:37 2004

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The third International CryoEM Course

so you think you want to try cryo-em but you are not sure which
procedure will work best for you
or
you have tried high pressure freezing or the Tokuyasu method but the
results didn't come up to expectations.

this is the course for you. Expert help with lots of experience with
a multitude of specimens

When: June 8 -June 17, 2004

Where: University of British Columbia, Vancouver, Canada

Main Topics: High Pressure Freezing, Freeze Substitution, Cryo
Ultramicrotomy, Tokuyasu Method, Plunge Freezing, Cryo TEM, Cryo SEM,
Immunolabelling, Nonogold gold enhancement and fluronanogold gold
enhancement

Core Faculty include Kent McDonald (UC Berkekley), Stan Erlandsen (U
Minnesota), George Postuma (U Utrecht, Netherlands), Doug Keene
(Shriner's Hospital, Portland) Lacey Samuels (UBC), Gethin Owen
(UBC), Elaine Humphrey (UBC).

Vendors include: Diatome, Emitech, Hitachi, Leica, Nonoprobes,
Quantifoil, Technotrade

For an application form see the website http://emlab.ubc.ca and click
on Third International CryoEM Course

This year we will be using nanogold labelling with gold enhancement
(not silver).

This course allows you to follow (with hands-on) the procedure all
the way through from freezing to presentation of results.

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 14:10:54 2004

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I suppose a response is not absolutely required, but you catch me in one of
those moods.

I had a discussion with a chemist friend years ago about chloroform and its
hazards. He strongly made the point that chloroform itself was not so bad
as a lot of the paperwork made it out to be. The hitch was that chloroform
is often not pure but contaminated with low levels of carbon tetrachloride,
a powerful carcinogen. It seemed that chloroform took the rap and has been
unable to acquit its name.

Now that is not to say that I am in favor of inhaling chloroform or
anything else unnecessarily. (It is definitely affecting Long). We should
be very careful to avoid becoming complacent and careless around the
chemicals we work with. I just don't like to see the dangers of the
chemicals exaggerated. It is a "boy crying wolf" scenario to me. I can get
used to discounting the dangers for the chemicals I am familiar with and
start discounting the dangers for those chemicals I am not so familiar with.

I suppose I was "poisoned" to such warnings when I read the MSDS for a
one-pound bottle of pure calcium carbonate. It allowed for disposal of the
material in "an approved chemical waste landfill". I suppose I should have
bought mine at the health food store or just scraped some off of the gravel
drive out back. That way I could just through the excess away when I was done.

Warren

At 10:47 AM 2/25/2004, you wrote:

} Long
}
} stop using chloroform immediately. It's harmful and should have been risk
} assessed - not only is it an anaesthetic it is harmful over a prolonged
} exposure by inhalation and a category 3 carcinogen. We only use chloroform
} in the fume hood these days.
}
} The safest method is to buy a heat pen - available at most e.m suppliers.
} This uses a hot tungsten wire to soften and spread your sections.
}
} Malcolm
}
} Malcolm Haswell
} e.m. unit
} School of Health, Natural and Social Sciences
} Fleming Building
} University of Sunderland
} Tyne & Wear
} UK
}
} ----- Original Message -----
} } From: Long Miao {lmiao-at-bio.fsu.edu}
} Date: Wednesday, February 25, 2004 3:37 pm
} Subject: [Microscopy] semi-thick sections wrinkles spreading?
} }
} } Dear list,
} }
} } During the past month, I have been working on semithick
} } sectioning. The
} } sections are around green-purple , which translates into thickness of
} } 120-250 micron. To spread the wrinkles , I used Chloroform and it
} } workedfine. However, it made me very sick, shortness of breath.
} } I am wondering
} } if any of you have better and safer methods to spread the thick
} } sections.
} } Thank you,
} }
} } Long
} }
} }
} } -----------------------------------------------
} } Miao, Long
} } Dept of Biological Science
} } 334 Bio. Unit1
} } Florida State University
} } Tallahassee, FL32306-4370
} } email: lmiao-at-bio.fsu.edu
} } Voice: (850)644-9817
} } FAX : (850)644-0481
} } -----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 14:32:18 2004

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Kestutis writes ...

} Shannan, I believe you have a classic case of the
} "jiggies". This phenomenon presents itself when you
} image a sample that is held loose in the SEM. The
} part must be clamped firmly to the base to get rid of
} the jiggies. This issue was addressed in a recent
} issue of "Microscopy Today".

There is a possibility the problem could be electromagnetic interference.
If the "jiggies" are mimimized for higher acceleration voltages, then it's
likely this type of interference. Otherwise, look for something like an
un-dampened vacuum pump hose.

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

} Shannan wrote:
}
} We are having problems with our Hitachi S-570 and a
} service technician is not available until the end of
} April. Perhaps someone has experienced a similar
} problem and can give us some advice.
}
} At low magnifications, everything appears to be okay
} (perhaps because the irregularity is too small to see)
} but around 2500 X the entire image on the CRT begins
} to wave. This waviness increases in size when the
} magnification is increased. For instance, if a
} straight line is focused on, a regular frequency wave
} appears to travel along the line. Magnify this image
} and the wave also magnifies. The problem is
} accentuated when moving from aperture 3 to aperture 2.
}
}
} We don't believe any other equipment is causing an
} external disturbance. We have changed the filament,
} cleaned the Wehnelt, anode, and movable and fixed
} apertures. Any ideas on a possible solution?
}
} Shannan
}
} Shannan Little
} Research Technician/Technicien de recherche
} Electron Microscopy and Image Analysis /
} Microscopie ilectronique et Analyse d'images
} Agriculture and Agri-Food Canada/Agriculture et
} Agroalimentaire Canada
} Telephone/Tiliphone: 403-317-3446
} Facsimile/Tilicopieur: 403-382-3156
} P.O. Box 3000 / CP 3000
} Lethbridge, Alberta T1J 4B1
} littlesm-at-em.agr.ca
} http://res2.agr.ca/lethbridge/emia/index_e.htm
}
} __________________________________
} Do you Yahoo!?
} Yahoo! Mail SpamGuard - Read only the mail you want.
} http://antispam.yahoo.com/tools
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 14:58:30 2004

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Try Epon 812 (or whatever substitute you prefer) 40g, DDSA 10g, NMA 20g. If
you have a rotator (the over-and-over type, not the circular motion type)
available, that helps, and you should extend your infiltration times
considerably. Add at least one extra change into freshly-made Epon mix plus
DMP30 (2%) and if possible leave it in the last change in the fridge under
vacuum overnight, before embedding in yet more Epon mix plus DMP30. After
embedding, leave it in a vacuum oven at 37 C for 48 hours then an ordinary
oven at 60 C for 7 days. This is my protocol for embedding blocks that are
not only bone but also very large - you might not need to be quite so
extreme for your material.

Lesley Weston.

on 24/02/2004 1:25 PM, Dusevich, Vladimir at DusevichV-at-umkc.edu wrote:

}
}
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--} -
}
} Hi,
}
} What is a good embedding media for bone ultramicrotomy?
} I use Epon 812 and Spurr resin, but penetration is not really
} good enough.
}
} Thanks,
}
} Vladimir M. Dusevich, Ph.D.
} Electron Microscope Lab Manager
} 3127 School of Dentistry
} 650 E. 25th Street
} Kansas City, MO 64108-2784
}
} Phone: (816) 235-2072
} Fax: (816) 235-5524
} Web: http://www.umkc.edu/dentistry/microscopy
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 15:01:08 2004

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Shannan,

It's always difficult to make any educated guesses about things like
this without seeing the images. However the one thing that puzzles me is
that it would be affected by a change in aperture size. If that's true I
can only think of two possibilities. First, you may have some charging
in your column or your sample and when you change the aperture you are
changing the beam current and therefore changing the charge/discharge
rate of whatever is charging. I'm not familiar with the Hitachi s-570
but if the aperture is heated, the second possibility is ripple from the
heater supply. I know the old JEOL-35 had a heated aperture and ripple
from the heater supply was a common problem.

Good Luck,
Bill

Shannan Little wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 15:05:40 2004

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Heat pens are good (Ted Pella sells them), but you might be able to remove
wrinkles by using a small wire loop to transfer the thick sections to a drop
of filtered de-ionised water on a slide, then leaving the slide on a
hot-plate set at about 60 C until the water is gone. Either method is much
safer than chloroform.

Lesley Weston.

on 25/02/2004 8:19 AM, Paula Sicurello at patpxs-at-gwumc.edu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
----------------------------------------------------------------------------
--} -
}
} Have you heard of a heat pen? Theycan be used to get rid of wrinkles. You
} hold it over the sections like you do the chloroform stick and the wrinkles
} should go away. I don't know which EM vendor has them, but it used to be tha
} all of the EM vendors sold them.
}
} Good luck and please get some fresh air,
}
} Paula :-)
}
} Paula Sicurello
} George Washington Univ. Medical Center
} Electron Microscope Lab
} Washington, DC 20037
} 202-994-2930 phone
} 202-994-2518 fax
} } } } "Long Miao" {lmiao-at-bio.fsu.edu} 02/25/04 10:51 AM } } }
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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--} -
}
} Dear list,
}
} During the past month, I have been working on semithick sectioning. The
} sections are around green-purple , which translates into thickness of
} 120-250 micron. To spread the wrinkles , I used Chloroform and it worked
} fine. However, it made me very sick, shortness of breath. I am wondering
} if any of you have better and safer methods to spread the thick sections.
}
} Thank you,
}
} Long
}
}
} -----------------------------------------------
} Miao, Long
} Dept of Biological Science
} 334 Bio. Unit1
} Florida State University
} Tallahassee, FL32306-4370
} email: lmiao-at-bio.fsu.edu
} Voice: (850)644-9817
} FAX : (850)644-0481
} -----------------------------------------------
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 15:38:28 2004

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You can try

10 mL HCl, 5 mL HNO3, 20 mL glicerol,
immerce in freshly prepared etchant for 1-5 min.

or

20 mL HNO3, 30 mL Acetic acid,
immerce in freshly prepared etchant for 5-60 sec.
I could be useful to heat etchant to 50 degrees Celsius.

Vladimir

}
} Email: tgardiner-at-mmtinc.com
} Name: Tammy
}
} Title-Subject: [Microscopy] [Filtered] NiChrome etchant
}
} Question: Does anyone know how to etch 80% Nickle 20% Chrome
} to see the microstructure.
}
} --------------------------------------------------------------
} -------------
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 15:52:37 2004

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Is it possible that these waves are due to a hard settling of the
chamber/column floatation system???

--
***************************************************************
Do not publicly post any of my correspondence without permission

Dee Breger
Mgr. SEM/EDX Facility
Lamont-Doherty Earth Observatory
61 Route 9W
Palisades, NY 10964 USA
T: 845/365-8640
F: 845/365-8155

http://www.ldeo.columbia.edu/micro
Journeys in Microspace (Columbia University Press, 1995)
http://www.lsc.org/antarctica/front.html

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 15:57:16 2004

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Greeting listers:

I had asked about microprobes late last year
and got several leads on probes. I was
following the Kleindiek MM3A probes but found
that they will only work up to 100C. I need
in-SEM probes that will work up to about 175C.
They need to be able to handle about 10mA DC
and be positionable to roughly 0.5u.

Any other ideas?

thanks,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 16:18:51 2004

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Gary,

We had some interaction with people at Zyvex (www.zyvex.com) regarding their MEMS based tools. You might want to contact them with your questions.

I also have this contact info for Peter Overland
Zyvex Corporation
Tel. 972-235-7881 ext 249
or ask for Phil Foster (Southwest rep)

Disclaimer: I have no financial interest in the company.

Jerzy

******************************************************
Jerzy Gazda, Ph.D. Advanced Micro Devices
Supervising Engineer 5204 E. Ben White Blvd. - MS 512
PCAL - AIM Section Austin, TX 78741
TEL: 1-800-538-8450, Ext. 51453
jerzy.gazda-at-amd.com
******************************************************

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Wednesday, February 25, 2004 4:11 PM
To: MSA listserver

Greeting listers:

I had asked about microprobes late last year
and got several leads on probes. I was
following the Kleindiek MM3A probes but found
that they will only work up to 100C. I need
in-SEM probes that will work up to about 175C.
They need to be able to handle about 10mA DC
and be positionable to roughly 0.5u.

Any other ideas?

thanks,
gary g.

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 16:18:11 2004

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Shannan,

We have a S-570 ourselves.
Some questions:
What kVs are you using? Does the problem get worse at a lower kV? The
570's column could be better shielded, and they're sensitive to EMF
variations at 5kV and less. Just moving in a chair when one is within
3 feet of the column will move the image. So an EMF field from
lights, computers and computer monitors can cause this. You can get
a Gauss meter fairly cheaply, and it's worthwhile having one to check
for fields. I moved the computer to 6' from the column, and that
helped with a problem we had.
Does the problem lessen or go away with slower scan speeds? Another
indication of EMF problems.

What working distance? Does the problem get worse at a longer WD? If
yes, this indicates mechanical vibrations.
One thing to check on the 570 is the "shock absorbers" on which the
column rests. In each corner, just below the console. If the rubber
accordion sleeves are cracked, they're no good. You should be able to
get new ones from Hitachi -- supposedly much cheaper from Hitachi
Canada than Hitachi US. Our service engineers tell me to fill a bad
mount with silicone chaulk. Layer in a bunch, let it set, layer in
more, let it set, repeat until the mount is full. This does seem to
work, and it's cheaper than buyng mounts. But, if you have a service
contract, this should pay for new mounts (maybe).

Did things change at all when you cleaned the apertures, etc.? If
yes, they may just need recleaning, especially if you used EtOH or
acetone as your final cleaning steps. Even absolute EtOH an 100%
acetone leave residues. The final rinse should be in the best water
you can get, then oven dry. The column may also need cleaning, not
just the apertures.

Do you have a Faraday cup? If yes, does the current vary at the same
frequency as the image waves? Does the emission current vary? If yes
to either, you may have gun problems.

Do you get bright flashes when using the stage rotation control? If
yes, then the stage is likely not grounded properly. The wire that
grounds the stage specimen mount could be better placed, and can get
worn or broken. Our wire wore through under one on the mounts (the
little "U" bracket), so that it shorted to the stage, which it's not
supposed to do. Bad grounding can cause the waviness you're seeing.
Take an ohmmeter to the capped plug (the cap is on, right?) on the
left side of the stage door. There should be no resistance from the
center pin to the specimen holder mount, but there should be an
"open" between the holder mount and the stage itself (try the flat
plate immediately to the right of the holder mount).

Phil

} We are having problems with our Hitachi S-570 and a service technician
} is not available until the end of April. Perhaps someone has experienced
} a similar problem and can give us some advice.
}
} At low magnifications, everything appears to be okay (perhaps because
} the irregularity is too small to see) but around 2500 X the entire image
} on the CRT begins to wave. This waviness increases in size when the
} magnification is increased. For instance, if a straight line is focused
} on, a regular frequency wave appears to travel along the line. Magnify
} this image and the wave also magnifies. The problem is accentuated when
} moving from aperture 3 to aperture 2.
}
} We don't believe any other equipment is causing an external
} disturbance. We have changed the filament, cleaned the Wehnelt, anode,
} and movable and fixed apertures. Any ideas on a possible solution?
}
} Shannan
}
} Shannan Little
} Research Technician/Technicien de recherche
} Electron Microscopy and Image Analysis /
} Microscopie électronique et Analyse d'images
} Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
} Telephone/Téléphone: 403-317-3446
} Facsimile/Télécopieur: 403-382-3156
} P.O. Box 3000 / CP 3000
} Lethbridge, Alberta T1J 4B1
} littlesm-at-em.agr.ca
} http://res2.agr.ca/lethbridge/emia/index_e.htm

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 17:43:22 2004

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By coincidence, someone just walked in with a copy of Microscopy Today
September/October 2003 which contains a Microscopy 101 article on zigzag
edges in SEM micrographs. I've had jaggies from 60Hz interference, from
vibration and, less intuitively, when a component of the stage was loose.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 17:46:11 2004

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Geoff,
The PELCO Heat Pen has a nichrome element that becomes incandescent during
use. A red hot tip like our Heat Pen has gives off a large amount of radiant
heat. This results in more efficient heating of the sample at a safer
distance. A hot tip that is not glowing red would have to be brought close
enough to the sample to heat it by air convection/conduction which would
take longer and put the sample at risk. Some other advantages are: Variable
element power (heat), quick response time of element temperature when
setting is changed, the level of the heat is visually indicated by a 10
color LED bar and a lightweight easily manipulated heating element wand.

Disclaimer: I work for Ted Pella, Inc which is the company that manufactures
the PELCO Heat Pen.

Regards,
Mark Armogida
VP Production and Engineering
Ted Pella, Inc.

Phone: 530-243-2200 ext. 212
Fax: 530-243-3761

mark_armogida-at-tedpella.com
www.tedpella.com

-----Original Message-----
} From: Geoff McAuliffe [mailto:mcauliff-at-umdnj.edu]
Sent: Wednesday, February 25, 2004 12:53 PM
To: Tom Phillips
Cc: Long Miao; Microscopy-at-msa.microscopy.com

Instead of a $300 heat pen how about a soldering iron/gun?

Geoff

Tom Phillips wrote:

} --------------------------------------------------------------------------
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} --------------------------------------------------------------------------
-----
}
}
} I bought a heat pen from Ted Pella (I have no financial interests in
} this company). It was expensive ($300??) but a lot better than the
} small battery operated units (~$40). I liked it so much, I bought two
} more for my other ultramicrotomes. We use it on both thin and
} semi-thin. It is a lot better and safer than chloroform (long term
} liver problems can result from repeated inhalation). good luck
}
}
} 10:37 AM 2/25/2004 -0500, you wrote:
}
}
} } -------------------------------------------------------------------------
-----
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
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} } -------------------------------------------------------------------------
------
} }
} }
} } Dear list,
} }
} } During the past month, I have been working on semithick sectioning. The
} } sections are around green-purple , which translates into thickness of
} } 120-250 micron. To spread the wrinkles , I used Chloroform and it
} } worked
} } fine. However, it made me very sick, shortness of breath. I am
} } wondering
} } if any of you have better and safer methods to spread the thick
} } sections.
} }
} } Thank you,
} }
} } Long
} }
} }
} } -----------------------------------------------
} } Miao, Long
} } Dept of Biological Science
} } 334 Bio. Unit1
} } Florida State University
} } Tallahassee, FL32306-4370
} } email: lmiao-at-bio.fsu.edu
} } Voice: (850)644-9817
} } FAX : (850)644-0481
} } -----------------------------------------------
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 17:45:58 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jennibean73-at-yahoo.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Wednesday, February 25, 2004 at 12:39:09
---------------------------------------------------------------------------

Email: jennibean73-at-yahoo.com
Name: Jen

Organization: N/A

Education: Graduate College

Location: City, State, Country

Question: I am counting bacteria at 1000X magnification. How would one calculate an approximation of bacterial counts in the entire sample?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 17:51:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ldemp-at-mse.ufl.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 25, 2004 at 13:25:21
---------------------------------------------------------------------------

Email: ldemp-at-mse.ufl.edu
Name: Luisa Amelia Dempere

Organization: University of Florida

Title-Subject: [Microscopy] [Filtered] MListserver: FSM,FLAVS,FLACerS 2004 Joint Symposium

Question:

Florida Society for Microscopy (FSM), Florida Chapter of the AVS Science and Technology Society (Fl AVS), Florida Section of the American Ceramic Society (Fl ACerS)
2004 Annual Joint Symposium
March 8-9, 2004, University of Central Florida Student Union, Orlando, Florida
Web: www.flavs.org
This is a reminder that the Program for the FL AVS, FSM and Fl-ACerS 2004 Annual Joint Symposium, being held March 8-9, 2004, at UCF, in Orlando, Fl, is available online. Technical Sessions include: Thin Films, Electronic Materials, Microscopy in the Physical and Biological Sciences, FIB Investigations of Mechanical Damage, Ceramic Coatings, MicroElectroMechanicalSystems (MEMS), Biomaterial Interfaces, Nanoscience, and Nanotechnology. Please visit our website at www.flavs.org for the program schedule and additional information on the symposium.
There is no registration fee to attend the symposium, reception, or equipment exhibit. On-line registration is suggested at http://www.flavs.org/RegForm.htm
The Equipment Exhibit will be held on Monday and Tuesday, March 8-9, 2004, in the UCF Student Union Pegasus Ballroom, in conjunction with the poster session, reception and coffee breaks. The exhibit will be opened from 11 am to 7 pm on Monday, and from 10 am to 3 pm on Tuesday.
On-line vendor registration is available at http://www.flavs.org/vendorregform.htm. For more information on the exhibit or to be an exhibitor, please refer to http://www.flavs.org/Equipment.htm.
Two AVS Short Course

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From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 18:28:51 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (info-at-klughammer.de) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, February 23, 2004 at 23:41:32
---------------------------------------------------------------------------

Email: info-at-klughammer.de
Name: Anneliese Schmaus

Organization: klughammer gmbh

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello,

I am looking for a glass slide which is covered by a flouerscent material. I need it for calibration purposes. Does anybody know where to get it or how to make it. I already used a text marker. This works but it was too week and very irregular.

Anneliese Schmaus

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 18:38:03 2004

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Dear Colleagues:

You are invited to participate to a Workshop on Advanced Techniques in Scanning Electron Microscopy & Microanalysis for materials Characterization. That workshop will be held from May 17 to 21, 2004 at McGill University, Montreal, Canada.

Attention: Registration deadline is April 15th 2004

Enjoy Montreal Joie de Vivre and top technical expertise from world class renomed instructors

The instructors are:

David C. Joy, University of Tennessee and Oak Ridge National Laboratory, USA

Eric Lifshin, State University of New York at Albany, USA

Raynald Gauvin, McGill University, Canada

Pierre Hovington, Hydro-Québec Research Center, Canada

Marin Lagacé, Hydro-Québec Research Center, Canada

For more information:

http://www.mcgill.ca/minmet/ebeamworkshop/

Very best regards

Raynald GAUVIN
************************************************************
Professor Raynald Gauvin
Department Mining, Metals and Materials Engineering
McGill University
M.H. Wong Building
3610 University Street
Montreal, H3A 2B2
Canada
Tel: (514) 398-8951
FAX: (514) 398-4492
http://www.minmet.mcgill.ca
EMAIL:Raynald.Gauvin-at-McGill.ca
************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 18:42:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donaldawbrey-at-texashealth.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, February 25, 2004 at 18:34:32
---------------------------------------------------------------------------

Email: donaldawbrey-at-texashealth.org
Name: Donald G. Awbrey

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] Image Analysis Salary

Question: Howdy fellow microscopists,

I know I've ask this question before, but I received a limited response. So here goes again.

Does any one in MSA land know of any salary survey for Image Analysis Technicians? Is there any information on median ranges of salaries/wages for IA?

Any information will be appreciated. If you are an Image Analysis Technician, or eguivilent, please contact me regarding this issue.

I thank everyone in advance....

Donald G. Awbrey HT(ASCP) QIHC
donaldawbrey-at-texashealth.org

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 19:06:40 2004

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Dear Anneliese,

We have a set of fluorescence calibration slides available that might suit your needs. Please visit www.MicroscopyEducation.com and look for FluorRef(TM).

Good hunting,
Barbara Foster
Microscopy/Microscopy Education, Inc. (MME, Inc.)
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Optimizing Light Microscopy is still available through MME. For information on ordering single or small quantities, visit our website. For discounts on classroom-sized, call us today.
^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&

At 06:42 PM 2/25/04 -0600, Klughammer - Anneliese Schmaus (by way of wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Feb 25 23:37:52 2004

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Luc Harmsen
ANASPEC South Africa

www.anaspec.co.za
Hi all
I have seen a few queries around the possibility of fields affecting a
system.
Can I point you to the RS Electronics website where you can buy a magnetic
field tester which will allow you to find hese fields very quickly and
easily.

If you ask your local RS Electronics store about it I am sure they can help.

The RS Electronics description and part number are:

ELF Magnetic 212-837 Price is Ł140.00

http://rswww.com/

and for the USA http://www.rselectronics.com
Good luck

Tel: +27 11 794 8340
Fax: +27 11 794 8349
P.O. Box 2561
Honeydew 2040
Gauteng, South Africa

-----Original Message-----
} From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
Sent: 25 February 2004 08:10
To: Shannan Little
Cc: Microscopy

Dear Shannon,
I have two S-570s and the problem you see is almost certainly a magnetic
field
affecting the image. Does it translate to 60-cycle from the mains? Does the
problem go away at higher magnifications, when the relays in the back
"click"? I
have seen this when the microscope was a bit too close to a circuit-breaker
box
or when there was a big instrument that drew a lot of current was
"downstream"
on the same electrical feed as the SEM or the SEM was too close to the power
lines in the room.
On the microscope, there are two relays that control magnification at the
back-right corner. You can hear them click when you go up and down in mag.
You
can get two more and replace them, if that is the problem. The other thing
that
could cause the ripple is a ripple in one of the power supplies. An
electronics
technician could put an oscilloscope on the various test points and see if
that
is the problem.
Waves and ripples on the image are usually mechanical vibration or mag
field,
but yours seems too severe to be vibration.
Good luck,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Shannan Little" {littlesm-at-agr.gc.ca}
To: {Microscopy-at-sparc5.microscopy.com}
Cc: "Byron Lee" {lee-at-agr.gc.ca}
Sent: Wednesday, February 25, 2004 8:34 AM

We are having problems with our Hitachi S-570 and a service technician
is not available until the end of April. Perhaps someone has experienced
a similar problem and can give us some advice.

At low magnifications, everything appears to be okay (perhaps because
the irregularity is too small to see) but around 2500 X the entire image
on the CRT begins to wave. This waviness increases in size when the
magnification is increased. For instance, if a straight line is focused
on, a regular frequency wave appears to travel along the line. Magnify
this image and the wave also magnifies. The problem is accentuated when
moving from aperture 3 to aperture 2.

We don't believe any other equipment is causing an external
disturbance. We have changed the filament, cleaned the Wehnelt, anode,
and movable and fixed apertures. Any ideas on a possible solution?

Shannan

Shannan Little
Research Technician/Technicien de recherche
Electron Microscopy and Image Analysis /
Microscopie électronique et Analyse d'images
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 403-317-3446
Facsimile/Télécopieur: 403-382-3156
P.O. Box 3000 / CP 3000
Lethbridge, Alberta T1J 4B1
littlesm-at-em.agr.ca
http://res2.agr.ca/lethbridge/emia/index_e.htm

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 03:04:22 2004

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I have been considering purchase of one of the wood burning
(pyrography) stations supplied by craft shops. Axminster Power
Tool Centre (www.axminster.co.uk) offer model ST-141 (20W,
constant 1V, 2 wire loop tips with fixed temp of 650oC) for Ł49.95
inc. VAT. Order code 014100, or model ST-171 (30W, variable 0.5-
1.6V, 3 wire tips, variable temp of 450-750oC) for Ł69.95 inc. VAT.
Order code 017100. The latter is obviously more controllable. Do
you think these would work for section flattening? The alternative is
5 to 10 times the price for the specialist kit from the EM suppliers,
but are they any better for the job?

Chris

==========================================
Dr. Chris Jeffree
University of Edinburgh
BIOSEM - Biological Sciences Electron Microscope Facility
Institute of Cell and Molecular Biology
Daniel Rutherford Building
King's Buildings, Mayfield Road
EDINBURGH, EH9 3JH, Scotland, UK
Tel. #44 (0) 131 650 5554
FAX. #44 (0) 131 650 5392
Mobile 07710 585 401
email c.jeffree-at-ed.ac.uk
=========================================

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 09:00:54 2004

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Colleagues

I am starting to get daily questions about rejected Email. I understand your frustration
however, please remember this is a necessary evil to insure that spam does not
overwhelm the listserver.

Although the details below have been said and posted many times, I am having to
individually explain this many times each week, and to be honest it is getting
to be a chore.

Please bear with me for a few minutes and take a moment to carefully read this message.

Let me paraphrase the most common complaint.

"Nestor --- why is my message being rejected I am/have been a subscriber for many years/months etc.......
please fix my problem."

95+% of the problems are due to either one or both of the following issues, which
are documented in the "rejection message". You have the ability to fix the
problem on your own with only a modicum of effort.

If you get a rejection message please take a moment and first READ the whole
message and see if you fall into one of the two classifications below.

If you do not fall within one of these two categories then by all means
contact me, but I would really appreciate your checking
first as it will save both of us time and effort.

In the body of the rejection message there is ALWAYS a reason documented.

It is preceeded by the following text

} --------------------------------------------------------
}
} Your mail has been rejected for the following reason(s):
}
} --------------------------------------------------------

Scroll down a few lines. You will find the reason documented. Here are
the 2 most common reasons.

#1) } Content-Type: multipart/alternative
} An Email Attachment was detected with your message!!!

This rejection message means you have an attachment in your Email.
Remember the Listserver automatically rejects
any Email having attachments. There are NO EXCEPTIONS.

Please realize that it may be a HIDDEN attachment. A number of you have
set your Email program to send formatted texted. MS Outlook and related
Email clients send this type of text as a HTML attachment in your Email this
is general done without your knowledge.

You must send your Email as PLAIN/ASCII text. Go to your Preferences
and change your Email client to send only PLAIN text. This should cure this
problem.

#2.) } Other: Suspect or Possibly an Unregistered User Address: [Name-at-EmailAddress]

In order to fight spam, your posting (FROM) address [Name-at-EmailAddress]
shown in the message above must exactly match your subscription address.
This additional filter was added about a year ago to combat SPAM.
Forged Email abounds and the filter now catches nearly
100 spam message/day! If I did not enforce this requirement, then the
Listserver would become useless to all of you as you would be swamped
with junk mail.

Each Email that goes through the Listserver system is checked with
the database and if an EXACT match is not found then your Email will
be rejected. What do I mean by exact match, it is a case insensitive character
by character comparison. For example,

zaluzec-at-aaem.amc.anl.gov and zaluzec-at-anl.gov

are both my Email addresses at work, they are NOT a match, one is an aliases which
forwards Email to my real address (zaluzec-at-aaem.amc.anl.gov). One
will be rejected (zaluzec-at-anl.gov) while the other will go through.

If your Email address has changed or you are using an forwarding
address to redirect messages from your old address to your new one, please
remember that the Listserver does not know this . It is a very simple
and literal program. You have 2 options in this situation.

a.) change the FROM address of your Email client program to match
your original subscription address

b.) unsubscribe your old address and subscribe your new one.

I recommend option ( b.)

If neither of these two descriptions fits your rejection problem and your in a rush, or can't
do the task outlined above then you can submit your Question/Comment
via the WWW based Form.

This form is located at:

http://www.microscopy.com/MicroscopyListserver

You will be presented with a WWW form, into which you can cut and paste
your Email. Remember this message is sent first to me, and is reviewed to
insure it is NOT SPAM/JUNK mail, and then manually forwarded. This of
course means there will be a delay in posting as I generally do all this adminstrative
stuff on the Listserver only once per day.

Lastly, you can always send me a message which explains your problem
if it is outside the bounds of the above and we can try to sort out what is
wrong. Although most of the problems fit into one of the two above, but there
are always exceptions.

Thanks for your patience.

Nestor
Your Friendly Neighborhood SysOp.

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 09:30:50 2004

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Postdoctoral position: Gold nanoparticle labels will be developed to
target genetic tags on expressed proteins for identification of subunits
and alignment for image processing of cryoelectron micrographs. Four areas
will be coordinated: 1) Chemical design and synthesis of specialized gold
nanoparticles, 2) genetic expression of tagged proteins, 3) cryoEM using
JEOL 2010F 200keV field emission with 2k CCD and STEM attachment and 4) 3-D
image reconstruction. The position available will focus on preparing
cryo-EM samples, using the TEM to collect data, performing computer image
analysis and reconstructions, and developing some specialized
software. Desired experience includes: TEM and cryoEM operation,
programming (Fortran, C), Fourier transforms, image reconstruction,
biochemistry, and structural biology. Contact Dr. James Hainfeld,
Brookhaven National Lab, Biology Dept., Long Island, NY, 11973.
hainfeld-at-bnl.gov, 631-344-3367.

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 09:31:48 2004

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Group,

I am interested in hearing from anyone that has rebuilt or upgraded a Jeol 733 Microprobe. I have a 25 year old machine that has multiple problems, so I am considering what my options are for its future.

I am also considering the option of adding a single WDS spectrometer to our new SEM if I can find an appropriate port in order to have some WDS capability.

If you have experience in any these options I would love to hear from you.

Thanks

Roy Beavers

Southern Methodist University
Department of Geological Sciences
P.O. Box 750395
Dallas, Tx 75275
Voice: 214-768-2756
Fax: 214-768-2701
Email: rbeavers-at-mail.smu.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 10:08:49 2004

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We are considering the purchase of ICDD/NIST/JCPDS database software
intended for the identification of unknown phases using chemical and
structural information from analytical TEM (EDXS, SAD, powder diffraction,
etc.). Ideally this database would be sufficiently broad
as to be useful to many TEM users (from materials physics, chemistry, and
geology). The ICDD (international centre for diffraction data) product
overview (http://www.icdd.com/products/overview.htm) is specific on the
contents of the various databases ("133,370 inorganic entries") but a bit
vague on the software used to interface with the database (no demo, screen
shots or other such descriptions). A key feature would be the ability to
perform combined (chemical and structural) searches to produce a list of
candidate phases. I only have experience searching the PDF with an older
version of JADE (3rd party software with no combined search capability and
also geared toward XRD data). I would appreciate any comments from users of
these databases for similar purposes. Also I would be interested in any
comparison of the larger PDF database with the various specialty databases
(NIST crystal data file/CDF or the electron diffraction database/EDD) or any
other similar products.

Thanks,
Kevin Croat, PhD
Physics Department
Washington University
email: tkc-at-wustl.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 10:18:29 2004

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Dear Colleague:

We would like to invite researchers and students to the COnsortium for
Materials Properties Research in Earth Sciences (COMPRES) Workshop on
Focused Ion Beam (FIB) applications in Earth Sciences, which will be held on
27/28 March 2004 at the world-famous Mission Inn, Riverside, CA. Please note
that the date of the workshop is only just over a month away.

The goal of the workshop is to demonstrate the power of the FIB and
Transmission Electron Microscopy (TEM) for research in the Earth Sciences.
It is the first step in an effort to establish a facility that would make
possible access to this very expensive instrument at a reasonable price for
a broad spectrum of Earth Scientists. In a nutshell, this new instrument
makes preparation of TEM foils of rocks and minerals a very simple and
precise task.

The workshop will entail lectures and real-time demonstrations of use of the
FIB to prepare electron-transparent foils from rocks and minerals for
examination by TEM. Those who are interested to bring with them a sample for
which a TEM foil might be cut should bring a polished specimen no larger in
area than a conventional thin section and an optical or SEM image that can
serve as a map to find the desired location. A few specimens will be chosen
for demonstration purposes from specimens provided.

Live demonstration of foil preparation by FIB will be provided courtesy of
FEI Company at a site on the UCR campus; shuttle transportation between the
Mission Inn and Campus will be provided.

COMPRES has provided funding to allow significant subsidy for members of the
United States Earth Sciences community to attend the workshop. Such
subsidies are intended primarily for scientists, postdocs, and graduate
students who are unfamiliar with the FIB and the opportunities it offers for
enhancing their research. International participants are encouraged to
attend but, unfortunately, subsidies are not available.

The Workshop will be free for all attendees, but registration is required.
Please visit our web site for Conference agenda and other information:
http://www.igpp.ucr.edu/Conferences.htm

Lodging (double-occupancy) for nights of 26 & 27 March at the Mission Inn
(workshop site) in downtown Riverside, CA. will be provided for the first 60
US scientists who register for the workshop and request support. Limited
additional help toward travel and subsistence expenses will also be
available, evaluated on a case-by-case basis. Those requesting such
assistance should contact Harry Green by email (hgreen-at-mail.ucr.edu).

We have reserved a block of rooms at the Mission Inn at rates that
approximate $100/night for single rooms and $50-70 each person for double
rooms. The workshop will be held on Sat/Sun 27/28 March so that all
participants can obtain lower-cost air fares by staying over a Saturday
night. The Mission Inn can only hold rooms firmly for this workshop until
5 March, hence you are encouraged to register and reserve your room early.
Later reservations may be unavailable or available only at higher prices.
Those wishing single accommodation or who prearrange a roommate are
encouraged to make their hotel reservations directly with the Mission Inn
at: (909) 784-0300. Inform the reservation desk that you are attending the
"UCR Workshop on FIB". Those desiring the conveners to assign roommates
should contact hgreen-at-mail.ucr.edu. Conveners are: HW Green, L
Dobrzhinestkaya, and KN Bozhilov of the Institute of Geophysics and
Planetary Physics of the University of California, Riverside.

Riverside and the Mission Inn are easily reached via Ontario International
Airport (ONT), Ontario, CA.
Free shuttle transportation (~25 min) to and from ONT is provided by the
Mission Inn for guests who request such transportation and provide their
flight numbers and arrival/departure times in advance. Los Angeles
International Airport (LAX) is approximately 65 miles distant;
transportation to and from LAX is available by commercial shuttle service,
taxi, etc.

We hope to see many of you on March 27/28.

Regards,

Harry Green

*******************************************************************
Dr. Harry W. Green, II
Distinguished Professor of Geology and Geophysics
Director, Central Facility for Advanced Microscopy and Microanalysis (CFAMM)
Institute of Geophysics and Planetary Physics
University of California
Riverside, CA 92521
Tel: (909) 787-4505
Fax: (909) 787-4324
email: hgreen-at-ucrac1.ucr.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 10:44:07 2004

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The New England Society for Microscopy announces its March meeting, to be
held March 8th. 2004 at the Worcester Polytechnic Institute in Worcester,
Massachusetts.

Three speakers, two from WPI and one from UMass, will present a forum on
Nanotechnology.

Registration begins at 5.00 p.m., followed by a reception and buffet dinner
from 5:30-7:00 p.m.

Full details, including the program, directions and registration details,
are available on the Society's web pages at

{http://www.msa.microscopy.com/MSALAS/NESM/NESMHome.htm} http://www.msa.microscopy.com/MSALAS/NESM/NESMHome.htm

Please note the deadline for receipt of registrations is March 5th.

See you there!

Tony Garratt-Reed.

***********************************************
Anthony J. Garratt-Reed, M.A., D.Phil.
MIT Room 13-1027
77 Massachusetts Avenue
Cambridge, MA 02139-4307
USA

Tel: 617-253-4622
Fax: 617-258-6478
************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 12:14:12 2004

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} From: James Jefferson [mailto:James.Jefferson-at-hitachi-hhta.com]
Sent: Thursday, February 26, 2004 11:56 AM
To: littlesm-at-em.agr.ca

Dear Roy,
I sympathize in trying to keep a 25-year-old EM instrument in good working order
and producing valid results. I inherited a 1967 JEOL JXA-3A, a copy of an
original Castaing design and struggled for years with balky electronics,
unstable spectrometers, etc. I replaced it with a Microspec WDX-3PC in 1987 and
it is still giving us sterling service and still remarkably stable. I have
upgraded the software, replaced the computer twice and one cable driving the
detector once, but it just keeps running and giving good results. Your decision
to replace the EPMA with a single spectrometer on an SEM depends on your usage.
For metallurgists testing one to six elements, doing line scans and mapping of
just a few elements, the SEM+WDX solution is fine. If you are a geologist that
wants to test 20 elements and do quantitative maps on all of them on 100
samples, a dedicated EPMA is necessary.
Microspec has been bought by Oxford and, of course, the system has been
extensively upgraded since I purchased mine. You can contact Oxford about prices
and compatible SEM ports.
Good luck,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Beavers, Roy" {rbeavers-at-mail.smu.edu}
To: "Microscopy Listserver" {Microscopy-at-sparc5.microscopy.com} ; "Microprobe
List" {microprobe-at-microanalysis.org}
Sent: Thursday, February 26, 2004 7:44 AM

I have a binocular Zeiss phase contrast microscope that came with a basic
assortment of lenses. A while back I bought a planapo 10/0.32 lens
(standard - no phase ring) and was stunned at the quality of the image. To
describe the image as "sharp" or even "crisp" doesn't do it justice. Some
stained thin sections have the appearance of stained glass and the image
almost takes on a three dimensional quality. I was impressed.

Recently, I was able to acquire a planapo 100/1.3 Ph3. Despite its very
impressive appearance, I have been much less impressed with the image
produced by this lens. Granted, the contrast is better than the standard
lens, but based on the difference I had seen at 10x I was expecting a little
more in the sharpness department.

Bear in mind that I fall in the "hobbyist" ranks. Some of these questions
are basic. I have set up Kohler illumination. I believe that I have the
phase rings aligned. Most of these questions apply to brightfield
observation anyway.

Questions:
1) Am I simply expecting too much at 1000x?
2) Is the phase ring degrading the performance?
3) My condenser only has an n.a. of 0.9. Is this the problem?
4) Even with this condenser, should I be using oil on it as well as the
objective?
5) With the phase stop in place performance is worse - lots of artifacts.
That is not the case with the 40x and 10x phase objectives.

One more general question:
Literature tells me that I should achieve optimum contrast/resolution with
the brightfield aperture closed about 1/3 of the way. I seem to get the best
results with the aperture closed just a little over half way. Am I not
sensitive enough to artifacts and confusing increased contrast for increased
resolution? Am I maybe using too much light?

Thanks for your help,

Bruce Girrell

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 16:24:33 2004

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Bruce,
You ask a lot of questions and I am not going to be able to
cover them all. In terms of the "crispness quotient", when you are
working with a ten x lens you are quite far from the diffraction
limit so points in the image are quite point like. However, when you
are working with a 100 x lens, now you are near the diffraction limit
so points in the image are much less sharp. That is why things always
look fuzzier with high mag lenses. But the fuzzy items seen at 100 x
are invisible at 10 x.

Yes, to take full advantage of your 1.3 NA lens, you need a
condenser that also is 1.3 NA. With a 0.9 NA condenser, the NA of
your objective is limited to 0.9 NA because no light reaches beyond.
But you can't just oil a 0.9 NA condenser and turn it into a 1.3 NA.
Darn. You need a different condenser (I think with the Zeiss design,
there is a front element that just screws in and out so you just need
to find the right front element). If your microscope is an older
style Zeiss (pre white pyramid type) you might have trouble locating
such an element but should not be altogether impossible. And then
yes, it would need to be oiled. Bear in mind that the improvement by
doing this while unquestion in theory in practice depends on your
sample and your detector. If you are looking at a thickish sample
with your eye, you might not notice a difference. With a nice thin
sample, your eye probably will be able to notice a small improvement,
and a video camera would pick up more.

For phase contrast, try working with green light, instead of
while. That might make the high mag images look a little 'nicer' to
your eye.

Hope these help.

Tobias
}
}
} I have a binocular Zeiss phase contrast microscope that came with a basic
} assortment of lenses. A while back I bought a planapo 10/0.32 lens
} (standard - no phase ring) and was stunned at the quality of the image. To
} describe the image as "sharp" or even "crisp" doesn't do it justice. Some
} stained thin sections have the appearance of stained glass and the image
} almost takes on a three dimensional quality. I was impressed.
}
} Recently, I was able to acquire a planapo 100/1.3 Ph3. Despite its very
} impressive appearance, I have been much less impressed with the image
} produced by this lens. Granted, the contrast is better than the standard
} lens, but based on the difference I had seen at 10x I was expecting a little
} more in the sharpness department.
}
} Bear in mind that I fall in the "hobbyist" ranks. Some of these questions
} are basic. I have set up Kohler illumination. I believe that I have the
} phase rings aligned. Most of these questions apply to brightfield
} observation anyway.
}
} Questions:
} 1) Am I simply expecting too much at 1000x?
} 2) Is the phase ring degrading the performance?
} 3) My condenser only has an n.a. of 0.9. Is this the problem?
} 4) Even with this condenser, should I be using oil on it as well as the
} objective?
} 5) With the phase stop in place performance is worse - lots of artifacts.
} That is not the case with the 40x and 10x phase objectives.
}
} One more general question:
} Literature tells me that I should achieve optimum contrast/resolution with
} the brightfield aperture closed about 1/3 of the way. I seem to get the best
} results with the aperture closed just a little over half way. Am I not
} sensitive enough to artifacts and confusing increased contrast for increased
} resolution? Am I maybe using too much light?
}
} Thanks for your help,
}
} Bruce Girrell

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 19:22:35 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (hudson-at-uoneuor.uoregon.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, February 26, 2004 at 14:00:15
---------------------------------------------------------------------------

Email: hudson-at-uoneuor.uoregon.edu
Name: JoAn Hudson

Organization: University of Oregon

Title-Subject: [Microscopy] [Filtered] Book Reviewers for the Journal

Question:
I am looking for individuals to read and write a book review for the M&M Journal. I have the folowing titles available:

"Morphological and Compositional Evolution of Thin Films",
editors; Michael J. Aziz, Norman C. Bartelt, Isabelle Berbezier, James B. Hannon and Sean J. Hearne.

"Scanning Tunneling Microscopy and its Applications", 2nd revised edition, by C. Bai.

"Structure-Property Relationships of Oxide Surfaces and Interfaces II", editors; Kathleen B. Alexander, C. Barry Carter, Robin W. Grimes, Xiaoqing Pan, and Thomas E, Wood.

"Scanning Electron Microscopy of Cerebellar Cortex" by Orlando J. Castejon.

"Forensic Uses of Digital Imaging", by John C. Russ.

"Color Atlas and Manual of Microscopy for Criminalists, Chemists, and Conservators", by Nicholas Petraco and Thomas Kubic.

If you are interested please contact me. The reviews need to be completed by June 1, 2004. I will look forward to hearing from you and thank you for your interest in the society's journal.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 19:21:45 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (madelman-at-usuhs.mil) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, February 26, 2004 at 09:51:53
---------------------------------------------------------------------------

Email: madelman-at-usuhs.mil
Name: Mark R. Adelman

Organization: Associate Professor; APG; USUHS

Title-Subject: [Microscopy] [Filtered] Image Processing

Question: I am trying to get information on software I believe is/was marketed by the IATIA Group in Australia. However, their Website (http://www.iatia.com.au/) has not responded in some time now and I have been unable to find an alternative mode of contact. Does anyone know if they are still "in business"? If so, any info on how to contact them? Thanks in advance.
Mark R. Adelman, Ph.D.
Associate Professor of Anatomy, Physiology & Genetics
Uniformed Services University of the Health Sciences
4301 Jones Bridge Road
Bethesda, MD 20814-4799
USA
Phone: 301-295-3208
FAX: 301-295-1786
Email: madelman-at-usuhs.mil
Website: http://bicmra.usuhs.mil/

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Feb 26 22:03:51 2004

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Hi All,

Problem: During the ion milling of the glass ceramic sample (LaBGeO5) the
samples turns green at places where ion beam has hit.
Que: Is there anyone with experience on ion milling of glass ceramic samples
who can help in avoiding the beam damage?

Thanks
Pradyumna
610 758 5590 Lab
http://www.lehigh.edu/~png2/png2.html
"Time is what prevents everything from happening all at once: J. A. Wheeler"

-------------------------------------------------
This mail sent through IMP: http://horde.org/imp/

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 07:01:14 2004

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To all Listers,

one year ago I posted the information about EDX line wall chart, and
that I intend to make an EDX-database program for common download. I
just finished the project. Now you can download the MA-Table program for
free:

http://www.microanalyst.net/registr.phtml

The program has following features:

- Display of all line energies, detectable with EDX-spectrometers (and
WDX spectrometers too)
- Searching for overlaps via input of a peak energy position or via
specified element and line
- Display of line energies and relative line heights (line-marks,
peak-series)
- Simulation of complete EPMA EDX-spectra (characteristic lines,
Bremsstrahlung, artefacts, noise, ...),
under consideration of excitation conditions (Eo, geometry,
countrate, acquisition time, ...)
- Simulation of overlap situations
- Calculation of detection limits, taking into account excitation
conditions and overlap situation
- ...

You will find a short manual and FAQ's there:

http://www.microanalyst.net/manual.html

Best regards to all, I am waiting for some feedback and hints to improve
something

Frank Eggert
http://www.microanalyst.net

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 07:11:55 2004

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Bruce,
Possible answers:
1) Am I simply expecting too much at 1000x?
May be. I don't use oil cause I dislike the mess.

2) Is the phase ring degrading the performance?
Slightly, but most of us do not notice it.

3) My condenser only has an n.a. of 0.9. Is this the problem?
Yes - Your condenser NA should match or exceed the objective's NA. Then
you close the condenser down you are really reducing the condenser and
objective NA. Resolution is limited by the lowest refractive index in the
condenser/specimen/objective system. If only the objective is oiled the
air is between the condenser and specimen will limit your resolution the
refractive index will be 1 and not 1.5 something.

4) Even with this condenser, should I be using oil on it as well as the
objective?
NO!!! This condenser may not be sealed and you'll get oil in between the
lenses. Never a good thing.

5) With the phase stop in place performance is worse - lots of artifacts.
That is not the case with the 40x and 10x phase objectives.
Not surprising, your condenser isn't matching you objective, the rings may
not be lined up perfectly and you are seeing more of the smaller particles
of junk that might be in the prep but not resolving them, all of which can
degrade the image. The lack of oil between the condenser and specimen will
degrade performance. I think you can see why I don't use oil. Try using a
green filter, our eyes have the best sensitivity to it and all objective
are well corrected for green light.

One more general question:
Literature tells me that I should achieve optimum contrast/resolution with
the brightfield aperture closed about 1/3 of the way. I seem to get the
best
results with the aperture closed just a little over half way. Am I not
sensitive enough to artifacts and confusing increased contrast for
increased
resolution? Am I maybe using too much light?

This is a highly subjective rule depending on the contrast of the specimen
and the media. I use to tell my students when I was teaching to find the
Umpph position. That's were the image snaps into just the right contrast.
Typically 1/3 to 2/3 depending on objective and specimen. The best
resolution should occur with the condenser iris is open right to the edge
of the objective back focal plane. In an idea system, contrast would be
controlled by the difference between mounting media and the sample,
illumination by the use of filters. This would allow the objective to
"capture" all the defracted light rays it possibly could, forming the best
possible image. Oh yes, I'd use a green filter.....

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 09:17:10 2004

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Bruce

You should expect several differences from a planapo high N.A. lens.
First, the field of view should be flat, with much less of the image
out of focus at the edges.
Second, the color correction should be better, so that there should
be less chromatic aberration (seen a colored fringes, mostly at
edges)
Third, because of the high NA, you should see an increase in
resolution. That is, you should be able to see more fine detail in
objects.

However, this does come at a price. You don't mention the working
distance of your lenses, either the original 100x or the new one. In
general, a high NA lens has a shorter working distance, since the
additional NA implies that the lens can be brought closer to the
sample. The tradeoff is that your depth of focus will decrease, so
that material above or below the plane of focus will be out of focus.
On a thick, complex sample, this can create a haze that surrounds
the in-focus region.

In order to check these possibilities, I would suggest that you
examine a resolution standard to see whether there is a difference
between the lenses. A classic resolution standard might be a
preparation of diatoms, whose shells show very fine structural
variations, or the surface of the easily obtainable cheek smear
cells, which have a very fine network of ridges and grooves --for
this you may need to use phase optics.

You should also check the thickness of the samples that you are now
examining.

Joel

}
}
} ----------------------------------------------------------------------
} -------- The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ----------------------------------------------------------------------
} ---------
}
} I have a binocular Zeiss phase contrast microscope that came with a
} basic assortment of lenses. A while back I bought a planapo 10/0.32
} lens (standard - no phase ring) and was stunned at the quality of the
} image. To describe the image as "sharp" or even "crisp" doesn't do it
} justice. Some stained thin sections have the appearance of stained
} glass and the image almost takes on a three dimensional quality. I was
} impressed.
}
} Recently, I was able to acquire a planapo 100/1.3 Ph3. Despite its
} very impressive appearance, I have been much less impressed with the
} image produced by this lens. Granted, the contrast is better than the
} standard lens, but based on the difference I had seen at 10x I was
} expecting a little more in the sharpness department.
}
} Bear in mind that I fall in the "hobbyist" ranks. Some of these
} questions are basic. I have set up Kohler illumination. I believe that
} I have the phase rings aligned. Most of these questions apply to
} brightfield observation anyway.
}
} Questions:
} 1) Am I simply expecting too much at 1000x?
} 2) Is the phase ring degrading the performance?
} 3) My condenser only has an n.a. of 0.9. Is this the problem?
} 4) Even with this condenser, should I be using oil on it as well as
} the objective? 5) With the phase stop in place performance is worse -
} lots of artifacts. That is not the case with the 40x and 10x phase
} objectives.
}
} One more general question:
} Literature tells me that I should achieve optimum contrast/resolution
} with the brightfield aperture closed about 1/3 of the way. I seem to
} get the best results with the aperture closed just a little over half
} way. Am I not sensitive enough to artifacts and confusing increased
} contrast for increased resolution? Am I maybe using too much light?
}
} Thanks for your help,
}
} Bruce Girrell
}
}
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 11:10:55 2004

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Hi All,

Does anybody have a recipe and/or protocol for zinc formalin fixation? My colleagues used it many many years ago, but seemed to have misplaced their protocol. We will be using it to fix mouse/rat/human teeth before doing IHC with LM, TEM, SEM, and possibly confocal.

Thanks so much,

Elke Pravda
Biostructure Core Facility
The Forsyth Institute
Boston, MA 02155

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 12:28:11 2004

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You need low angle, low energy, and cooled samples. One question, though. Do your samples change back if you slightly heat them. If they are brittle, you can use the small angle cleavage technique on them without ion milling at all. Got to the South Bay Technology web site and look at the associated PDF files for their Microcleave kit. They have a poster on SACT that includes a short description on how to do glasses in it. You could also use Phil Swab's microtoming technique for preparting the samples. Both of these techniques have been discussed in this forum in the past.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: PrAdyUMna [mailto:png2-at-lehigh.edu]
Sent: Thursday, February 26, 2004 11:17 PM
To: microscopy-at-ns.microscopy.com

Hi All,

Problem: During the ion milling of the glass ceramic sample (LaBGeO5) the
samples turns green at places where ion beam has hit.
Que: Is there anyone with experience on ion milling of glass ceramic samples
who can help in avoiding the beam damage?

Thanks
Pradyumna
610 758 5590 Lab
http://www.lehigh.edu/~png2/png2.html
"Time is what prevents everything from happening all at once: J. A. Wheeler"

-------------------------------------------------
This mail sent through IMP: http://horde.org/imp/

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 12:57:38 2004

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Thanks for the reply and wonderful suggestions. I have not yet done the
heating so can not say for sure that what will happen after heating. But i saw
that same coloring of the sample occurs during X-Rray diffraction experiment
which makes me suspect that it may be due to formation of color centers.

Thnaks
Pradyumna

Quoting "Walck, Scott D." {walck-at-ppg.com} :

} You need low angle, low energy, and cooled samples. One question, though.
} Do your samples change back if you slightly heat them. If they are brittle,
} you can use the small angle cleavage technique on them without ion milling at
} all. Got to the South Bay Technology web site and look at the associated PDF
} files for their Microcleave kit. They have a poster on SACT that includes a
} short description on how to do glasses in it. You could also use Phil Swab's
} microtoming technique for preparting the samples. Both of these techniques
} have been discussed in this forum in the past.
}
} -Scott
}
} Scott D. Walck, Ph.D.
} PPG Industries, Inc.
} Glass Technology Center
} P. O. Box 11472 (letters)
} Guys Run Rd. (packages)
} Pittsburgh, PA 15238-0472
} Walck-at-PPG.com
} (412) 820-8651 (office)
} (412) 820-8515 (fax)
}
}
} -----Original Message-----
} From: PrAdyUMna [mailto:png2-at-lehigh.edu]
} Sent: Thursday, February 26, 2004 11:17 PM
} To: microscopy-at-ns.microscopy.com
} Subject: [Microscopy] Ion Milling: Beam damege, Glass Ceramic Sample
}
}
}
}
} -----------------------------------------------------------------------------
-
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------------
--
}
} Hi All,
}
} Problem: During the ion milling of the glass ceramic sample (LaBGeO5) the
} samples turns green at places where ion beam has hit.
} Que: Is there anyone with experience on ion milling of glass ceramic samples
}
} who can help in avoiding the beam damage?
}
} Thanks
} Pradyumna
} 610 758 5590 Lab
} http://www.lehigh.edu/~png2/png2.html
} "Time is what prevents everything from happening all at once: J. A. Wheeler"
}
}
} -------------------------------------------------
} This mail sent through IMP: http://horde.org/imp/
}

610 758 5590 Lab
http://www.lehigh.edu/~png2/png2.html
"Time is what prevents everything from happening all at once:J. A. Wheeler"

-------------------------------------------------
This mail sent through IMP: http://horde.org/imp/

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 14:24:39 2004

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Dear Pradyumna:

There was a paper published by Bernie Kestel describing a damage free preparation
technique involving chemical polishing methods. The technique involved first
dimpling (South Bay Technology D500i Dimpler®) a glass sample followed by chemical
thinning using a single vertical jet polishing instrument (specifically the South
Bay Technology Model 550). Although this is a labor intensive method it provided
some nice results from a damage free perspective. The reference is: Preparation of
Damage Free Glass TEM Specimens Bernard J. Kestel, Ultramicroscopy, Vol.83,
pp:61-66,(2000).

Along those same lines, the use of low energy ion thinning using Argon ions has
been successful in minimizing and eliminating damage in semiconductor samples like
Si and GaAs. Ion beam thinning at low voltages around 200 eV has been used for
improving high resolution imaging of these types of materials. We have not had any

experience in using this on glass materials but I would imagine it could perhaps
be extended to these material systems as well. We also offer a low energy ion
milling system and I would be happy to provide details.

DISCLAIMER: South Bay Technology produces equipment and supplies as described above
and, therefore, has a vested interest in promoting their use.

Best Regards,

Shane Roberts
Applications Engineering Manager
South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673
www.southbaytech.com
roberts-at-southbaytech.com
phone: 949.492.2600

PrAdyUMna wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi All,
}
} Problem: During the ion milling of the glass ceramic sample (LaBGeO5) the
} samples turns green at places where ion beam has hit.
} Que: Is there anyone with experience on ion milling of glass ceramic samples
} who can help in avoiding the beam damage?
}
} Thanks
} Pradyumna
} 610 758 5590 Lab
} http://www.lehigh.edu/~png2/png2.html
} "Time is what prevents everything from happening all at once: J. A. Wheeler"
}
} -------------------------------------------------
} This mail sent through IMP: http://horde.org/imp/

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy,
Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and
confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this
communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 14:52:22 2004

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Does anyone know why BEEM capsules are not available? I've talked to some
of the EM suppliers there stocks are gone. Does anyone know what is
happening with the company?

Tom Bargar
CEMRF-UNMC

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 15:30:26 2004

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Do you mean size 00 embedding capsules or actual capsule manufactured by BEEM?

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax

} } } {tbargar-at-unmc.edu} 02/27/04 04:05PM } } }

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Does anyone know why BEEM capsules are not available? I've talked to some
of the EM suppliers there stocks are gone. Does anyone know what is
happening with the company?

Tom Bargar
CEMRF-UNMC

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 15:32:09 2004

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The University of Texas Health Science Center will host a symposium
sponsored by
Hamamatsu Photonics KK
on

FRET, FLIM and Spectral Imaging:
Advanced Fluorescence Techniques for Biological Imaging

June 5-6, 2004

at

The Sheraton Gunter Hotel
205 E. Houston St.
San Antonio, TX

Registration Fees
Student: $300 ($400 after March 1st)
Academic/Corporate: $400 ($500 after March 1st)

Meeting, lodging and travel information may be found at:

www.uthscsa.edu/csb/imaging-course.html

or contact

Victoria Centonze Frohlich (frohlich-at-uthscsa.edu)

Speakers:
Ramesh Ahuja, LaVision Inc.
George Barisas, Colorado State University
Wolfgang Becker, Becker and Hickl
Robert Clegg, University of Illinois
Mary Dickinson, CalTech
Paul French, Imperial College London
Hans Gerritsen, University of Utrech
Brian Herman, University of Texas HSC, San Antonio
Jeremy Lerner, LightForm, Inc.
Rainer Pepperkok, EMBL Heidelberg
Ammasi Periasamy, University of Virginia
Herbert Schneckenburger, Universitat Ulm
Sebastian Tille, Carl Zeiss
Ton Visser, Wageningen University

In recent years, innovative methods in optical imaging, such as
Fluorescence Resonance Energy Transfer (FRET) and Fluorescent Lifetime
Imaging Microscopy (FLIM), and Fluorescence Spectral Detection, have piqued
the interest of the scientific community. These methods provide the
scientist with tools to solve complex biological problems. FRET imaging
enables the detection of complex structural associations at resolution
limits beyond conventional optical imaging. FLIM allows for a direct
measurement of FRET as well as faster, more accurate and quantitative
measurement of cell physiological changes. Fluorescence spectral detection
enables the investigator to discriminate signal from closely related
fluorophores beyond that which is capable with conventional filters. These
techniques are also being implemented in high-throughput screening regimes
for drug discovery. Invited lectures by a distinguished group of academic
and commercial speakers will concentrate on new technical developments in
these advanced optical imaging techniques and their applications in
biological and industrial settings.

We anticipate that this will be a most enjoyable as well as intellectually
stimulating symposium.

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 16:11:16 2004

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}
} Does anyone know why BEEM capsules are not available? I've talked to some
} of the EM suppliers there stocks are gone. Does anyone know what is
} happening with the company?
}
} Tom Bargar
} CEMRF-UNMC

Beem is alive & well & Ted Pella sells their products.
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 17:17:09 2004

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We have released version 1.0 of EDM (Electron Direct
Methods) software, available from http://www.numis.northwestern.edu/edm
Versions are available for Windows, Mac, various unix systems as well
as a GNU-like source-code build structure. The main features of the
code are:

* User friendly mouse-driven interface
* Crystallographic operations (e.g. symmetry averaging) on HREM images
with good numerical accuracy
* A number of image processing options, including Wiener-filtering,
masked/windowed Fourier Transforms and a Hanning Window Fourier
Transform
* Accurate cross-correllation based methods of measuring spot diffraction
intensities and user-friendly symmetry averaging with or without Friedel
symmetry
* Accurate methods of extracting phases from HREM images
* Includes Direct Methods code fs98 to solve structures, which can also
be used with other types of data (e.g. surface x-ray diffraction)
* Multislice code ncemss (seperate package), installed by default for
quantitative analysis of HREM images
* Free, GNU-like low-level source code which will run on almost any
computer with a viable X-windows system
* Listserver to help answer questions

-----------------------------------------------
Laurence Marks
Department of Materials Science and Engineering
Northwestern University
Evanston, IL 60201, USA
Tel: (847) 491-3996 Fax: (847) 491-7820
mailto:ldm2-at-risc4.numis.nwu.edu
http://www.numis.nwu.edu
-----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Feb 27 18:41:12 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Tom Bargar wrote:
============================================================
} Does anyone know why BEEM capsules are not available? I've talked to some
} of the EM suppliers there stocks are gone. Does anyone know what is
} happening with the company?
============================================================
A Google.com search on {BEEM capsules} will generate a worldwide list of
those offering BEEM capsules and other products made by BEEM, Inc.

Disclaimer: SPI Supplies is one of those firms offering products of BEEM,
Inc. (and with good stock).

Chuck
============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Sat Feb 28 13:49:35 2004

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Dear fellow microscopists,

Those of you who also fancy yourselves poets may be interested in
this competition:

At 1:38 AM -0500 2/27/04, Marc Abrahams wrote:
} 2004-03-12 Watch What You Eat Limerick Contest
}
} We invite you to enter the first and last annual WATCH WHAT YOU
} EAT LIMERICK COMPETITION, for the best (NEWLY composed!) limerick
} that elucidates this research report, which was brought to our
} attention by investigator Larry Camilli:
}
} "A Scanning Electron Microscopy Study of
} Japanese Noodles," J. E. Dexter, R. R. Matsuo,
} and B. L. Dronzek, Cereal Chemistry, vol. 56, 1979, p. 202.
}
} RULES: Please make sure your rhymes actually do, and that your
} limerick at least pretends to adhere to classic limerick form.
}
} PRIZE: The winning poet will receive a free electron-microscope-
} scannable issue of the Annals of Improbable Research. Send entries
} (one entry per entrant) to:
}
} WATCH WHAT YOU EAT LIMERICK CONTEST
} c/o {marca-at-chem2.harvard.edu}

best regards,
Steven Slap

From MicroscopyL-request-at-ns.microscopy.com Sun Feb 29 16:04:27 2004

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Dear friends,
I'd appreciate materials (pdf, ppt etc) and hints about the utilization
of microscopical techniques in conservation (arts).
Thank you
Alby
.......................................................................
...................................
.. non basta, resistere, resistere...resistere
^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
Alberto Diaspro
Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genoa, Italy
voice: +39-0103536426/480 fax 010314218
diaspro-at-fisica.unige.it, http://www.lambs.it
http://wiley.com/cda/product/0,,0471409200,00.html

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 08:18:15 2004

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Meeting Announcement
Midwest Microscopy and Microanalysis Society
Co-sponsor: Biological Imaging Facility,
Northwestern University, Evanston

Friday, March 26, 2004
Northwestern University
Pancoe Life Sciences Building
Pancoe/ENH Auditorium
Evanston, IL 60208
Meeting Schedule

Morning Session

9:00 Registration

9:45 Welcome and introduction

10:00 Stephen Paddock, University of Wisconsin-Madison: Butterflies, Zebras and Fairy Tales
- Applications of Three-Color Confocal Imaging

11:00 William Klein, Northwestern University: Imaging a New Molecular Basis for Alzheimer's
Disease

11:30 Richard Sumner, Rush Medical College: Assessment of Bone Formation
and Mineralization by Backscatter SEM

12:00-12:45 Lunch

12:45 Business Meeting

Afternoon session

1:00 Simon Watkins, University of Pittsburgh: Imaging Opportunities in the 21st Century

2:00 Pam Kreeger, Northwestern University: Alginate Matrices for the In Vitro Culture of
Immature Murine Ovarian Follicles

2:30 John Pedersen, Northwestern University: Cell/Extracellular Matrix Coupling in 3D
Hydrogels

3:00 Reception

RSVP Required

Please send RSVP via email, phone, or fax to:
Arvid Casler, MMMS Program Coordinator
c/o MAI
P. O. Box 394
Mundelein, IL 60060
phone/FAX: (847) 566-7716
email: arvid_casler-at-fmo.com

Admission: Free to MMMS Members

MMMS Membership: $10.00

MMMS membership available at registration

Driving directions to Northwestern University Evanston Campus available on the Web.

} From the north or northwest, via Interstate 88, Interstate 90 or Interstate 190
(Note: these are the directions to follow if traveling from O'Hare International Airport)
http://www.northwestern.edu/campus/directions/evanston-north-northwest.html

} From the west, via Interstate 94
http://www.northwestern.edu/campus/directions/evanston-west.html

} From the west or southwest, via Interstate 55 or Interstate 80

http://www.northwestern.edu/campus/directions/evanston-west-southwest.html

} From the south or southeast, via Interstate 94, Interstate 90, Interstate 80 or Interstate 57
http://www.northwestern.edu/campus/directions/evanston-south-southeast.html

Robert Mierzwa
JEOL USA, Inc.
3906 Lisa Ave.
Sheboygan WI 53083
TEL (920) 803-8945
FAX (920) 803-8946
Email: {mailto:mierzwa-at-jeol.com} mierzwa-at-jeol.com

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 09:40:55 2004

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Immunogold Workshop Announcement

Dear Researcher:

      The Electron Microscopy Facility-Medical School at the University
of Wisconsin is hosting a three-day workshop on immunogold techniques
from May 24-26, 2004. Dr. Jan Luenissen from Aurion Immunogold Reagents
& Accessories, an internationally known expert in the field, will be
the instructor for the workshop. The workshop will include lectures,
hands-on training, round table discussions, and presentations on
applications. Also, participants of the workshop will be able to work
on their own samples during the workshop. The workshop main curriculum
is detailed below. If you are interested in attending or need more
information about the workshop, please contact the workshop technical
coordinator Hong Yi by phone (404-727-8692) or email (hyi-at-emory.edu).

MAIN CURRICULUM

The properties of gold particles and their protein conjugates.
Theories underlying immunogold labeling protocols.
Silver enhancement of gold particles
Immunogold labeling on a variety of sample preparations for LM.
Immunogold labeling for EM
a. Pre-embedding immunogold labeling using ultrasmall gold conjugates
and silver enhancement.
b. Post-embedding immunogold labeling using conventional colloidal gold
conjugates and   ultrasmalll gold conjugates.
Pre- and post-embedding double immunogold labeling.
Background minimization in immunogold labeling
Signal amplification in immunogold labeling.

Thanks and we hope to see you in Madison.

Randall Massey
Operations Manager
UW-Electron Microscope Facility
1300 University Ave.
Madison, WI 53706
voice (608)262-2993
Fax  (608)262-7306

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 10:18:08 2004

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Ted Pella had a 6 month back-order for BEEM capsules when I tried to order
capsules a couple of weeks ago. I purchased capsules from EMS; they had
plenty in stock when I ordered, so you might try them.

Jessica Cervantes
Bend Research, Inc
64550 Research Rd
Bend, OR 97701
(541) 382-4100 page
(541) 382-0212 x240
(541) 382-6177 fax

-----Original Message-----
} From: Caroline Schooley [mailto:schooley-at-mcn.org]
Sent: Friday, February 27, 2004 2:25 PM
To: tbargar-at-unmc.edu
Cc: Microscopy-at-MSA.Microscopy.Com

}
} Does anyone know why BEEM capsules are not available? I've talked to some
} of the EM suppliers there stocks are gone. Does anyone know what is
} happening with the company?
}
} Tom Bargar
} CEMRF-UNMC

Beem is alive & well & Ted Pella sells their products.
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 16:10:07 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

All,
I need to purchase a closed perfusion/temperature chamber to use on a
confocal/MP equipped Nikon E-800 (an upright.) I would like to be able to
image cell cultures and tissues (e.g. brain slices.) After sifting through
the archive and doing online searches I have come up with two, the Dvorak
chamber with various temperature controllers, and the Harvard Apparatus
LU-CPC-CEH Leiden chamber. Would any one like to comment on these systems,
and do you have any other suggestions? Vendors (and anyone not wanting to
post to the server) are welcome to contact me directly.
Thanks,
Tom

Thomas Moninger (thomas-moninger-at-uiowa.edu)
University of Iowa Central Microscopy Research Facility
(www.uiowa.edu/~cemrf)
View expressed are my own.

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 17:01:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (forensic-at-mindspring.com) from on Monday, March 1, 2004 at 15:08:37
---------------------------------------------------------------------------

Email: forensic-at-mindspring.com
Name: Doug Byron

Organization: F.A.S.T. Inc.

Education: Graduate College

Location: Atlanta, Ga. USA

Question: Is there any protocols for microscopy examination for soot? The source is unknown, possible from candles, furnace or wildfire.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 22:07:08 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (maloneyb-at-fiu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, March 1, 2004 at 13:40:25
---------------------------------------------------------------------------

Email: maloneyb-at-fiu.edu
Name: Barbara

Organization: FCAEM/FIU

Title-Subject: [Microscopy] [Filtered] Liposomes

Question: Dear Group - have any of you been able to successfully image any liposomes on a SEM?
Thanks
Barb

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 1 23:17:33 2004

Contents Retrieved from Microscopy Listserver Archives
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I do believe you could use freeze-fracture or freeze-etching with or
without shadowing to visualize liposomes in modern SEMs. There are a few
companies on the market who sell special attachments to SEMs, so you may
process your sample (freeze, fracture, etch, shadow etc) and transfer in
SEM without breaking vacuum. I did see such machine from Gatan, but I am
sure other companies have similar equipment. This is a great way to
visualize practically any emulsion/suspension (it's widely used in cosmetic
industry). I hope it helps. Sergey
No interest in any manufacturer.

At 08:20 PM 3/1/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 08:00:38 2004

Contents Retrieved from Microscopy Listserver Archives
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O.k., I'm being dense here, could someone explain to me how using a higher
accellerating voltage could/would/should decrease chromatic aberations in the
EM? Particluarly in the TEM. Unless we're talking really low Kev (i.e. 100ev -
1,000ev vs 100,000ev - which is why I suspect one reason why low eV in
SEM's is generated by decellerating the electrons at the bottom on the lens
system) why would the energy spread of the primary electron beam vary?

Thank you.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 08:09:31 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

}
}
} } } } } }
} } } } } } Available immediately: Electroscan E3 Environmental scanning electron
} } } } } } microscope. Asking $30,000 or best offer. Buyer is responsible for
} } } } } } disassembly, rigging and shipping from Ithaca, NY. The instrument is
} } } } } } working, and was on a service contract until last June. There are
} } } } } } numerous accessories including a peltier stage, hot-stage, 1000 lb.
} } } } } } tensile stage, micromanipulator and microinjector. Two of the
} } } } } } mechanical pumps are equipped with Fomblin oil as is one of the
} } } } } } diffusion pumps. The Oxford X-ray detector window is broken and
} } has not
} } } } } } been used for several years; Reply directly to hunt-at-ccmr.cornell.edu
} } } } } } or call 607-255-3789 and speak with John Hunt
} } } } } }
} } } } } } This item is sold where is/as is, no warranties implied or given,
} } } } } } payment in full due at transfer, all packing and shipping costs are
} } the buyers.
} } } } } }
} } } } } } John Hunt
} } } } }
} } } } } CCMR Microscopy Facility
} } } } } 255-0108
} } }

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 08:49:14 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tomsk-at-clondiag.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 2, 2004 at 02:13:05
---------------------------------------------------------------------------

Email: tomsk-at-clondiag.com
Name: thomas kaiser

Organization: clondiag

Title-Subject: [Microscopy] [Filtered] miniaturized confocal

Question: hey all,
we would like to use a miniaturized confocal microscope
(with fibers as connectors and pinholes) to set up an
fluorescence detection apparatus. Do you know any
commercial available systems which could be used...since
we don`t want to invent the wheel again?
Many thanks Thomas

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 08:54:40 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Richard,

We just covered this a few weeks ago in my course:

The equation for the diameter of the disc of least confusion (d) for
chromatic aberration is:

d = Cc . alpha . (delta E / Eo)

Cc is the coefficient for chromatic aberration, alpha is the convergence
angle of the beam, delta E is the energy difference, and Eo is essentially
the beam energy. For thermionic emission from a tungsten filament, the
initial energy of the electrons varies between about 0 and 2 eV or so --
this is, I believe, a function of variations in their intitial thermal
energies within the filament.

As a result, if the accelerating voltage is 2 kV, (delta E / Eo) is 0.001;
if the accelerating voltage is 20 kV, (delta E / Eo) becomes 0.0001; and if
the accelerating voltage is 200 kV, (delta E / Eo) is 0.00001. Thus, the
diameter of the disc of least confusion for chromatic aberration is
basically inversely proportional to the accelerating voltage you're using.

Hope this helps,

Ellery

---------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
Department of Geology & Geophysics
University of Minnesota - Twin Cities
Lab Website: http://probelab.geo.umn.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 09:13:26 2004

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Dear Colleagues,

On behalf of the organizers I would like to invite you to a workshop
entitled "Multidimensional data presentation techniques" which will take
place on April 4 from 12:30 to 4:30 just before the opening of the
"Focus on Microscopy 2004" Conference in Philadelphia.

http://www.cyto.purdue.edu/FOM2004/ - workshop web page
http://www.focusonmicroscopy.org/ - FOM2004 web page

This workshop will include an interactive tutorial on the use of a
variety of techniques for multidimensional microscopy data presentation.
Many advanced visualization packages for microscopists are commercially
available. Similarly, plenty of applications for video processing and
presentations can be found on the market. However, transforming complex
data sets into the actual presentation for use in lectures or in web
sites is not as easy as it seems. There are a variety of
tricks-of-the-trade, useful suggestions, and some very nice inexpensive
or free software obtainable. We would like to share our experiences and
tell you about them!

You will learn how to present static 2D images as well as 3D datasets in
the most efficient way. We will show you how to produce short animations
using data from confocal/MP systems in highly compressed MPEG4-based
formats. You will receive a handout and CD-ROM containing key materials
presented in the workshop as well as a significant number of really
valuable free utility software packages.

We will demonstrate:
* How to compress microscopy data. What are the pros and cons of
compression? Does it affect final results? What about lossy and lossless
compression?
* How you should present your 3D data. How to prepare 3D image
reconstruction? How to create anaglyphs? How to protect the data in an
anaglyph when you compress it? How to make a movie anaglyph/animation?
* How to create an animation from a 3D construction.
* How to create movies that are playable in PowerPoint, on web pages, or
with other media.
* How to understand codecs and their associated problems.
* How to edit animations/movies using high-speed command line processing.
* How to you add your name, logo of your institution, or other info into
the movie.
* How to deal with sound overlays.
* How to reproduce a movie-making process. You will learn simple command
line macros that are really fast!

If you are registered for the workshop, please take some time to take
our pre-workshop survey. Your participation will help us greatly with
the workshop preparation. We would like to know about your expectations,
your level of experience in multimedia multidimensional data
presentation techniques, and the issues you consider to be important.
The link to the survey is present on the workshop web page.

Bartek Rajwa

rajwa at flowcyt.cyto.purdue.edu
Purdue University Cytometry Laboratories

------------------------------------------------------------------------------

The organizers of the workshop gratefully acknowledge the assistance of
Media Cybernetics Corporation, the producer of Image-Pro Plus - an image
analysis software package for fluorescence imaging, quality assurance,
materials imaging, and various other scientific, medical, and industrial
applications.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 09:55:27 2004

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Bioptechs has a line of temperature controlled chambers, with good
design for the flow so that they can handle fairly large flow volume
without tearing your sample off the coverslip. They also sell
temperature controlled collars for the objectives, so that your oil
immersion doesn't act as a huge temperature sink.

If you are heating the objectives I strongly recommend the Boekel Warmer
they carry, or its like, to keep the objectives warm at all times. You
want to minimize the temperature cycling on the lenses, as it will over
time induce strain on the elements. That can lead to unwanted
polarization effects or other problems, very unpleasant with an
expensive objective.

http://www.bioptechs.com/

Note that I'm a bit biased - I don't work for Bioptechs, but I helped
test these some 15 years ago when they were first designed...

-- Kevin Ryan
kevin-at-mediacy.com

-----Original Message-----
} From: Moninger, Thomas [mailto:thomas-moninger-at-uiowa.edu]
Sent: Monday, March 01, 2004 5:23 PM
To: 'Microscopy-at-MSA.microscopy.com'

All,
I need to purchase a closed perfusion/temperature chamber to use on a
confocal/MP equipped Nikon E-800 (an upright.) I would like to be able
to image cell cultures and tissues (e.g. brain slices.) After sifting
through the archive and doing online searches I have come up with two,
the Dvorak chamber with various temperature controllers, and the Harvard
Apparatus LU-CPC-CEH Leiden chamber. Would any one like to comment on
these systems, and do you have any other suggestions? Vendors (and
anyone not wanting to post to the server) are welcome to contact me
directly. Thanks, Tom

Thomas Moninger (thomas-moninger-at-uiowa.edu)
University of Iowa Central Microscopy Research Facility
(www.uiowa.edu/~cemrf)
View expressed are my own.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 09:57:49 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Richard

I'm not sure if this is what you mean. But if
resoln (Chromatic) = constant x focal length x semi angle x delta V/V
then if a finite change in voltage occurs (delta V) increasing V must improve resolution. Part of this may due to the optics of the system but a major consideration is the thickness of specimen where I'd always understood that the loss of voltage was roughly finite (I won't say linear) then increasing the overall accelerating voltage should improve resolution. This does work even at 60kv+.

I hope I haven't baffled anyone with my 'Noddy' science.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
UK

----- Original Message -----
} From: Richard Edelmann {edelmare-at-muohio.edu}

I am thinking that the energy spread of the the source should be the
same reguardless of accellerating voltage and the accellerator adds
the exact same elctron volts to all electrons so the energy
(chromatic) spread arriving at any lens should be the same no matter
the accelerating voltage. Chromatic aberation, however, is a function
of the relative energy spread compared to the final ev. The
deflection error due to the spread at the source has a much smaller
contribution to the total deflection in a higher voltage TEM lens.

My 2 ev worth

Dave

--
David Barnard
Wadsworth Ctr
NYS Dept Health
Albany NY 12201-0509
barnard-at-wadsworth.org
518 473-5299 voice
518 474-7992 fax

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 12:12:03 2004

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Listers,

Here is the table of contents for the March/April 2004 issue of Microscopy
Today.

New Subscriptions via http://www.microscopy-today.com only, please.
New subscriptions will close on Friday March 5th for this issue.

WE ARE PURGING NON-MSA MEMBER, NON-NORTH AMERICAN, UNSUBSCRIBED INDIVIDUALS!
WE ARE AWAITING THE LATEST INPUT FROM THE MSA MEMBER RENEWAL PROCESS BEFORE
COMPLETING THE PURGING PROCESS. SEVERAL HUNDRED NON-QUALIFIED SUBSCRIBERS
HAVE ALREADY BEEN DROPPED.

March/April Microscopy Today Contents:

Carmichael and Lingle: Fluorescent Speckle Microscopy

Hall: The Nematode Caenorhabditis elegans, A Model Animal "Made for
Microscopy"

Sedgewick: Digital Movies for Others to See

Galvez, Giberson, & Cardiff: Microwave Mechanisms - The Energy/Heat
Dichotomy

Neal: Photoshop and 12-bit Digital Microscope Camera Images

Nester: Guidance for Choosing When to Use Electron and/or Light Microscopy
and Related ASTM E4 Standards

Simmons: The Role of Microscopy in Indoor Air Quality Investigations

Humphrey: How to Promote a Facility in Order to Increase Use, Acquire New
Equipment and, as a Result, Increase Revenue

Hudson, Benedict, & Flaitz: TEM Specimen Preparation Technique for Small
Semiconductor Devices

Duke: Lens Cleaning - Best Practices Review

Stephenson and Gabel: Use of Fishing Weight Putty for Quickly Mounting SEM
Specimens

Sepsenwol: A Homemade Vacuum Forceps For Mounting Small SEM Samples

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 13:27:10 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

O.k., I'm being dense here, could someone explain to me how using a higher
accellerating voltage could/would/should decrease chromatic aberations in the
EM? Particluarly in the TEM. Unless we're talking really low Kev (i.e. 100ev -
1,000ev vs 100,000ev - which is why I suspect one reason why low eV in
SEM's is generated by decellerating the electrons at the bottom on the lens
system) why would the energy spread of the primary electron beam vary?

Thank you.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 13:47:04 2004

Contents Retrieved from Microscopy Listserver Archives
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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

}
}
} } } } } }
} } } } } } Available immediately: Electroscan E3 Environmental scanning electron
} } } } } } microscope. Asking $30,000 or best offer. Buyer is responsible for
} } } } } } disassembly, rigging and shipping from Ithaca, NY. The instrument is
} } } } } } working, and was on a service contract until last June. There are
} } } } } } numerous accessories including a peltier stage, hot-stage, 1000 lb.
} } } } } } tensile stage, micromanipulator and microinjector. Two of the
} } } } } } mechanical pumps are equipped with Fomblin oil as is one of the
} } } } } } diffusion pumps. The Oxford X-ray detector window is broken and
} } has not
} } } } } } been used for several years; Reply directly to hunt-at-ccmr.cornell.edu
} } } } } } or call 607-255-3789 and speak with John Hunt
} } } } } }
} } } } } } This item is sold where is/as is, no warranties implied or given,
} } } } } } payment in full due at transfer, all packing and shipping costs are
} } the buyers.
} } } } } }
} } } } } } John Hunt
} } } } }
} } } } } CCMR Microscopy Facility
} } } } } 255-0108
} } }

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 13:50:22 2004

Contents Retrieved from Microscopy Listserver Archives
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I am the keeper of the MSA videos and am in the process of transferring
them to DVD. Several masters are in bad condition and I do not have any
other copies. If there is anyone out there who has a copy of number 214,
3D Deconvolution from 1998, I would appreciate the opportunity to borrow
it so that it may be restored to the collection. You may expect to hear
from me in the future with similar requests.
Thanks in advance

Greg Erdos

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 14:11:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Thomas

Try contacting Martin Harris at Optiscan Imaging, Melbourne, Australia
(martinh-at-optiscan.com) they specialise in miniture confocal instruments
for edoscopy and the like.

Ian

Ian Hallett
HortResearch
Mt Albert Research Centre, Private Bag 92 169
Auckland, New Zealand
Fax +64 9 815 4201
Telephone +64 9 815 4200
EMail ihallett-at-hortresearch.co.nz

} } } by way of MicroscopyListserver {tomsk-at-clondiag.com} 3/03/2004
4:02:27 } } }

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America

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (tomsk-at-clondiag.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, March 2, 2004 at 02:13:05
---------------------------------------------------------------------------

Email: tomsk-at-clondiag.com
Name: thomas kaiser

Organization: clondiag

Title-Subject: [Microscopy] [Filtered] miniaturized confocal

Question: hey all,
we would like to use a miniaturized confocal microscope
(with fibers as connectors and pinholes) to set up an
fluorescence detection apparatus. Do you know any
commercial available systems which could be used...since
we don`t want to invent the wheel again?
Many thanks Thomas

---------------------------------------------------------------------------

______________________________________________________
The contents of this e-mail are privileged and/or confidential to the
named recipient and are not to be used by any other person and/or
organisation. If you have received this e-mail in error, please notify
the sender and delete all material pertaining to this e-mail.
______________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 17:23:15 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (njws-at-aol.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 2, 2004 at 15:56:37
---------------------------------------------------------------------------

Email: njws-at-aol.com
Name: norman woodside

Organization: retired vendor sales

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: For anyone in the Baltimore/Washington area or anyone else willing to pick them up, I have the following items to donate free of charge. I have retired after 40 years in the field of electron microscopy and would like not to have to leave these things at the curb for regular Thursday pick-up. All must be taken(not piecemeal) and no shipping. Anyone interested should e-mail me to set up a time.

BOOKS:
Biology of animal viruses,vol I, II
Histological techniques for electron microscopy
A color atlas and text for histopathology
Immunology for students of medicine
Electron microscopic anatomy
Positive staining for electron microscopy
X-ray microanalysis in the electron microscope
Principles and techniques of electron microscopy,Hyatt
Principles and techniques in histochemistry
Ultramicrotomy,Reid
Cell pathology
Ultrastructural pathology of the cell
An introduction to virology
Diagnostic electron microscopy
Viral immunodiagnosis
Low temperature methods in electron microscopy
Histology-a text and atlas,Rhodin
A textbook of histology,Bloom and Fawcett
An atlas of ultrastructure,Rhodin
Ultrastructural aspects of disease

OTHER:

Ohaus triple bneam balance
Fisher water bath
2 stereo heads
approx8 boxes various sized glass strips (LKB)

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 2 18:09:13 2004

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Colleagues

There was a virus attack on Dee Breger's computer.

The virus is sending out alot of email with her name on
it and since the faked Email address is one of a valid
"subscriber" the messages are getting through the filter.

There was a slew of them which appeared between ~ 5:30-6 PM
Central Standard Time on 3/2/04

Please trash any Email with her name on it immediately.
I am in the process of trying to block any new postings.

Please be aware that spam attacks like this frequently
are intended to embarrass the person whose "ID" was
stolen/forged. Or to use them as a source of continued infection.
Do not reply, I would even suggest that you do not even open
the messages.

On behalf of Dee, who has also called me, she apologizes that this has happened
and hopes that you will all understand.

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 02:58:05 2004

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-- Hi everybody,
We have to confirm the identity of polypropylene and polyethylene in a
film embedded in a resin using TEM. We cut with the ultramicrotome the
sections and stain with OsO4 during 30 minutes. It is the first time
that we do this and the results aren´t good, because there isn´t
reaction with the OsO4.
Has everyone done this type of work? We need sugerences.
A lot of thanks in advance

*************************************************************
Dra. María Belén López Mosquera
Unidade de Microscopía
Servicios Xerais de Apoio á Investigación
Universidade da Coruńa
Edificio Servicios Centrais de Investigación
Campus de Elvińa s/n
E-15071 A Coruńa

Teléfono: 34 981 167 000 ext.: 2087
Telecopia: 34 981 167 068
Correo eléctrónico: sxaimic-at-udc.es
**************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 03:09:38 2004

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A related question:

} From 'Polymer Microscopy' by Saywer and Grubb I got the idea that it's not
the energy
spread of the primary beam that limits resolution but the energy spread due
to the specimen.
I assume that the same formula for the disk of least confusion applies no
matter what the source
of deltaE, but I'm wondering which energy spread is really limiting for high
resolution TEM
of 2D protein crystals for example.

Here comes a somewhat lengthy discussion that I wrote when I read that book.
I'd be grateful
if somebody could tell me whether I'm on the right track:

The most probable inelastic interaction is the 'plasmon production' with a
most probable energy

loss to the scattered electrons of around 25 eV for carbon (EELS Atlas).

The mean free path for plasmon loss scattering is in the order of 100 nm for
100 keV electrons

(table in Williams and Carter, page 657, which unfortunately doesn't include
carbon).

I think the argument used in 'Polymer Microscopy' by Sawyer and Grubb runs
as follows:

} From the data above an electron loses about 25 eV of energy every 100 nm or
0,25 eV per nm of

specimen thickness it traverses.

Since this energy loss is stochastic the beam also suffers an energy-spread
deltaE of about

the same magnitude. Due to the chromatic aberration of the objective lens
this energy-spread limits the

attainable resolution to a value that depends on the thickness given by the
following rule of thumb:

One should not expect to resolve details smaller than one tenth of the
specimen thickness for

carbonacious specimens.

My comment: This argument is only valid for specimens that are at least 100
nm thick. If the specimen

is considerably thinner than the mean free path for inelastic scattering
(for example 10-20 nm as is usual

in structure determination of proteins (excluding viruses)) only relatively
few electrons have been

inelastically scattered at all and it doesn't make sense to speak of an
energy spread due to the specimen.

The unscattered (which form the majority) and elastically scattered
electrons have the same energy-spread

as the incoming electrons. Most of the inelastically scattered electrons
have an energy spread that's given

by the width of the plasmon loss curve, that means a deltaE of about 50 eV
(Ahn, Krinanek: EELS-Atlas).

In the weak phase-weak amplitude approximation only the unscattered and
elastically scattered electrons

are regarded as taking part in image formation, whereas the inelastically
scattered electrons lead to

background noise. Therefore the energy-spread of the inelastically scattered
electrons is irrelevant.

Sawyer and Grubb treat energy-loss as a continuous process (". will cause a
100 keV electron to loose

about 0.25 eV per nanometer of thickness on average."). In fact an electron
either losses the energy of a

plasmon (10 to 50 eV) or it doesn't and on average it does so every 100 nm
it travels through the specimen.

Only when the specimen is thicker than the mean free path does it make sense
to speak of an average

energy loss per nm thickness.

For faster electrons (for example 300 keV) the mean free paths are longer
and accordingly all thickness

limits higher.

Philip Koeck
Svdertvrns Hvgskola and
Karolinska Institutet
Dept. of Bioscience at Novum
S-14157 Huddinge
Sweden
phone: +46-8-6089186
fax: +46-8-6089290
http://www.biosci.ki.se/em

'This winter I am giving courses to three students, of whom one is only
moderately prepared,
the other less than moderately, and the third lacks both preparation and
ability.
Such are the burdens ...' Carl Friedrich Gauss (1810)
______________________________________________

----- Original Message -----
} From: "Ellery Frahm" {frah0010-at-umn.edu}
To: {edelmare-at-MUOHIO.EDU} ; {microscopy-at-MSA.Microscopy.com}
Sent: Tuesday, March 02, 2004 4:07 PM

Folks:

Thank you for the info! I was not aware of the chromatic aberation
equation. Thank you.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 08:20:42 2004

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Hello: I would try staining with Ruthenium Tetraoxide (RuO4). Even though
both polymers will stain they should stain at different rates. According
to "Ruthenium Tetraoxide Staining of Polymers for Electron Microscopy" by
Trent et al published in Macromolecules 1983 16, 589-598 polyethylene oxide
will stain faster than isotactic polypropylene. I would stain only for
between 5 min and 15 min. Both RuO4 and OsO4 are very dangerous chemicals
so please be sure to observe proper safety procedures.
Also you will need to use a cryo-ultramicrotome or the polypropylene phase
will smear. Good luck. Steve

-- Hi everybody,
We have to confirm the identity of polypropylene and polyethylene in a
film embedded in a resin using TEM. We cut with the ultramicrotome the
sections and stain with OsO4 during 30 minutes. It is the first time
that we do this and the results aren´t good, because there isn´t
reaction with the OsO4.
Has everyone done this type of work? We need sugerences.
A lot of thanks in advance

Stephen McCartney
Research Associate
Materials Research Institute
2108 Hahn Hall
Va Tech
Blacksburg, VA 24061
540-231-9765 - phone
540-231-8517 - FAX

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 08:44:22 2004

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A very reasonable argument, alas wrong.

To first-order plasmons don't change the angle of the electrons,
so an image with the plasmons is very close to an image with
the no-loss electrons shifted in focus (the chromatic aberration
term). A rough approximation is to consider the electrons which
have lost energy as a background term, say B, in which case
your contrast goes down by ~1/(1+B) so you lose apparent resolution
because your signal-to-noise ratio is getting worse. (Noise from
counting statistics; there is only one electron in the column at a
time and you don't collect that many in an image.) For a thicker
sample you should also reduce the amplitude/intensity of the zero-
loss electrons, another reduction in your contrast. Note that it
is contrast relative to noise that matters. (There are some non-linear
imaging effects, and the imaging theory for electrons which have
lost energy is a bit more complicated than this, but these effects
is probably not relevant for proteins.)

N.B. I suspect that you are understimating the mean-free path,
particularly for a low-density protein.

-----------------------------------------------
Laurence Marks
Department of Materials Science and Engineering
Northwestern University
Evanston, IL 60201, USA
Tel: (847) 491-3996 Fax: (847) 491-7820
mailto:ldm2-at-risc4.numis.nwu.edu
http://www.numis.nwu.edu
-----------------------------------------------

On Wed, 3 Mar 2004, Philip Koeck wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} A related question:
}
} } From 'Polymer Microscopy' by Saywer and Grubb I got the idea that it's not
} the energy
} spread of the primary beam that limits resolution but the energy spread due
} to the specimen.
} I assume that the same formula for the disk of least confusion applies no
} matter what the source
} of deltaE, but I'm wondering which energy spread is really limiting for high
} resolution TEM
} of 2D protein crystals for example.
}
} Here comes a somewhat lengthy discussion that I wrote when I read that book.
} I'd be grateful
} if somebody could tell me whether I'm on the right track:
}
} The most probable inelastic interaction is the 'plasmon production' with a
} most probable energy
}
} loss to the scattered electrons of around 25 eV for carbon (EELS Atlas).
}
} The mean free path for plasmon loss scattering is in the order of 100 nm for
} 100 keV electrons
}
} (table in Williams and Carter, page 657, which unfortunately doesn't include
} carbon).
}
}
}
} I think the argument used in 'Polymer Microscopy' by Sawyer and Grubb runs
} as follows:
}
} } From the data above an electron loses about 25 eV of energy every 100 nm or
} 0,25 eV per nm of
}
} specimen thickness it traverses.
}
} Since this energy loss is stochastic the beam also suffers an energy-spread
} deltaE of about
}
} the same magnitude. Due to the chromatic aberration of the objective lens
} this energy-spread limits the
}
} attainable resolution to a value that depends on the thickness given by the
} following rule of thumb:
}
} One should not expect to resolve details smaller than one tenth of the
} specimen thickness for
}
} carbonacious specimens.
}
}
}
} My comment: This argument is only valid for specimens that are at least 100
} nm thick. If the specimen
}
} is considerably thinner than the mean free path for inelastic scattering
} (for example 10-20 nm as is usual
}
} in structure determination of proteins (excluding viruses)) only relatively
} few electrons have been
}
} inelastically scattered at all and it doesn't make sense to speak of an
} energy spread due to the specimen.
}
} The unscattered (which form the majority) and elastically scattered
} electrons have the same energy-spread
}
} as the incoming electrons. Most of the inelastically scattered electrons
} have an energy spread that's given
}
} by the width of the plasmon loss curve, that means a deltaE of about 50 eV
} (Ahn, Krinanek: EELS-Atlas).
}
} In the weak phase-weak amplitude approximation only the unscattered and
} elastically scattered electrons
}
} are regarded as taking part in image formation, whereas the inelastically
} scattered electrons lead to
}
} background noise. Therefore the energy-spread of the inelastically scattered
} electrons is irrelevant.
}
} Sawyer and Grubb treat energy-loss as a continuous process (". will cause a
} 100 keV electron to loose
}
} about 0.25 eV per nanometer of thickness on average."). In fact an electron
} either losses the energy of a
}
} plasmon (10 to 50 eV) or it doesn't and on average it does so every 100 nm
} it travels through the specimen.
}
} Only when the specimen is thicker than the mean free path does it make sense
} to speak of an average
}
} energy loss per nm thickness.
}
}
}
} For faster electrons (for example 300 keV) the mean free paths are longer
} and accordingly all thickness
}
} limits higher.
}
}
}
}
}
}
}
} Philip Koeck
} Svdertvrns Hvgskola and
} Karolinska Institutet
} Dept. of Bioscience at Novum
} S-14157 Huddinge
} Sweden
} phone: +46-8-6089186
} fax: +46-8-6089290
} http://www.biosci.ki.se/em
}
} 'This winter I am giving courses to three students, of whom one is only
} moderately prepared,
} the other less than moderately, and the third lacks both preparation and
} ability.
} Such are the burdens ...' Carl Friedrich Gauss (1810)
} ______________________________________________
}
}
} ----- Original Message -----
} } From: "Ellery Frahm" {frah0010-at-umn.edu}
} To: {edelmare-at-MUOHIO.EDU} ; {microscopy-at-MSA.Microscopy.com}
} Sent: Tuesday, March 02, 2004 4:07 PM
} Subject: [Microscopy] Re: KeV vs chromatic aberation
}
}
} }
} }
} } --------------------------------------------------------------------------
} ----
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------------
} -----
} }
} } Hi Richard,
} }
} } We just covered this a few weeks ago in my course:
} }
} } The equation for the diameter of the disc of least confusion (d) for
} } chromatic aberration is:
} }
} } d = Cc . alpha . (delta E / Eo)
} }
} } Cc is the coefficient for chromatic aberration, alpha is the convergence
} } angle of the beam, delta E is the energy difference, and Eo is essentially
} } the beam energy. For thermionic emission from a tungsten filament, the
} } initial energy of the electrons varies between about 0 and 2 eV or so --
} } this is, I believe, a function of variations in their intitial thermal
} } energies within the filament.
} }
} } As a result, if the accelerating voltage is 2 kV, (delta E / Eo) is 0.001;
} } if the accelerating voltage is 20 kV, (delta E / Eo) becomes 0.0001; and
} if
} } the accelerating voltage is 200 kV, (delta E / Eo) is 0.00001. Thus, the
} } diameter of the disc of least confusion for chromatic aberration is
} } basically inversely proportional to the accelerating voltage you're using.
} }
} } Hope this helps,
} }
} } Ellery
} }
} } ---------------
} } Ellery E. Frahm
} } Research Scientist/Manager
} } Electron Microprobe Laboratory
} } Department of Geology & Geophysics
} } University of Minnesota - Twin Cities
} } Lab Website: http://probelab.geo.umn.edu
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 09:20:03 2004

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We are looking for a new critical point dryer and would appreciate any
feedback users can provide. We currently have a Polaron Jumbo, that is
about 30 years old. It works, but the temperature rises very high - it is
controlled just by hot water - and each run seems to have different
conditions. We would like to get a machine that might be more constant from
one run to the next, and that students might find somewhat easier to use.
Most of the CPDs we have seen through our web hunts seem to have very small
sample chambers, though. We would like to know 1) what CPDs people like, 2)
whether sample chamber size seems to be a problem, 3) any other concerns
that users have and would alert us to.
Many thanks,

Dr. Sally Leys
Assistant Professor and Canada Research Chair
in Evolutionary Developmental Biology
Department of Biological Sciences CW 405
The University of Alberta
Edmonton, Alberta
Canada
T6G 2E9

Telephone: (780) 492-6629
Fax: (780) 492-9234
Email: sleys-at-ualberta.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 09:40:48 2004

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Hello fellow Microscopists,

How can we best prepare our soil samples for SEM and micro analysis? We are novices at this. We have great equipment (Hitachi FESEM 4500 and EDAX Genesis) We are interested in phosphorus and iron in river sediments. We are having difficulty in interpreting the results we have been getting (we crushed soil to double sticky tape, mounted on Al stubs and coated with AuPd). The preps look good at the SEM with little charging.

What we see is grains and some organic matter (OM) and coatings. The spectrum shows some OM and SiO2 along with other particles of mixed composition.

My question is how can we interpret this? What about references etc? We need your expertise!

Your help will be greatly appreciated.
Carol Bronick

Agricultural Research Station
Box 9061
Virginia State University
Petersburg, VA 23806
804.524.6822
cbronick-at-vsu.edu

____________________________________________________________________
Check your SchoolEmail at http://www.CampusI.com
Find the LOWEST PRICES on books at http://www.campusi.com/BookFind !

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 09:57:51 2004

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Slight correction to my previous post. Of course you will have problems
with both the polyethylene and polypropylene if you don't use a cryo system
when microtoming. Steve

Hello: I would try staining with Ruthenium Tetraoxide (RuO4). Even though
both polymers will stain they should stain at different rates. According
to "Ruthenium Tetraoxide Staining of Polymers for Electron Microscopy" by
Trent et al published in Macromolecules 1983 16, 589-598 polyethylene oxide
will stain faster than isotactic polypropylene. I would stain only for
between 5 min and 15 min. Both RuO4 and OsO4 are very dangerous chemicals
so please be sure to observe proper safety procedures.
Also you will need to use a cryo-ultramicrotome or the polypropylene phase
will smear. Good luck. Steve

Stephen McCartney
Research Associate
Materials Research Institute
2108 Hahn Hall
Va Tech
Blacksburg, VA 24061
540-231-9765 - phone
540-231-8517 - FAX

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 10:52:52 2004

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Dear Sally,
I recently needed to buy a CPD for my new lab and after
looking into the options I bought a Tousimis Samdri PVT-3D. This unit
has cooling for the chamber provided by letting CO2 from the tank run
past the chamber, so it is easy to cool. I like not having to mess
with water cooling. I also like to do my ethanol CO2 exchanges around
0C. The chamber size is 1.25 in round by 1.25 in tall. There is an
accessory available to make a much bigger chamber (not wider, just
longer). I also have been extremely impressed by the Tousimis company
support, with nice instructions and extras, and prompt responses to
my frequent questions.

I have no financial interest in the company, just a happy customer,

Tobias

}
} We are looking for a new critical point dryer and would appreciate
} any feedback users can provide. We currently have a Polaron Jumbo,
} that is about 30 years old. It works, but the temperature rises very
} high - it is controlled just by hot water - and each run seems to
} have different conditions. We would like to get a machine that might
} be more constant from one run to the next, and that students might
} find somewhat easier to use. Most of the CPDs we have seen through
} our web hunts seem to have very small sample chambers, though. We
} would like to know 1) what CPDs people like, 2) whether sample
} chamber size seems to be a problem, 3) any other concerns that users
} have and would alert us to.
} Many thanks,
}
} Dr. Sally Leys
} Assistant Professor and Canada Research Chair
} in Evolutionary Developmental Biology
} Department of Biological Sciences CW 405
} The University of Alberta
} Edmonton, Alberta
} Canada
} T6G 2E9
}
} Telephone: (780) 492-6629
} Fax: (780) 492-9234
} Email: sleys-at-ualberta.ca

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 12:21:22 2004

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The previous responders have made mostly made good points, but have neglected one important possibility. Zeiss planapo lenses of that era are of high optical quality, but unfortunately they frequently suffer from a separation of lens elements known as delamination, caused by a failure of the lens cement. Used objectives also frequently have dust or a deposit of fine, misty oil droplets on the surface of the back lens. If you have a "phase telescope" you should focus through the objective and look for contamination, or delamination, which may appear as gray patches or show interference colors, and usually start at the edges and work their way inward. You can also use a dissecting microscope to look through the objective (put a light source in front of the objective and look through the back).

Either contamination or delamination will cause a haziness of the image, which will be reduced with stopping down of the condenser, explaining why the best image is seen when the condenser is stopped down past it's theoretical optimal position. Stopping down also causes dirt or other artifacts in the optical path to become much more noticeable. If you can't locate the points of contamination with the phase telescope, try rotating the objective to see if the artifacts move with it. Haze, dirt, and delamination may also be present in the condenser. Most used objectives and condensers I have come across were in need of a good cleaning.

If you want to use your 100x planapo or any other oil lens, not using oil between the specimen and the objective is not an option. With my Zeiss microscope and 1.4 NA condenser, oiling the condenser noticeable improves the contrast as well as resolution. As others have said, you should definitely not oil your 0.9 NA condenser. Also be aware that different types of immersion oil should never be allowed to mix, and that some types of oil can damage the mounting cement of some brands of lenses. Using Zeiss immersion oil with some Nikon lenses, for example, can be disastrous.

Ralph Common
Electron Microscopist
Michigan State University
Division of Human Pathology
A608 East Fee Hall
East Lansing, MI 48824
517-355-7558; fax 517-432-1053
ralph.common-at-ht.msu.edu

-----Original Message-----
} From: Bruce Girrell [mailto:bigirrell-at-microlinetc.com]
Sent: Thursday, February 26, 2004 5:08 PM
To: Microscopy-at-msa.microscopy.com

I have a binocular Zeiss phase contrast microscope that came with a basic
assortment of lenses. A while back I bought a planapo 10/0.32 lens
(standard - no phase ring) and was stunned at the quality of the image. To
describe the image as "sharp" or even "crisp" doesn't do it justice. Some
stained thin sections have the appearance of stained glass and the image
almost takes on a three dimensional quality. I was impressed.

Recently, I was able to acquire a planapo 100/1.3 Ph3. Despite its very
impressive appearance, I have been much less impressed with the image
produced by this lens. Granted, the contrast is better than the standard
lens, but based on the difference I had seen at 10x I was expecting a little
more in the sharpness department.

Bear in mind that I fall in the "hobbyist" ranks. Some of these questions
are basic. I have set up Kohler illumination. I believe that I have the
phase rings aligned. Most of these questions apply to brightfield
observation anyway.

Questions:
1) Am I simply expecting too much at 1000x?
2) Is the phase ring degrading the performance?
3) My condenser only has an n.a. of 0.9. Is this the problem?
4) Even with this condenser, should I be using oil on it as well as the
objective?
5) With the phase stop in place performance is worse - lots of artifacts.
That is not the case with the 40x and 10x phase objectives.

One more general question:
Literature tells me that I should achieve optimum contrast/resolution with
the brightfield aperture closed about 1/3 of the way. I seem to get the best
results with the aperture closed just a little over half way. Am I not
sensitive enough to artifacts and confusing increased contrast for increased
resolution? Am I maybe using too much light?

Thanks for your help,

Bruce Girrell

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 13:23:26 2004

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Greetings:

This is a question about TEM objective apertures, mostly about thickness
and selection of hole size.

We have a JEOL 1200, I wanted to replace the objective aperture, old one
was not cleaning up well. Ordered one from EM supplier we get most
everything else from. Picked one that was for JEOL, a Pt strip .1 mm thick,
three holes, 50, 100, 150. Sounded perfect.

Tried to put it in yesterday. Way too thick. Aperture holder accepts the
strip by slipping it in a fixed sandwich kind of space, not with a separate
screw down holder over the top. Old aperture was way thinner than the new
one, even though new one was called 'thin'.

Checked all the other catalogs I have, most had apertures with the same
dimensions. Don't have much experience with this so I am hoping to be
educated.

Are the apertures for this instrument something special? Where do I get an
aperture to fit? Is JEOL the only source? What criteria do I use to select
the hole size? etc.

Help me out on this one.

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 13:38:11 2004

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First of all, Au lines will overlap with P, so in this
case coating with Au is not acceptable.

Then I am not sure about a goal of your research.
If you need just to determine whether Fe and P are in
your samples, then EDS is not the best choice of method.
Depending on anticipated levels of elements the XRF,
wet chemistry or even mass spectrometry could be a better
choice.

If detection limit of 0.5% is OK, then I would use
high intensity beam current (so that dead time is about
20-50%)to acquire spectrum from pretty big field of view,
at magnification of x100 or x200, for at least 5 min.
Sometimes fast mapping (again at high beam current and at
magnifications when many particles are visible) can
help to localize the place of interest.

Regards,

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

} Hello fellow Microscopists,
}
} How can we best prepare our soil samples for SEM and micro
} analysis? We are novices at this. We have great equipment
} (Hitachi FESEM 4500 and EDAX Genesis) We are interested in
} phosphorus and iron in river sediments. We are having
} difficulty in interpreting the results we have been getting
} (we crushed soil to double sticky tape, mounted on Al stubs
} and coated with AuPd). The preps look good at the SEM with
} little charging.
}
} What we see is grains and some organic matter (OM) and
} coatings. The spectrum shows some OM and SiO2 along with
} other particles of mixed composition.
}
} My question is how can we interpret this? What about
} references etc? We need your expertise!
}
} Your help will be greatly appreciated.
} Carol Bronick
}
} Agricultural Research Station
} Box 9061
} Virginia State University
} Petersburg, VA 23806
} 804.524.6822
} cbronick-at-vsu.edu
}
} ____________________________________________________________________
} Check your SchoolEmail at http://www.CampusI.com
} Find the LOWEST PRICES on books at http://www.campusi.com/BookFind !
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 14:05:24 2004

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From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 14:16:18 2004

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Why don't you use JEOL spares as your first choice?

At least you then know that they will fit and work.

Down here, at least, JEOL parts are not exhorbitantly expensive.

cheers

rtch (a satisfied customer of JEOL Sydney)

Date sent: Wed, 3 Mar 2004 11:17:01 -0800
To: Microscopy-at-sparc5.microscopy.com
} From: jmkrupp-at-cats.ucsc.edu (Jon Krupp)

Jonathan
I do believe, the apertures in JEM1200 are made from molybdenum (or
tungsten?), definitely not a Pt. Perhaps you have to contact JEOL for
specification (they are quite friendly). Personally, I would avoid "after
market" spare parts especially objective apertures (they are designed in
the way they are actually self-cleaning under the beam). Aperture in my
microscope is "in" for more than 5 years and I never cleaned it. Deposits
on the objective aperture usually indicates problem with vacuum. You may
easily clean original JEOL aperture by heating up in tantalum or tungsten
boat in good vacuum (5x10-6 torr or better) for a minute or less. It
cleans everything. The problem there is that it's possible to damage the
hole itself (well, it means, it's time to buy new one) if overheat. It's
important, the boat made from different material than aperture, otherwise,
the strip will stick to the boat. I am using 25-50-100 um objective
aperture strip. In 95% cases we are using 50um spot - it provides enough
light with decent contrast. I am using 25um spot (not recommended to use
with plastic sections!) for very weak W shadowed samples only . I never
used 100 um. I hope it helps. Sergey

At 11:17 AM 3/3/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 15:36:57 2004

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Actually, P K alpha and Au M alpha don't overlap but
are indeed very close by 108eV. Pt might be an option
but its M alpha is even closer to the P K alpha.
The 108eV distance at low eV is not always a
problem with Genesis. The EDAX HPD feature is
very powerful for deconvoluting peaks. A quant
with low intensity errors will give very good
results. Any element that has high (} 20%) intensity
error should be discarded or re-run at different KV.

At F, my detector is about 56-59eV (give or take) resolution
and how one calculates this. Calibrated rez at Al
and Cu is typically 128eV at 102uS. No spec wars please.

Potting the soil in metallurgical mounting media
then polishing should provide good results.
The irregularity of un-polished (3-D) soil grains
is not good for EDS. Flat, polished surfaces are
best.

Collect at 102uS with at least 1,000cps and do it
for about 300 live seconds. Keep DT { 25%. Then
do peak ID, HPD and finally, quant and look at the
Inten. Error values.

I look at C, F, O, P, Al, Si, Fe, S, Cu, W, Ta, Hf, Zr,
and many others (not all at the same time!!) that
are Au/Pd coated. At 2X KV of highest value, I can't
recall a time that I could not define the constituents
with EDAX EDS. Organics/polymers are another story--
need FTIR or WDS for that.

gary g.

At 11:51 AM 3/3/2004, Dusevich, Vladimir wrote:

} First of all, Au lines will overlap with P, so in this
} case coating with Au is not acceptable.
}
} Then I am not sure about a goal of your research.
} If you need just to determine whether Fe and P are in
} your samples, then EDS is not the best choice of method.
} Depending on anticipated levels of elements the XRF,
} wet chemistry or even mass spectrometry could be a better
} choice.
}
} If detection limit of 0.5% is OK, then I would use
} high intensity beam current (so that dead time is about
} 20-50%)to acquire spectrum from pretty big field of view,
} at magnification of x100 or x200, for at least 5 min.
} Sometimes fast mapping (again at high beam current and at
} magnifications when many particles are visible) can
} help to localize the place of interest.
}
} Regards,
}
} Vladimir
}
}
} Vladimir M. Dusevich, Ph.D.
} Electron Microscope Lab Manager
} 3127 School of Dentistry
} 650 E. 25th Street
} Kansas City, MO 64108-2784
}
} Phone: (816) 235-2072
} Fax: (816) 235-5524
} Web: http://www.umkc.edu/dentistry/microscopy
}
}
} } Hello fellow Microscopists,
} }
} } How can we best prepare our soil samples for SEM and micro
} } analysis? We are novices at this. We have great equipment
} } (Hitachi FESEM 4500 and EDAX Genesis) We are interested in
} } phosphorus and iron in river sediments. We are having
} } difficulty in interpreting the results we have been getting
} } (we crushed soil to double sticky tape, mounted on Al stubs
} } and coated with AuPd). The preps look good at the SEM with
} } little charging.
} }
} } What we see is grains and some organic matter (OM) and
} } coatings. The spectrum shows some OM and SiO2 along with
} } other particles of mixed composition.
} }
} } My question is how can we interpret this? What about
} } references etc? We need your expertise!
} }
} } Your help will be greatly appreciated.
} } Carol Bronick
} }
} } Agricultural Research Station
} } Box 9061
} } Virginia State University
} } Petersburg, VA 23806
} } 804.524.6822
} } cbronick-at-vsu.edu
} }
} } ____________________________________________________________________
} } Check your SchoolEmail at http://www.CampusI.com
} } Find the LOWEST PRICES on books at http://www.campusi.com/BookFind !
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 15:39:14 2004

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In response to Sergey and Jonathan's questions let me say this: Ladd, as
most people know, produces probably 97% of all apertures made in the U.S.
We customize apertures for all microscopes to fit the user's needs. For
instance in Sergey's case, he could have two or even three 50um holes if he
wanted. The "after market" apertures offer you this customization
opportunity. We can machine in various materials, such as moly, platinum,
etc. and provide strips or discs as thin as 0.025mm.

Generally, apertures in the "after market" are quite a bit less expensive,
more readily available and, as I mentioned, can be customized to meet your
needs. We put as many as 20 holes in some plates and strips for specialized
equipment.

As a matter of fact most apertures are "after market" because EM
manufacturers tend not to produce their own apertures. I am not impartial
on this matter, but for flexibility and value the "after market" is the
place to look for apertures.

Disclaimer: Ladd Research sells EM supplies including apertures and
specialized micro-holes to EM users and microscope manufacturers.

John Arnott

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com
----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
To: {Microscopy-at-sparc5.microscopy.com}
Sent: Wednesday, March 03, 2004 3:56 PM

John
I LOVE "after market" especially if it provides CHEAP solution. I also
like your point on customization (which, perhaps, will be more
expensive...). From another hand Jonathan's message shows the reality: he
bought "after market" aperture (I would think he did specify, which
aperture he needs), which does not fit... As I told in my original
message, aperture on JEM1200 survived for many years and it was cost to me
something like $100 from JEOL. How much I could save on "after market"?
$30 perhaps or even less? To me it would be probably easier to get stuff
from guaranteed source (JEOL) rather than spent time looking for aperture,
which will "fit"... Sergey

At 01:52 PM 3/3/2004, you wrote:
} In response to Sergey and Jonathan's questions let me say this: Ladd, as
} most people know, produces probably 97% of all apertures made in the U.S.
} We customize apertures for all microscopes to fit the user's needs. For
} instance in Sergey's case, he could have two or even three 50um holes if he
} wanted. The "after market" apertures offer you this customization
} opportunity. We can machine in various materials, such as moly, platinum,
} etc. and provide strips or discs as thin as 0.025mm.
}
} Generally, apertures in the "after market" are quite a bit less expensive,
} more readily available and, as I mentioned, can be customized to meet your
} needs. We put as many as 20 holes in some plates and strips for specialized
} equipment.
}
} As a matter of fact most apertures are "after market" because EM
} manufacturers tend not to produce their own apertures. I am not impartial
} on this matter, but for flexibility and value the "after market" is the
} place to look for apertures.
}
} Disclaimer: Ladd Research sells EM supplies including apertures and
} specialized micro-holes to EM users and microscope manufacturers.
}
} John Arnott
}
} Ladd Research
} 83 Holly Court
} Williston, VT 05495
}
} On-line Catalog: http://www.laddresearch.com
}
} tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
} fax: 1-802-660-8859
} e-mail: sales-at-laddresearch.com
} ----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
} To: {Microscopy-at-sparc5.microscopy.com}
} Sent: Wednesday, March 03, 2004 3:56 PM
} Subject: [Microscopy] Re: TEM apertures
}
}
} }
} }
} } --------------------------------------------------------------------------
} ----
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------------
} -----
} }
} } Jonathan
} } I do believe, the apertures in JEM1200 are made from molybdenum (or
} } tungsten?), definitely not a Pt. Perhaps you have to contact JEOL for
} } specification (they are quite friendly). Personally, I would avoid "after
} } market" spare parts especially objective apertures (they are designed in
} } the way they are actually self-cleaning under the beam). Aperture in my
} } microscope is "in" for more than 5 years and I never cleaned it. Deposits
} } on the objective aperture usually indicates problem with vacuum. You may
} } easily clean original JEOL aperture by heating up in tantalum or tungsten
} } boat in good vacuum (5x10-6 torr or better) for a minute or less. It
} } cleans everything. The problem there is that it's possible to damage the
} } hole itself (well, it means, it's time to buy new one) if overheat. It's
} } important, the boat made from different material than aperture, otherwise,
} } the strip will stick to the boat. I am using 25-50-100 um objective
} } aperture strip. In 95% cases we are using 50um spot - it provides enough
} } light with decent contrast. I am using 25um spot (not recommended to use
} } with plastic sections!) for very weak W shadowed samples only . I never
} } used 100 um. I hope it helps. Sergey
} }
} } At 11:17 AM 3/3/2004, you wrote:
} }
} }
} }
} } ---------------------------------------------------------------------------
} ---
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} } ---------------------------------------------------------------------------
} ----
} } }
} } } Greetings:
} } }
} } } This is a question about TEM objective apertures, mostly about thickness
} } } and selection of hole size.
} } }
} } } We have a JEOL 1200, I wanted to replace the objective aperture, old one
} } } was not cleaning up well. Ordered one from EM supplier we get most
} } } everything else from. Picked one that was for JEOL, a Pt strip .1 mm
} thick,
} } } three holes, 50, 100, 150. Sounded perfect.
} } }
} } } Tried to put it in yesterday. Way too thick. Aperture holder accepts the
} } } strip by slipping it in a fixed sandwich kind of space, not with a
} separate
} } } screw down holder over the top. Old aperture was way thinner than the new
} } } one, even though new one was called 'thin'.
} } }
} } } Checked all the other catalogs I have, most had apertures with the same
} } } dimensions. Don't have much experience with this so I am hoping to be
} } } educated.
} } }
} } } Are the apertures for this instrument something special? Where do I get
} an
} } } aperture to fit? Is JEOL the only source? What criteria do I use to
} select
} } } the hole size? etc.
} } }
} } } Help me out on this one.
} } }
} } } Thanks
} } }
} } } Jonathan Krupp
} } } Microscopy & Imaging Lab
} } } University of California
} } } Santa Cruz, CA 95064
} } } (831) 459-2477
} } } jmkrupp-at-cats.ucsc.edu
} }
} } _____________________________________
} }
} } Sergey Ryazantsev Ph. D.
} } Electron Microscopy
} } UCLA School of Medicine
} } Department of Biological Chemistry
} } 10833 Le Conte Ave, Room 33-089
} } Los Angeles, CA 90095
} }
} } Phone: (310) 825-1144 (office)
} } (310) 206-1029 (Lab)
} } FAX (departmental): (310) 206-5272
} } mailto:sryazant-at-ucla.edu
} }
} }
} }
} }

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 3 20:20:51 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jvonreis-at-columbiabasin.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, March 3, 2004 at 11:20:34
---------------------------------------------------------------------------

Email: jvonreis-at-columbiabasin.edu
Name: Jennifer von Reis

Organization: Columbia Basin College

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have information on how to use hexamethyldisilazene (HMDS) instead of a critical point drier to prepare specimens, that have been fixed and dehydrated in alcohol, for SEM observation?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 00:16:16 2004

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Dear Carol

We have done quite a bit so far. Most investigations were done on on sidiments ranging between 1m below the surface up to rocks at ~100 m Below the surface. My preference is still to mount in Araldite (the cheap version you can get from fiberglass hobby shops) under vacuum to get rid of trapped gas and polish to 1 micron surface finish. Do not crush. You losse info like pore density and distibution/relationship of the different components. Weathering is more clear in a cross section. Most of the investigation is in BSE mode. Carbon coating is preferred since it interfere less with the EDS spectrum. If you can work in Low Vacuum range (0.1 torr - 1 torr) it helps with reducing charging.

A reasonable refernce is (more suitable to rocks) is "Bachscattred Scanning
Electron Microscopy and Image analysis of Sediments and Sedimentary Rocks"
by D. H. Kringsly and other authers. Cambridge press ISBN 0-521-45346-1

Hope this helps

-----Original Message-----
} From: cbronick-at-vsu.edu [mailto:cbronick-at-vsu.edu]
Sent: Wed 3/3/2004 5:21 PM
To: Microscopy-at-MSA.Microscopy.Com
Cc:

Hello fellow Microscopists,

How can we best prepare our soil samples for SEM and micro analysis? We are novices at this. We have great equipment (Hitachi FESEM 4500 and EDAX Genesis) We are interested in phosphorus and iron in river sediments. We are having difficulty in interpreting the results we have been getting (we crushed soil to double sticky tape, mounted on Al stubs and coated with AuPd). The preps look good at the SEM with little charging.

What we see is grains and some organic matter (OM) and coatings. The spectrum shows some OM and SiO2 along with other particles of mixed composition.

My question is how can we interpret this? What about references etc? We need your expertise!

Your help will be greatly appreciated.
Carol Bronick

Agricultural Research Station
Box 9061
Virginia State University
Petersburg, VA 23806
804.524.6822
cbronick-at-vsu.edu

____________________________________________________________________
Check your SchoolEmail at http://www.CampusI.com
Find the LOWEST PRICES on books at http://www.campusi.com/BookFind !

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 00:25:17 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1a ] --

Jennifer von Reis wrote:
==================================================================
Question: Does anyone have information on how to use hexamethyldisilazene
(HMDS) instead of a critical point drier to prepare specimens, that have
been fixed and dehydrated in alcohol, for SEM observation?
==================================================================
A good overview on this topic was published in MICROSCOPY TODAY, May 1997 by
Phil Oshel. It has been republished on the SPI Supplies website with
permission at URL
http://www.2spi.com/catalog/chem/hmds.html

Disclaimer: SPI Supplies is a supplier of HMDS used in electron microscopy
applications.

Chuck

============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 00:49:29 2004

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Sergey;
Best way to clean apertures is with a dual beam FIB. That way,
you can cut away any dirt, burs, eccentricity, and inspect with the SEM
while you are in there!

John Mardinly
Intel

-----Original Message-----
} From: Sergey Ryazantsev [mailto:sryazant-at-ucla.edu]
Sent: Wednesday, March 03, 2004 12:57 PM
To: Microscopy-at-sparc5.microscopy.com

Jonathan
I do believe, the apertures in JEM1200 are made from molybdenum (or
tungsten?), definitely not a Pt. Perhaps you have to contact JEOL for
specification (they are quite friendly). Personally, I would avoid
"after
market" spare parts especially objective apertures (they are designed in

the way they are actually self-cleaning under the beam). Aperture in my

microscope is "in" for more than 5 years and I never cleaned it.
Deposits
on the objective aperture usually indicates problem with vacuum. You
may
easily clean original JEOL aperture by heating up in tantalum or
tungsten
boat in good vacuum (5x10-6 torr or better) for a minute or less. It
cleans everything. The problem there is that it's possible to damage
the
hole itself (well, it means, it's time to buy new one) if overheat.
It's
important, the boat made from different material than aperture,
otherwise,
the strip will stick to the boat. I am using 25-50-100 um objective
aperture strip. In 95% cases we are using 50um spot - it provides enough

light with decent contrast. I am using 25um spot (not recommended to
use
with plastic sections!) for very weak W shadowed samples only . I never

used 100 um. I hope it helps. Sergey

At 11:17 AM 3/3/2004, you wrote:

} -----------------------------------------------------------------------
-------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 04:32:48 2004

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A lot of thanks for the information!
I am sure that I will contact with you. Thank you
--
*************************************************************
Dra. María Belén López Mosquera
Unidade de Microscopía
Servicios Xerais de Apoio á Investigación
Universidade da Coruńa
Edificio Servicios Centrais de Investigación
Campus de Elvińa s/n
E-15071 A Coruńa

Teléfono: 34 981 167 000 ext.: 2087
Telecopia: 34 981 167 068
Correo eléctrónico: sxaimic-at-udc.es
**************************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 07:10:04 2004

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O.k., folks I know a number of you are still using TEM film as we are. And
due to the pricing of the 250 sheet boxes vs. the 100 sheet boxes you're
buying the 250 sheet boxes. Great deal on film cost but the lousy plastic
boxes aren't much use.

Those little yellow kodak (or white Ilford) 100 sheet film boxes are great for lots
of things but we've been using them for transporting exposed film from the
scope rooms to the dark room for processing. I assume that other folks have
been doing the same since I've come across this practice at every TEM lab
I've ever worked at. But since we've been buying the plastic 250 sheet boxes
our supply of the yellow cardboard boxes has been dwindling slowly. SO now
the quesiton is what do we replace the 100 sheet cardboard boxes with? Has
anyone found the answer yet?

The $40 price premium for buying 100 sheet boxes of film is a bit much for
replacing the cardboard boxes withy new cardboard boxes.

The $20K and upwards price for a CCD camera to move to digital is also a bit
much.

So before I have my shop folks here make me up some replacment metal
boxes, are there any other suggestions out there?

Any of the TEM FIlm vendors out there willing to sell expired 100 sheet film
really cheap? (You can even keep the film!)

Thanks.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 08:15:31 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (R.H.Olley-at-reading.ac.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, March 4, 2004 at 03:53:49
---------------------------------------------------------------------------

Email: R.H.Olley-at-reading.ac.uk
Name: Robert H. Olley

Title-Subject: [Microscopy] [Filtered] TEM of Polymers

Question: In answer to the question from Dra. Maria BelČn LŰpez Mosquera:

One way of looking at polymers, especially hydrocarbon polymers like polypropylene and polyethylene, is to prepare a surface and etch with a permanganic reagent. The etched surface is then either:
- replicated and the replica examined under TEM;
- gold coated and examined under SEM.

It is very easy to distinguish polyethylene and polypropylene this way.

We have a picture gallery of etched surfaces, albeit for specimens with special thermal or mechanical treatment, on:

http://www.personal.rdg.ac.uk/~spsolley/Picture_Gallery/new_pgal.html

-----------------------------------
Robert H. Olley
Reply to: R.H.Olley-at-reading.ac.uk
URL: http://www.personal.rdg.ac.uk/~spsolley
-----------------------------------

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From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 08:31:43 2004

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Boxes that hold 4x5 sheet film work well, although the film slides
around a bit. If you know someone who uses a 4x5 camera, you're set. If
not, try your local pro film processing lab for empty boxes.

Geoff

Richard Edelmann wrote:

} O.k., folks I know a number of you are still using TEM film as we are. And due to the pricing of the 250 sheet boxes vs. the 100 sheet boxes you're buying the 250 sheet boxes. Great deal on film cost but the lousy plastic boxes aren't much use.
}
} Those little yellow kodak (or white Ilford) 100 sheet film boxes are great for lots of things but we've been using them for transporting exposed film from the scope rooms to the dark room for processing. I assume that other folks have been doing the same since I've come across this practice at every TEM lab I've ever worked at. But since we've been buying the plastic 250 sheet boxes our supply of the yellow cardboard boxes has been dwindling slowly. SO now the quesiton is what do we replace the 100 sheet cardboard boxes with? Has anyone found the answer yet?
}
} The $40 price premium for buying 100 sheet boxes of film is a bit much for replacing the cardboard boxes withy new cardboard boxes.
}
} The $20K and upwards price for a CCD camera to move to digital is also a bit much.
}
} So before I have my shop folks here make me up some replacment metal
} boxes, are there any other suggestions out there?
}
} Any of the TEM FIlm vendors out there willing to sell expired 100 sheet film really cheap? (You can even keep the film!)
}
} Thanks.
}
}
} Richard E. Edelmann, Ph.D.
} Electron Microscopy Facility Supervisor
} 350 Pearson Hall
} Miami University, Oxford, OH 45056
} Ph: 513.529.5712 Fax: 513.529.4243
} E-mail: edelmare-at-muohio.edu
} http://www.emf.muohio.edu
}
} "RAM disk is NOT an installation procedure."
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
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From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 08:42:16 2004

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I was going to reply, but Chuck already did, sort of. There's also
the U. of Florida EM web site "Tips and Tricks":
http://www.biotech.ufl.edu/EM/tips/index.html search on
How you do the procedure depends a lot on your samples. What are they?
Phil

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Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 08:56:07 2004

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I have been using the (same) black cardboard box system for some time for
transporting film to darkroom! Looks like I will hold onto it. Sorry I don't
have any extras; they are in use throughout the lab.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOHIO.EDU]
Sent: Thursday, March 04, 2004 8:23 AM
To: microscopy-at-MSA.Microscopy.com

O.k., folks I know a number of you are still using TEM film as we are.
And
due to the pricing of the 250 sheet boxes vs. the 100 sheet boxes you're
buying the 250 sheet boxes. Great deal on film cost but the lousy plastic
boxes aren't much use.

Those little yellow kodak (or white Ilford) 100 sheet film boxes are great for
lots
of things but we've been using them for transporting exposed film from the
scope rooms to the dark room for processing. I assume that other folks have
been doing the same since I've come across this practice at every TEM lab
I've ever worked at. But since we've been buying the plastic 250 sheet boxes
our supply of the yellow cardboard boxes has been dwindling slowly. SO now
the quesiton is what do we replace the 100 sheet cardboard boxes with? Has
anyone found the answer yet?

The $40 price premium for buying 100 sheet boxes of film is a bit much for
replacing the cardboard boxes withy new cardboard boxes.

The $20K and upwards price for a CCD camera to move to digital is also a bit
much.

So before I have my shop folks here make me up some replacment metal
boxes, are there any other suggestions out there?

Any of the TEM FIlm vendors out there willing to sell expired 100 sheet film
really cheap? (You can even keep the film!)

Thanks.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 09:22:36 2004

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Hello: We have a Reichert-Jung FC4D cryo attachement and are having a
problem with some the heaters. We are trying to get through to someone at
Leica to help with some questions but in the meantime I was hoping someone
might have the name etc of a person we could contact for help. Any help is
greatly appreciated because as usual this thing failed just as I have a
large backlog of cryo samples. Thanks in advance. Steve

Stephen McCartney
Research Associate
Materials Research Institute
2108 Hahn Hall
Va Tech
Blacksburg, VA 24061
540-231-9765 - phone
540-231-8517 - FAX

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 09:31:38 2004

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Richard,

Just check with ANY Photographic/darkroom supply place. Look for
something called a Paper Safe. They come in a variety of sizes and range
in price from about $13(for 8x10 size that holds about 100 sheets) to
around $75(for a DELUXE version). Serve same function as cardboard
boxes....just more durable since they are usually made out of ABS plastic
See this website for an example(picture) of a Paper Safe ===}
http://www.freestylephoto.biz/sc_prod.php?cat_id=1603&pid=1526

Kelly A. Ramos
Metallurgical Engineer / Supervisor
Argo-Tech Materials Laboratories
23555 Euclid Avenue
Cleveland, OH 44117
216-692-5904 or 216-692-5446
(fax) 216-692-5816
http://www.atclabs.com

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 09:42:40 2004

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When I bought my TEM 12 years ago, it came with two tin cans. The can
look very much like a ordinary can except that the inside of lid has a
piece of 10 mm black foam. There is a gap between the side of lid and
the foam. It is light tight when the closed.

I think a candy/cooky can of proper size and a piece of black foam
inside the lid will do the job.

Ann Fook

} } } "Sherwood, Margaret " {MSHERWOOD-at-PARTNERS.ORG} 03/04/04 10:03AM
} } }

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I have been using the (same) black cardboard box system for some time
for
transporting film to darkroom! Looks like I will hold onto it. Sorry
I don't
have any extras; they are in use throughout the lab.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOHIO.EDU]
Sent: Thursday, March 04, 2004 8:23 AM
To: microscopy-at-MSA.Microscopy.com

O.k., folks I know a number of you are still using TEM film as
we are.
And
due to the pricing of the 250 sheet boxes vs. the 100 sheet boxes
you're
buying the 250 sheet boxes. Great deal on film cost but the lousy
plastic
boxes aren't much use.

Those little yellow kodak (or white Ilford) 100 sheet film boxes are
great for
lots
of things but we've been using them for transporting exposed film from
the
scope rooms to the dark room for processing. I assume that other folks
have
been doing the same since I've come across this practice at every TEM
lab
I've ever worked at. But since we've been buying the plastic 250 sheet
boxes
our supply of the yellow cardboard boxes has been dwindling slowly. SO
now
the quesiton is what do we replace the 100 sheet cardboard boxes with?
Has
anyone found the answer yet?

The $40 price premium for buying 100 sheet boxes of film is a bit much
for
replacing the cardboard boxes withy new cardboard boxes.

The $20K and upwards price for a CCD camera to move to digital is also
a bit
much.

So before I have my shop folks here make me up some replacment metal
boxes, are there any other suggestions out there?

Any of the TEM FIlm vendors out there willing to sell expired 100 sheet
film
really cheap? (You can even keep the film!)

Thanks.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 10:27:48 2004

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Dear Richard,
My TEM puts the exposed film into a box in the camera, but we found out the hard
way that it wasn't quite light tight. I wrap the box in the black plastic bag
that the photo paper comes in. These bags work for all types of light-tight
transport.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Richard Edelmann" {edelmare-at-MUOHIO.EDU}
To: {microscopy-at-MSA.Microscopy.com}
Sent: Thursday, March 04, 2004 5:23 AM

Hi,
I need to purchase a number of Philips 6V 10W bayonet style,
single contact bulbs for use in the illuminator boxes from Ernst
Leitz GMBH Wetzlar transformer housing assemblies. The bulb part
number appears to be 6814. Another number that appears on the bulb
is k15679. The transformer/bulb housing assemblies are model #
307-127.002.
I've searched light bulb web sites and I've tried our local
microscope sales rep, no luck on either front. Can anyone out there
help?

TIA
Mike
--
********************************************************************
Michael M. Cheatham
312 Heroy Geology Laboratory Phone (315)-443-1261
Syracuse University Fax (315)-443-3363
Syracuse, NY 13244-1070

email:mmcheath-at-mailbox.syr.edu
http://www.geochemistry.syr.edu/cheatham/InstrPages.html

owner of PLASMACHEM-L: http://listserv.syr.edu/archives/plasmachem-l.html
owner of XRF-L: http://listserv.syr.edu/archives/xrf-l.html
owner of TIMS-L: http://listserv.syr.edu/archives/tims-l.html
owner of SIRIS-L: http://listserv.syr.edu/archives/siris-l.html
********************************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 14:39:06 2004

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Mike:

You may want to try Don's Bulbs. They have a locating service that you
can access here:

http://www.donsbulbs.com/cgi-bin/r/t.pl/bulblocatingservice.html

I hope this helps.

DISCLAIMER: I have no financial or other interest in the reference
quoted above.

Best regards-

David

--
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Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

Michael Cheatham wrote:

}
}
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} -------------------------------------------------------------------------------
}
}
} Hi,
} I need to purchase a number of Philips 6V 10W bayonet style,
} single contact bulbs for use in the illuminator boxes from Ernst Leitz
} GMBH Wetzlar transformer housing assemblies. The bulb part number
} appears to be 6814. Another number that appears on the bulb is
} k15679. The transformer/bulb housing assemblies are model # 307-127.002.
} I've searched light bulb web sites and I've tried our local
} microscope sales rep, no luck on either front. Can anyone out there
} help?
}
} TIA
} Mike

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 16:40:21 2004

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Try
http://www.microlites.com/

Bob

On 4 Mar 2004, at 14:25, Michael Cheatham wrote:

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From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 17:52:12 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (nagashim-at-ncifcrf.gov) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Thursday, March 4, 2004 at 11:17:23
---------------------------------------------------------------------------

Email: nagashim-at-ncifcrf.gov
Name: Kunio Nagashima

Organization: NCI Frederick/SAIC Frederick

Education: Graduate College

Location: Frederick, Maryland

Question: I have a problem to mount thin-sections on a thin-bar hexagon grid. The sections do not adhere well and cause many wrinkles on section. There is a glue pen, but I want to know if I can buy solution so I can apply a drop on to grid and let it dry to have a better attachment on.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 4 19:26:35 2004

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Richard
I do find those plastic boxes quite useful to store the film. As for
transportation - I have vacuum desiccator with film set in the
dark-room. It's quite convenient: you don't need load-reload films. We
are using the rule: each magazine with film should be developed immediately
and re-loaded with new film. Nevertheless, for the last two years nobody
is willing to use film - we go digital all the time. So, I still keep
dark-room in the working order and pay salary to my technician... This is
our fate: each new technology adds load to your budget, not relieve.
Sergey

At 05:23 AM 3/4/2004, you wrote:

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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 09:03:44 2004

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My undergrad histology class has given me a new and novel problem. One of
the students is experiencing severe motion sickness while she views
specimens on a standard binocular compound microscope. I have had students
bothered when viewing specimens on the 6-headed scope and someone else is
moving the specimen field but this is a first. Any one have an easy
suggestion?

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 09:52:14 2004

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KUNIO-
The best way to get them flat is to make a convex water surface in
the boat. That makes the point of contact high where you bring the
grid down on the sections and makes the section spread uniformly
across the plastic film. It is impossible to prevent all the
wrinkles, but this method reduces them to a maneagable number or
frequency.
Carol

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--
__
Carol A. Heckman, Ph.D.
Professor of Biological Sciences
Director, Center for Microscopy & Microanalysis
Bowling Green State University, Bowling Green, OH 43403
fax: (419) 372-2024 email: heckman-at-bgnet.bgsu.edu
___________________________________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:13:08 2004

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Hmmm, I remember that I used to get sick while looking at some immunofluorescent
slides...I found that if I slowed down (instead of rapidly scanning the slides for
areas of interest) and took frequent breaks, I was OK. I would not have called it
"severe" motion sickness, though.

When I was on the multi-headed scope with several people and my boss "driving"
(i.e. changing magnification, focusing and moving the slide), I learned to
anticipate the changes and look away from the scope as the changes were being made.

Not sure if this helps-maybe if she took standard antimotion sickness medicine
before getting on the scope would help?

Good luck to you and her-
Kathleen Roberts
Principal Lab Technician
Neurotoxicology Labs
Dept of Pharmacology and Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

Tom Phillips wrote:

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} My undergrad histology class has given me a new and novel problem. One of
} the students is experiencing severe motion sickness while she views
} specimens on a standard binocular compound microscope. I have had students
} bothered when viewing specimens on the 6-headed scope and someone else is
} moving the specimen field but this is a first. Any one have an easy
} suggestion?
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:17:03 2004

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Hi Dr. Phillips,

I think the easiest, though certainly not the cheapest, solution would be
to get either a digital or even a simple video camera mounted on the
microscope, then project the live image onto a large monitor or screen. I
would bet that with the student's field of view not restricted by looking
into eyepieces, the feeling would be greatly reduced. If you coupled this
with some type of image capture ability, then you would have the added
benefit of being able to provide the students with digital micrographs
from their actual session.

Good luck!

David

David Bell
Scientist
Electron Microscopy Lab
Millipore Corporation
80 Ashby Road
Bedford, MA 01730
(781) 533-2108

Tom Phillips {phillipst-at-missouri.edu}
03/05/2004 10:16 AM

To: Microscopy-at-msa.microscopy.com
cc:
Subject: [Microscopy] motion sickness on LM?

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My undergrad histology class has given me a new and novel problem. One of

the students is experiencing severe motion sickness while she views
specimens on a standard binocular compound microscope. I have had students

bothered when viewing specimens on the 6-headed scope and someone else is
moving the specimen field but this is a first. Any one have an easy
suggestion?

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:20:44 2004

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Tom,
My college room mate had that same problem when she was taking
Embryology and had to scan slides to find structures. Her way of
coping was to take a does of Dramamine about 1/2 hour before her lab
class.
I had a similar problem, but at the TEM, when I was pregnant.
Obviously, a pharmacological solution was out of the question. I
found that I could cope with it if I moved the image slowly, glanced
away briefly and took a few slow, deep breaths.
Your student should make sure that she takes the time to fully adjust
the binocular head to her individual needs...set up each eyepiece at
focus, so that she can relax her vision. As someone stated last week
on this site...she should look THROUGH the microscope, not AT or IN
it.
That's my 2 cents worth,
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:31:56 2004

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I'm basing this reply based on explanations and advice
from my MD in relation to my own problems with more
traditional causes of motion sickness. This is a
mixture of the "technical" terms I remember, and the
practical explanations that went with them. My doctor
is really kind of neat that way.

The basic cause for most motion sickness is a
difference in "inputs" from the eyes and the innter
ears. In the case of binocular microscopes, both eyes
are seeing a moving field, and the ears are saying
"we're not moving" and the brain is getting confused.
It responds by trying to "cancel out" the stationary
input from the ears (vision has priority), and you get
dizzy, upset stomache....

This type of case is kind of the inverse of normal
motion sickness, where the ears sense movement, but
the eyes are not because the surroundings (boat, car
interior) are stationary "relative" to the person. (A
"special" case of the theory of relativity.)

What the victim needs to do, is take steps to keep the
visual stimulus and the inner ear stimulus "in sync".
I hate to say it, but she is concentrating too hard on
the view in the mircroscope. The user needs to take
more frequent and/or longer looks away from the
microscope. Looking around the room, and not just at
the table may also help. She may also need to get up
and walk a little once in a while. Having identified
this as a problem for the individual, it is important
that she take these steps throughout the session, from
the start, not just when she starts feeling poorly.
By then it is too late, and brain is starting the
process of fighting the confilicting input stimula.
It will be an uphill battle to reign things back in.

Another option that may help would be to only use one
occular for most viewing, and keep the unused eye
open, and looking at something stationary. Those who
have used single occular microscopes know that this is
not a natural thing to do (at least for the untrained)
but it may help balance the stimula.

Different folks react differently to the problem, and
need to find a "personalized" solution. This is a
game the brain is playing, and it isn't happy about
having to do it. Once it starts, it can be difficult
to reverse, and an extended break might be the best
bet.

I hope this helps.

John W. Raffensperger, Jr.

--- Tom Phillips {phillipst-at-missouri.edu} wrote:
}
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} My undergrad histology class has given me a new and
} novel problem. One of
} the students is experiencing severe motion sickness
} while she views
} specimens on a standard binocular compound
} microscope. I have had students
} bothered when viewing specimens on the 6-headed
} scope and someone else is
} moving the specimen field but this is a first. Any
} one have an easy
} suggestion?
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:33:54 2004

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Hi Tom,

As one who suffers from serious motion sickness I can sympathize with your student.

I think the problem may lie in the oculars not being set up perfectly for her eyes. Another could be that she has sinus problems/inner ear issues and the positioning of her head may be causing imbalance to occur.

Try getting her to fit the oculars better. As we all have experienced when first using LM's not every one know how to optimally set those puppies up. Students are loath to fess up to this and will suffer in silence, or not in the case of your motion sick student.

How this helps,

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax
} } } Tom Phillips {phillipst-at-missouri.edu} 03/05/04 10:39 AM } } }

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My undergrad histology class has given me a new and novel problem. One of
the students is experiencing severe motion sickness while she views
specimens on a standard binocular compound microscope. I have had students
bothered when viewing specimens on the 6-headed scope and someone else is
moving the specimen field but this is a first. Any one have an easy
suggestion?

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:35:07 2004

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Thomas,
I do know from experience that this can occur when one is pregnant
and when the operator has an ear infection.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
}
} My undergrad histology class has given me a new and novel problem.
} One of the students is experiencing severe motion sickness while she
} views specimens on a standard binocular compound microscope. I have
} had students bothered when viewing specimens on the 6-headed scope
} and someone else is moving the specimen field but this is a first.
} Any one have an easy suggestion?
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 10:48:21 2004

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Could there be issues with UV light or ozone from a mercury or xenon lamphouse?

Alan Stone
ASTON

At 09:16 AM 3/5/2004, you wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 14:30:45 2004

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On Mar 5, 2004, at 7:16 AM, Tom Phillips wrote:

} My undergrad histology class has given me a new and novel problem.
} One of the students is experiencing severe motion sickness while she
} views specimens on a standard binocular compound microscope. I have
} had students bothered when viewing specimens on the 6-headed scope and
} someone else is moving the specimen field but this is a first. Any
} one have an easy suggestion?
}
On Mar 5, 2004, at 8:44 AM, John Raffensperger wrote:

} The basic cause for most motion sickness is a
} difference in "inputs" from the eyes and the innter
} ears. In the case of binocular microscopes, both eyes
} are seeing a moving field, and the ears are saying
} "we're not moving" and the brain is getting confused.

Dear Tom and John,
I am not an expert, but I understand that this input mismatch is
treated by the brain as a nervous system malfunction like those from
ingestion of a toxin, and that the response (motion sickness) has
evolved to eliminate the possible toxin--thus the nausea. If the
student is having difficulty fusing the two images, this could be
another source of input mismatch, so suggest that the student look only
with one eye and see if that reduces the problem. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 15:26:40 2004

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Postdoctoral scientist position
Biology Department, Brookhaven National Laboratory
Long Island, New York

The position requires a Ph.D. in biophysics, biochemistry, or related
field and a strong background in structural biology. Outstanding
candidates from physical sciences are also encouraged to apply. The
position involves structural study of macromolecular protein complexes
by cryo transmission electron microscopy. The ideal candidates should
have experience with electron microscopy and computer programming for
image process. Facilities include a Jeol 2010FasTEM, a Jeol1200EX, and
SGI workstations and a full biochemistry lab.

Interested candidates should send a CV and 3 references to hli-at-bnl.gov

--
Huilin Li
Brookhaven National Laboratory
Biology Dept. Bldg. 463
Upton, NY 11973
Email: hli-at-bnl.gov
phone: (631)344-2931 or (631)344-5066
fax: (631)344-3407
http://www.biology.bnl.gov/structure/li.html

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 15:31:31 2004

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Tom -

The simple solution is to see if she experiences the problem when using
only one eye. Monocular scopes work just fine - especially for those of us
that have a strongly dominant eye :-)

If you have a videomicroscope setup available, you might try that too.

Have you also considered the possibility that an odor is enhancing the
"motion sickness" effect? The few times I have experienced the problem I
have been in situations that normally wouldn't bother me - but someone had
on a strong perfume/aftershave or had used a vehicle "deodorizer" that was
strongly scented. She may be reacting to a combination of scent and sight.
If so, either removing the problem odor or having a small fan blow fresh
air past her face may help.

- Louise

Louise Harner
Research Microscopist
Albany International Research Co.
777 West Street, P.O. Box 9114
Mansfield, MA 02048
508-337-9529 phone
508-339-4996 fax
Louise_Harner-at-albint.com

= = =

Tom Phillips {phillipst-at-missouri.edu} 03/05/2004 10:16 AM

My undergrad histology class has given me a new and novel problem. One of
the students is experiencing severe motion sickness while she views
specimens on a standard binocular compound microscope. I have had students
bothered when viewing specimens on the 6-headed scope and someone else is
moving the specimen field but this is a first. Any one have an easy
suggestion?

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 16:09:42 2004

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I have advertised Kodak 4489 film on the surplus equipment listing and not
have received any inquiries. If you have a Zeiss 9 and need film and/or
film racks, please contact me off the listserver. I hate to through this
out, but it looks like I must in short order.

Thanks,
Ken
_______________________________________
Kenneth L. Tiekotter, Adjunct Professor
The University of Portland
Department of Biology
5000 N Willamette Blvd.
Portland, OR 97203 USA

Tel.: 503.943.8861

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 5 19:21:55 2004

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NOTICE: THE ZEISS 9s2 USES 7CM X 7CM SIZE FILM, NOT 8.3CM X 10.2CM FILM

I have advertised Kodak 4489 film on the surplus equipment listing and not
have received any inquiries. If you have a Zeiss 9 and need film and/or
film racks, please contact me off the listserver. I hate to throw this out,
but it looks like I must in short order.

Thanks,
Ken
_______________________________________
Kenneth L. Tiekotter, Adjunct Professor
The University of Portland
Department of Biology
5000 N Willamette Blvd.
Portland, OR 97203 USA

Tel.: 503.943.8861

From MicroscopyL-request-at-ns.microscopy.com Sun Mar 7 10:18:07 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (MBA2038-at-AOL.COM) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, March 7, 2004 at 10:02:25
---------------------------------------------------------------------------

Email: MBA2038-at-AOL.COM
Name: steve yutz

Organization: NONE

Title-Subject: [Microscopy] [Filtered] How much bench work time needs to finish 1kidney, 2 kidney and 3 kidney EM cases without scope from start to finish

Question: i would like to know how much total bench work time needs to finish 1 case of kidny electon microscopy(EM), 2 cases of kidney electon microscopy and 3 cases of kidney microscopy.

Q1. if suppose i wants to do one kidney case of EM, how much total time i have to spent bench work from start to finish without scope.

Q2. if suppose i wants to process two cases of kidney EM together how much total time i have to spent bench work from start to finish without scope.

Q3. if suppose i wants to process three cases of kidne EM together how much total time i have to spent bench work from start to finish without scope.

Q4. how many maximum cases kidney EM can be done per week in 40 hours.

Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Mar 7 11:49:33 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (MBA2038-at-AOL. COM) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, March 7, 2004 at 10:26:41
---------------------------------------------------------------------------

Email: MBA2038-at-AOL. COM
Name: steve yutz

Organization: NONE

Title-Subject: [Microscopy] [Filtered] Learning EM Programs

Question: i would like to learn Electron microscopy. Is there any program i can go to school in NY, NJ, DE, MD or PA state areas or i can learn on job.

Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 8 06:52:42 2004

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Greetings Listers,

Weill Cornell Medical College is welcoming a new TEM to our facility and
the following TEM is available for immediate sale:

JEOL JEM-100CXII
20 - 100kV
ASID/TEI Attachment Unit with 4x5 camera accessory
3 Specimen holders
1 Dual specimen holder
1 ASID/TEM specimen holder
1 BSD specimen holder
Chiller
Extra Filaments
100 Film plates with extra Cassette magazine and receiver
All associated support supplies and extra parts that we have on hand.

This microscope has been an excellent performer for us, as we still use
it on a daily basis and we are sorry to see it go. It has been under a
service contract since it's installation and has had two PM's every year.

Please contact us off list for further specifications and details
regarding this great opportunity.

Thanks in advance,

Michael Ganger: mtg2003-at-med.cornell.edu
Omayra Velez: omv2001-at-med.cornell.edu
Weill Cornell Medical College
Department of Pathology
Electron Microscopy Laboratory
1300 York Ave
New York, NY 10021
212-746-6437

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 8 08:03:27 2004

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----- Original Message -----
} From: Carol Heckman {heckman-at-bgnet.bgsu.edu}

Question: Is it possible to strictly confine the illuminated area on a
sample to a few square microns (using an aperture) when working in TIRF
geometry ?

We use an objektive-based TIRF microscope consisting of an Zeiss Axiovert
200 inverted microscope and an 100x NA1.45 Zeiss objective. To switch to
TIRF-mode we tilt a mirror at the entrance of the incident light device (its
position is conjugated to the sample plane).

We have a small aperture (rectangular, 2x2microns virtual size on the
sample) which is (in epifluorescent wide-field mode) reproduced nicely and
sharply on the sample, but when switching to TIRFM angle, the illuminated
field seems to blur on one side. Moreover, the illumination of our aperture
is no longer homogenous; there seems to be an intensity gradient along the
axis from the sharp to the blurry edge.

Sketch:

-------------------------
| Our aperture | {- This edge gets blurry.
| |
| | To reach TIRF geometry,
------------------------- we tilt our laser beam in
this direction --}
| This Side
Seems
To get darker.

At www.biophysics.jku.at/bioph/staf/brames/TIRF_problem.htm you can see a
comparison between wide-field illumination and TIRF-illumination and you can
also see our problem nicely.

So, is there a possibility to image an aperture sharply when using total
internal reflection microscopy?

Thanks in advance for your help

Mario Brameshuber

______________________________________
Mario Brameshuber
Institute for Biophysics
Johannes Kepler University of Linz,Austria
Altenbergerstraße 69
4040 Linz

phone: +43/732/2468/9288

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 8 12:05:12 2004

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I have a colleague who has an old (1960s vintage?) Zeiss petrographic
scope (reflected and transmitted light) which is missing its polarizing
lenses. He recently got a price quote on some repairs, including
replacement lenses, which comes to several hundreds of dollars -- money
he is not ready to spend. To cut costs, the microscope owner is
planning to cut polarizers out of a sheet of polaroid film. It seems to
me like this shouldn't cause too much of a problem, aside from the
possibility that the film might rotate around as he takes the
polarizers in and out, but I thought I might put the question out there
for people who are more knowledgeable than I. Also, will this
cost-cutting really save him much money? How much do polarizing lenses
usually cost, anyway?

Thanks,

Peter Selkin
pselkin-at-ucsd.edu

Lecturer/Postdoc
Scripps Institution of Oceanography, UC San Diego

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 8 15:22:12 2004

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Howdy,

I am looking for LM equipment with which to analyze particles on skin,
with particular interest in deposition levels. Optimally, I would like to
do this with a handheld microscope in the range of 300-1000x. I have a
lead or two, but am looking for more options, particularly cost-efficient
ones.

If anyone has some leads on companies or ideas for other ways to analyze
this microscopically, please contact me. Thanks!

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 8 16:07:32 2004

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Hi,
Generally speaking, polarized light microscopes have
polarizing "elements", not lenses. I think there have been a few
specialty scopes built in which an actual lens also controls the
state of polarization, but the usual tactic is to have flat elements,
rather like the film but manufactured to greater tolerance (ie, more
uniform surface, better extinction). THe main advantage and I suppose
expense is that it is essential to be able to rotate one of these
elements. So one of them usually has the mechanical bits to let you
rotate (and to read off the angle of rotation). The big problem your
colleague will have with the do it your self approach is that without
being able to rotate one of the films it will be extremely difficult
to get good extinction. On the other hand, if you had the element
that could rotate but was missing its optics and you put polarizing
film in, that would probably serve quite well.

I would have thought that a few hundred dollars would be fair
but many hundreds might be steep. There is always ebay...
Tobias

}
}
} I have a colleague who has an old (1960s vintage?) Zeiss
} petrographic scope (reflected and transmitted light) which is
} missing its polarizing lenses. He recently got a price quote on some
} repairs, including replacement lenses, which comes to several
} hundreds of dollars -- money he is not ready to spend. To cut
} costs, the microscope owner is planning to cut polarizers out of a
} sheet of polaroid film. It seems to me like this shouldn't cause too
} much of a problem, aside from the possibility that the film might
} rotate around as he takes the polarizers in and out, but I thought I
} might put the question out there for people who are more
} knowledgeable than I. Also, will this cost-cutting really save him
} much money? How much do polarizing lenses usually cost, anyway?
}
} Thanks,
}
} Peter Selkin
} pselkin-at-ucsd.edu
}
} Lecturer/Postdoc
} Scripps Institution of Oceanography, UC San Diego

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 03:30:52 2004

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We use a sem (cameca Su-30) and have to use epoxy mounts for coarse samples.
We can not mount them on aluminium sample holders. We can not put them in
sem because of their volume. We have to use epoxy. But is epoxy conductive?
I mean a ground problem occurs? Thanks.

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
SEM laboratory

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 04:09:52 2004

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Hi all!

What textbooks and multimedia teaching aids for EM in general, SEM and
EDS in particular, would you recommend? I am especially looking for
those with (at least some) emphasis on low voltage FEG-SEM and low
vacuum techinques and theory.

tia,
Stefan

+++++++++++++++++++++++++++++++++++++++++++++++++++++++
Dr Stefan Gunnarsson
Evolutionsbiologiskt Centrum Evolutionary Biology Centre
Enheten för biologisk strukturanalys Microscopy and Imaging Unit
Norbyvägen 18A
SE75236 Uppsala, Sweden Tel & Fax: +46 - 18 471 2638
+++++++++++++++++++++++++++++++++++++++++++++++++++++++

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 04:53:53 2004

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If he buys high quality film it should work well. McCrone Institute
sells them for as little as $4 per 2X2 sheet and they have 1/4 an 1/2
wave plates as well.

If you really want to do it rig get come Gnarled lens cement and put
glass covers on the plastic filters and mount them in a metal ring to
fit the scope. The extra effort will quickly pay off

Gordon
Gordon Couger
I collect Microscopy links and documentation posted at
http://www.couger.com/microscope/links/gclinks.html
http://www.science-info.org/
Attributed and anonymous contributions welcome

Tobias Baskin wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hi,
} Generally speaking, polarized light microscopes have polarizing
} "elements", not lenses. I think there have been a few specialty
} scopes built in which an actual lens also controls the state of
} polarization, but the usual tactic is to have flat elements, rather
} like the film but manufactured to greater tolerance (ie, more uniform
} surface, better extinction). THe main advantage and I suppose expense
} is that it is essential to be able to rotate one of these elements.
} So one of them usually has the mechanical bits to let you rotate (and
} to read off the angle of rotation). The big problem your colleague
} will have with the do it your self approach is that without being able
} to rotate one of the films it will be extremely difficult to get good
} extinction. On the other hand, if you had the element that could
} rotate but was missing its optics and you put polarizing film in, that
} would probably serve quite well.
}
} I would have thought that a few hundred dollars would be fair but
} many hundreds might be steep. There is always ebay...
} Tobias
}
}
} }
} }
} } I have a colleague who has an old (1960s vintage?) Zeiss
} } petrographic scope (reflected and transmitted light) which is missing
} } its polarizing lenses. He recently got a price quote on some repairs,
} } including replacement lenses, which comes to several hundreds of
} } dollars -- money he is not ready to spend. To cut costs, the
} } microscope owner is planning to cut polarizers out of a sheet of
} } polaroid film. It seems to me like this shouldn't cause too much of a
} } problem, aside from the possibility that the film might rotate around
} } as he takes the polarizers in and out, but I thought I might put the
} } question out there for people who are more knowledgeable than I.
} } Also, will this cost-cutting really save him much money? How much do
} } polarizing lenses usually cost, anyway?
} }
} } Thanks,
} }
} } Peter Selkin
} } pselkin-at-ucsd.edu
} }
} } Lecturer/Postdoc
} } Scripps Institution of Oceanography, UC San Diego
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 05:28:44 2004

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The book below is one of the first to have a section on low
vacuum/ESEM.

Dave

3rd Edition (2003)
Scanning electron microscopy and X-ray microanalysis a text for
biologists, materials scientists, and geologists Joseph I. Goldstein
... [et al]

On Tue, 9 Mar 2004 11:28:33 +0100 Stefan Gunnarsson
{Stefan.Gunnarsson-at-ebc.uu.se} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi all!
}
} What textbooks and multimedia teaching aids for EM in general, SEM and
} EDS in particular, would you recommend? I am especially looking for
} those with (at least some) emphasis on low voltage FEG-SEM and low
} vacuum techinques and theory.
}
} tia,
} Stefan
}
} +++++++++++++++++++++++++++++++++++++++++++++++++++++++
} Dr Stefan Gunnarsson
} Evolutionsbiologiskt Centrum Evolutionary Biology Centre
} Enheten för biologisk strukturanalys Microscopy and Imaging Unit
} Norbyvägen 18A
} SE75236 Uppsala, Sweden Tel & Fax: +46 - 18 471 2638
} +++++++++++++++++++++++++++++++++++++++++++++++++++++++
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 05:30:26 2004

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Thanks Richard for his reply and advice.
But I doubt about the contact of epoxy and sample holder of SEM (which has 6
holes for aluminium cylinder shaped sample holders). With epoxy there will
be no conductance with ground. I will coat the surface of epoxy and sample
with carbon but we have to screw it from the body of cylinder shaped epoxy.
So do we need to coat the sides of cylinder to make conductance with ground?
Or paint the sides of cylinder epoxy with silver?

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
SEM laboratory

-----Original Message-----
} From: Richard Beanland [mailto:richard.beanland-at-bookham.com]
Sent: 09 Mart 2004 Sali 12:23
To: 'Orkun Ersoy'

Orkun;

There are epoxies that are conductive. For example, there are silver loaded epoxies used in the semiconductor industry to attach microdevices. They are conductive through their bulk and usually have a silver content of } 90% by volume. Epotek and others make these products.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Orkun Ersoy [mailto:oersoy-at-hacettepe.edu.tr]
Sent: Tuesday, March 09, 2004 6:46 AM
To: Microscopy-at-MSA.Microscopy.Com

Thanks Richard for his reply and advice.
But I doubt about the contact of epoxy and sample holder of SEM (which has 6
holes for aluminium cylinder shaped sample holders). With epoxy there will
be no conductance with ground. I will coat the surface of epoxy and sample
with carbon but we have to screw it from the body of cylinder shaped epoxy.
So do we need to coat the sides of cylinder to make conductance with ground?
Or paint the sides of cylinder epoxy with silver?

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
SEM laboratory

-----Original Message-----
} From: Richard Beanland [mailto:richard.beanland-at-bookham.com]
Sent: 09 Mart 2004 Sali 12:23
To: 'Orkun Ersoy'

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Mike_Steves-at-Pall.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, March 8, 2004 at 14:43:01
---------------------------------------------------------------------------

Email: Mike_Steves-at-Pall.com
Name: Mike Steves

Organization: Pall Corp

Title-Subject: [Microscopy] [Filtered] MListserver: SEM

Question: Is there a stain for cellulose only? we need to see how far it penetrates into a polyethylene substrate, when viewed (X-Sec)in the SEM
Would Iodine work?
We have the capability to do X-Ray maps as well.
Thanks.

---------------------------------------------------------------------------

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For TEM we developed an enzyme-gold label. Details can be found here.
Berg, R.H., G.W. Erdos, M. Gritzali and R. Brown 1988. Enzyme-gold
affinity labeling of cellulose. ]. EM Tech. 8:371-380

For LM applications, Calcofluor is another option, but requires UV
illumination.

At 09:34 AM 3/9/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 08:44:16 2004

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Hi,
For light microscopy, a classic stain is "Calcofluor white"
(also known as Cellufluor, and some other names too). This is a
fluorescent dye, excited by UV and emitting blue. It will stain other
beta 1-4 linked polymers so that in a plant cell wall it is not
absolutely specific for cellulose. However, it does stain cellulose
brightly and in an artificial composite of cellulose and say
polyethylene, it should work perfectly, provided you can accept the
lower resolution of the light microscope.

To do this at higher magnification is harder, as far as I
know. There are cellulose binding proteins that can be coupled to
colloidal gold. These have been used in TEM to detect cellulose, and
could probably work in SEM provided you had the magnification to
detect the gold particles (typically 5 to 10 nm in diameter). Also I
believe that the gold-cellulose binding domain probe is not for
sale--you have to make it your self.

Hope this helps,
Tobias Baskin

}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (Mike_Steves-at-Pall.com) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html
} on Monday, March 8, 2004 at 14:43:01
} ---------------------------------------------------------------------------
}
} Email: Mike_Steves-at-Pall.com
} Name: Mike Steves
}
} Organization: Pall Corp
}
} Title-Subject: [Microscopy] [Filtered] MListserver: SEM
}
} Question: Is there a stain for cellulose only? we need to see how
} far it penetrates into a polyethylene substrate, when viewed
} (X-Sec)in the SEM
} Would Iodine work?
} We have the capability to do X-Ray maps as well.
} Thanks.
}
}
} ---------------------------------------------------------------------------

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 09:08:29 2004

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Mike,

I would be extremely reluctant to use iodine on samples to be introduced into a SEM due to the aggressivity of iodine vapor in causing corrosion. In any case, iodine forms a complex with starches which would seem not
to be the specificity that you are seeking. Iodine is also well known for adding to unsaturated bonds in organic compounds, adding another potential source of confusion.

If you can work with fluorescence microscopy instead of SEM there are some fluorescent dyes in the stilbene class that are often used for tagging cellulose. "Calcofluor" is one of these that is available from
histology suppliers. They work in a manner analogous to fabric "whiteners" in detergent that make the laundry fluoresce.

John Twilley
Conservation Scientist

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
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} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Mike_Steves-at-Pall.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, March 8, 2004 at 14:43:01
} ---------------------------------------------------------------------------
}
} Email: Mike_Steves-at-Pall.com
} Name: Mike Steves
}
} Organization: Pall Corp
}
} Title-Subject: [Microscopy] [Filtered] MListserver: SEM
}
} Question: Is there a stain for cellulose only? we need to see how far it penetrates into a polyethylene substrate, when viewed (X-Sec)in the SEM
} Would Iodine work?
} We have the capability to do X-Ray maps as well.
} Thanks.
}
} ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 09:37:02 2004

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Buehler, and I am sure others, sells a powdered nickel that can be added to
their epoxy, rendering the whole mass conductive, I believe. I made a
mount for my Philips XL 20 to hold round epoxy samples. It screws into the
stage in place of the pin mount holder.

Ron L

-----Original Message-----
} From: Orkun Ersoy [mailto:oersoy-at-hacettepe.edu.tr]
Sent: Tuesday, March 09, 2004 6:46 AM
To: Microscopy-at-MSA.Microscopy.Com

Thanks Richard for his reply and advice.
But I doubt about the contact of epoxy and sample holder of SEM (which has 6
holes for aluminium cylinder shaped sample holders). With epoxy there will
be no conductance with ground. I will coat the surface of epoxy and sample
with carbon but we have to screw it from the body of cylinder shaped epoxy.
So do we need to coat the sides of cylinder to make conductance with ground?
Or paint the sides of cylinder epoxy with silver?

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
SEM laboratory

-----Original Message-----
} From: Richard Beanland [mailto:richard.beanland-at-bookham.com]
Sent: 09 Mart 2004 Sali 12:23
To: 'Orkun Ersoy'

Not sure what your specimen stub looks like but
I do large metallurgical epoxy embedded specimens
all the time. They are mounted in an Aluminum
coupon cup and are retained on the SEM stage via
standard 3.1mm diameter pin. For a smaller
specimen, I would think that the same approach
would work.

Sputter coat the embedded specimen. Use a thin,
flexible double sticky tab (EMS or Fullam) that
just hits the top of the mount and runs down the
side. When mounted in the SEM, it will be
conductive.

gary g.

At 01:46 AM 3/9/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 10:54:11 2004

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Hi,

Though I don't work with it much these days, I was
lucky enough to have taken the "Polarized Light
Microscopy" course taught by Mr. McCrone here
at work. As far as the lenses go, there aren't
polarizing lenses, but there are lenses that are
specially made for polarized light microscopy.
They are a special variety of achromats called
"strain-free". From the McCrone book: "They
are carefully made, from the slow cooling of the
glass to the final assembly of the lens components,
so as to avoid causing strains in the glass which
would become visible when used in polarized
light microscopy." (*) There are also strain free
condenser lenses.

The other suggestions for making the polarizer
and analyzer are great, I just thought some may
be interested in the lens information.

* Polarized Light Microscopy
McCrone, McCrone, & Delly
Pub: McCrone Research Institute
ISBN 0-250-40262-9

Regards,
Darrell

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 17:30:53 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (StAmourOwl-at-charter.net) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 9, 2004 at 13:33:24
---------------------------------------------------------------------------

Email: StAmourOwl-at-charter.net
Name: Rick Dreiling

Organization: SIUE- Dental School

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am trying to purchase a bottle to store Osmium in. I am running into difficulty about how to clean the bottle. I have found recommendations of cleaning the glass with 5 % Hydrofluroic acid or 30% Nitric Acid. I am not too keen on either of these methods.

Has anyone been able to find a vendor that sells bottles already cleaned?

How do others deal with cleaning the bottles prior to storing Osmium in it? Is their another method I am unaware of?

If you forgo this cleaning step how long does your Osmium last?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 21:10:21 2004

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Dear listers,

I am analysing polished sections containing small (3 -10µm), globular, calcium aluminium oxide inclusions in a steel matrix. Naturally the analysis totals are high as the surrounding steel influences my oxide analysis. Is there a way/formula of determining how much metallic steel is being measured and thus removing it from the results (even though there may be up to 4% iron oxide present)? I have noticed that the amount of iron present is almost equal to the amount that the total exceeds 100. Is it that simple? Does the presence of metallic steel in the analysis affect the ratio of oxides present?

Thank you,

Jodi Reynolds.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 21:25:14 2004

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I'm not sure that I understand your problem.

I do metallographic specimens on a somewhat
routine basis. For best results, these are
epoxy embedded and polished.

If this is done, my EDAX Genesis EDS will do
a superior job on analyzing the specimen.
The analysis can be a simple ZAF or a more
complex PhiZAF or PhiRhoZAF. In either
event, the results are very good. The
key to obtaining valid quant data is to
achieve low Intensity Ratio errors. The
EDAX Genesis EDS system helps you do this.

For other systems, I do not know. For stainless
steel varieties, I routinely find 0.5-1.5% Fe
without problem. Perhaps your collection
system is not congruent with your specimens?

gary g.

At 07:26 PM 3/9/2004, you wrote:

} Dear listers,
}
} I am analysing polished sections containing small (3 -10µm), globular,
} calcium aluminium oxide inclusions in a steel matrix. Naturally the
} analysis totals are high as the surrounding steel influences my oxide
} analysis. Is there a way/formula of determining how much metallic steel
} is being measured and thus removing it from the results (even though there
} may be up to 4% iron oxide present)? I have noticed that the amount of
} iron present is almost equal to the amount that the total exceeds 100. Is
} it that simple? Does the presence of metallic steel in the analysis
} affect the ratio of oxides present?
}
} Thank you,
}
} Jodi Reynolds.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 21:38:01 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Possibly you are right about the collection system, we have a kevex detector and some good 'Oxford type' software provided by a local (Australian) genius. What I want to be able to do is discrimnate between the iron from the surrounding steel and the iron present as iron oxide in the non-metallic inclusion, using the resources I have.

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Wednesday, 10 March 2004 2:41 PM
To: Reynolds, Jodi JI
Cc: MSA listserver

I have no financial interest in EDAX whatsoever.
I am a totally satisfied user. Granted, their
software is very complex and quite intense.

I don't claim to be an expert with it. However....
I'm not all that shabby with it. Their HPD
feature is very powerful for identifying
true and false peaks.

You might send me a specimen and I can run
a complete analysis on it. It does not really
take all that long.

As with any EDS specimen, it should be polished,
flat and non-conductive. I can fix the conductive
aspect with coating. So, don't despair in this
regard.

Perhaps the EDAX could be a baseline for you
relative to your Oxford. Dunno. I have not
used that brand nor any others. Thus, the EDAX
could be a single data point. But, it really works.
IMO.

Again--big disclaimer. No financial interest
in EDAX. Just a super satisfied customer.

gary g.

At 07:54 PM 3/9/2004, you wrote:
} Possibly you are right about the collection system, we have a kevex
} detector and some good 'Oxford type' software provided by a local
} (Australian) genius. What I want to be able to do is discrimnate between
} the iron from the surrounding steel and the iron present as iron oxide in
} the non-metallic inclusion, using the resources I have.
}
} -----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Wednesday, 10 March 2004 2:41 PM
} To: Reynolds, Jodi JI
} Cc: MSA listserver
} Subject: [Microscopy] Re: SEM metallography
}
}
} I'm not sure that I understand your problem.
}
} I do metallographic specimens on a somewhat
} routine basis. For best results, these are
} epoxy embedded and polished.
}
} If this is done, my EDAX Genesis EDS will do
} a superior job on analyzing the specimen.
} The analysis can be a simple ZAF or a more
} complex PhiZAF or PhiRhoZAF. In either
} event, the results are very good. The
} key to obtaining valid quant data is to
} achieve low Intensity Ratio errors. The
} EDAX Genesis EDS system helps you do this.
}
} For other systems, I do not know. For stainless
} steel varieties, I routinely find 0.5-1.5% Fe
} without problem. Perhaps your collection
} system is not congruent with your specimens?
}
} gary g.
}
}
}
} At 07:26 PM 3/9/2004, you wrote:
}
}
} } Dear listers,
} }
} } I am analysing polished sections containing small (3 -10µm), globular,
} } calcium aluminium oxide inclusions in a steel matrix. Naturally the
} } analysis totals are high as the surrounding steel influences my oxide
} } analysis. Is there a way/formula of determining how much metallic steel
} } is being measured and thus removing it from the results (even though there
} } may be up to 4% iron oxide present)? I have noticed that the amount of
} } iron present is almost equal to the amount that the total exceeds 100. Is
} } it that simple? Does the presence of metallic steel in the analysis
} } affect the ratio of oxides present?
} }
} } Thank you,
} }
} } Jodi Reynolds.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 23:02:16 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I can show you spectra that look totally good and
very valid-looking but are totally wrong. This
is not known until applying the EDAX HPD feature.
The curve does not follow the spectra peaks. This
means that the elements in the list are wrong.
Plus, the Intensity Ratio values are also likely
too huge. Again, a big indicator of wrong data.

A quick, dumb, analysis will result in a seemingly
accurate result of element x and y and z. However,
one or more of them are not actually there. HPD is
the differentiation about this. I deal with Si and
Al, W, Ti, Os, Hf, Fe, Ta, et. al. and have to deal
with pile up at low eV. EDAX HPD makes sense out of
this. The ability to deconvolve is quite powerful.

Ordinarily, an EDS analysis may look OK, but in
reality, it is flat wrong. For example a nice peak
that shows Fe at 705eV (L alpha) turns out to be
F at 677eV (K alpha). So this is the issue of false
versus true peaks. It can get very complex and
very difficult without software assistance.

It is really identifying real elements versus wrong
elements. Easy to do if not careful.

gary g.

At 09:02 PM 3/9/2004, you wrote:
} What do you mean by 'true and false' peaks? My samples are polished and
} flat but why non-conductive? Shouldn't the surface be able to conduct so
} that any surface charge can be drawn away and reduce flaring? Hence
} carbon coating?
}
} Jodi.
}
} -----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Wednesday, 10 March 2004 3:51 PM
} To: Reynolds, Jodi JI
} Cc: MSA listserver
} Subject: [Microscopy] RE: SEM metallography
}
}
} I have no financial interest in EDAX whatsoever.
} I am a totally satisfied user. Granted, their
} software is very complex and quite intense.
}
} I don't claim to be an expert with it. However....
} I'm not all that shabby with it. Their HPD
} feature is very powerful for identifying
} true and false peaks.
}
} You might send me a specimen and I can run
} a complete analysis on it. It does not really
} take all that long.
}
} As with any EDS specimen, it should be polished,
} flat and non-conductive. I can fix the conductive
} aspect with coating. So, don't despair in this
} regard.
}
} Perhaps the EDAX could be a baseline for you
} relative to your Oxford. Dunno. I have not
} used that brand nor any others. Thus, the EDAX
} could be a single data point. But, it really works.
} IMO.
}
} Again--big disclaimer. No financial interest
} in EDAX. Just a super satisfied customer.
}
} gary g.
}
}
} At 07:54 PM 3/9/2004, you wrote:
} } Possibly you are right about the collection system, we have a kevex
} } detector and some good 'Oxford type' software provided by a local
} } (Australian) genius. What I want to be able to do is discrimnate between
} } the iron from the surrounding steel and the iron present as iron oxide in
} } the non-metallic inclusion, using the resources I have.
} }
} } -----Original Message-----
} } From: Gary Gaugler [mailto:gary-at-gaugler.com]
} } Sent: Wednesday, 10 March 2004 2:41 PM
} } To: Reynolds, Jodi JI
} } Cc: MSA listserver
} } Subject: [Microscopy] Re: SEM metallography
} }
} }
} } I'm not sure that I understand your problem.
} }
} } I do metallographic specimens on a somewhat
} } routine basis. For best results, these are
} } epoxy embedded and polished.
} }
} } If this is done, my EDAX Genesis EDS will do
} } a superior job on analyzing the specimen.
} } The analysis can be a simple ZAF or a more
} } complex PhiZAF or PhiRhoZAF. In either
} } event, the results are very good. The
} } key to obtaining valid quant data is to
} } achieve low Intensity Ratio errors. The
} } EDAX Genesis EDS system helps you do this.
} }
} } For other systems, I do not know. For stainless
} } steel varieties, I routinely find 0.5-1.5% Fe
} } without problem. Perhaps your collection
} } system is not congruent with your specimens?
} }
} } gary g.
} }
} }
} }
} } At 07:26 PM 3/9/2004, you wrote:
} }
} }
} } } Dear listers,
} } }
} } } I am analysing polished sections containing small (3 -10µm), globular,
} } } calcium aluminium oxide inclusions in a steel matrix. Naturally the
} } } analysis totals are high as the surrounding steel influences my oxide
} } } analysis. Is there a way/formula of determining how much metallic steel
} } } is being measured and thus removing it from the results (even though there
} } } may be up to 4% iron oxide present)? I have noticed that the amount of
} } } iron present is almost equal to the amount that the total exceeds 100. Is
} } } it that simple? Does the presence of metallic steel in the analysis
} } } affect the ratio of oxides present?
} } }
} } } Thank you,
} } }
} } } Jodi Reynolds.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 23:07:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Oh...sorry for the second posting.

Depending on your specimen, it may or may not
be conductive. For normal high vacuum work,
it needs to be conductive. Now, depending
on what the specimen actually is, and ignoring
this, I use Au/Pd or Pt coating. At 50A thickness,
this shows up as a very tiny peak in the EDS spectra.
I just click them out of the analysis for quant.

I do not use Carbon. Too messy. Os is better
but VP is ideal.

gary g.

At 09:02 PM 3/9/2004, you wrote:
} What do you mean by 'true and false' peaks? My samples are polished and
} flat but why non-conductive? Shouldn't the surface be able to conduct so
} that any surface charge can be drawn away and reduce flaring? Hence
} carbon coating?
}
} Jodi.
}
} -----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Wednesday, 10 March 2004 3:51 PM
} To: Reynolds, Jodi JI
} Cc: MSA listserver
} Subject: [Microscopy] RE: SEM metallography
}
}
} I have no financial interest in EDAX whatsoever.
} I am a totally satisfied user. Granted, their
} software is very complex and quite intense.
}
} I don't claim to be an expert with it. However....
} I'm not all that shabby with it. Their HPD
} feature is very powerful for identifying
} true and false peaks.
}
} You might send me a specimen and I can run
} a complete analysis on it. It does not really
} take all that long.
}
} As with any EDS specimen, it should be polished,
} flat and non-conductive. I can fix the conductive
} aspect with coating. So, don't despair in this
} regard.
}
} Perhaps the EDAX could be a baseline for you
} relative to your Oxford. Dunno. I have not
} used that brand nor any others. Thus, the EDAX
} could be a single data point. But, it really works.
} IMO.
}
} Again--big disclaimer. No financial interest
} in EDAX. Just a super satisfied customer.
}
} gary g.
}
}
} At 07:54 PM 3/9/2004, you wrote:
} } Possibly you are right about the collection system, we have a kevex
} } detector and some good 'Oxford type' software provided by a local
} } (Australian) genius. What I want to be able to do is discrimnate between
} } the iron from the surrounding steel and the iron present as iron oxide in
} } the non-metallic inclusion, using the resources I have.
} }
} } -----Original Message-----
} } From: Gary Gaugler [mailto:gary-at-gaugler.com]
} } Sent: Wednesday, 10 March 2004 2:41 PM
} } To: Reynolds, Jodi JI
} } Cc: MSA listserver
} } Subject: [Microscopy] Re: SEM metallography
} }
} }
} } I'm not sure that I understand your problem.
} }
} } I do metallographic specimens on a somewhat
} } routine basis. For best results, these are
} } epoxy embedded and polished.
} }
} } If this is done, my EDAX Genesis EDS will do
} } a superior job on analyzing the specimen.
} } The analysis can be a simple ZAF or a more
} } complex PhiZAF or PhiRhoZAF. In either
} } event, the results are very good. The
} } key to obtaining valid quant data is to
} } achieve low Intensity Ratio errors. The
} } EDAX Genesis EDS system helps you do this.
} }
} } For other systems, I do not know. For stainless
} } steel varieties, I routinely find 0.5-1.5% Fe
} } without problem. Perhaps your collection
} } system is not congruent with your specimens?
} }
} } gary g.
} }
} }
} }
} } At 07:26 PM 3/9/2004, you wrote:
} }
} }
} } } Dear listers,
} } }
} } } I am analysing polished sections containing small (3 -10µm), globular,
} } } calcium aluminium oxide inclusions in a steel matrix. Naturally the
} } } analysis totals are high as the surrounding steel influences my oxide
} } } analysis. Is there a way/formula of determining how much metallic steel
} } } is being measured and thus removing it from the results (even though there
} } } may be up to 4% iron oxide present)? I have noticed that the amount of
} } } iron present is almost equal to the amount that the total exceeds 100. Is
} } } it that simple? Does the presence of metallic steel in the analysis
} } } affect the ratio of oxides present?
} } }
} } } Thank you,
} } }
} } } Jodi Reynolds.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 9 23:30:43 2004

Contents Retrieved from Microscopy Listserver Archives
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Aaahh. Thank you, I can see how that would be a problem with a certain combination of elements. I am lucky in that respect as my sample is not entirely unknown. The inclusions are literally manufactured and the presence of elements which over lap with say Mg, Al and Si the low eV range is highly unlikely, if not totally impossible. Also, since my K alpha iron line (the lement of interset) also overlaps with some highly unlikely candidates (other than manganese and then I'd see the Mn K alpha line too) I am quite confident in my element selection.

Jodi.

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Wednesday, 10 March 2004 4:18 PM
To: Reynolds, Jodi JI
Cc: MSA listserver

Dear listers,

is there anybody who knows a web-based or other description of
EMSA-spectra file format standard?

Thanks in advance

Frank Eggert

===========================================
http://www.microanalyst.net
===========================================

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 05:16:19 2004

Contents Retrieved from Microscopy Listserver Archives
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Frank,

A full description of the standard, including example formats, can be
found at:
http://www.amc.anl.gov/ANLSoftwareLibrary/02-EMMPDL/Xeds/EMMFF/Emmff.Total

David Vowles
Electron Microscope Unit
Dept of Materials Science and Metallurgy
University of Cambridge
Pembroke St Cambridge
UK CB2 3QZ
Tel: +44 (0)1223 334325
Fax: +44 (0)1223 334567
Email: djv23-at-cam.ac.uk

On Wed, 10 Mar 2004, Frank Eggert wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear listers,
}
} is there anybody who knows a web-based or other description of
} EMSA-spectra file format standard?
}
} Thanks in advance
}
} Frank Eggert
}
}
} ===========================================
} http://www.microanalyst.net
} ===========================================
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 05:31:05 2004

Contents Retrieved from Microscopy Listserver Archives
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David,

thank you, that was, what I was searching, but not found.

Frank

David Vowles wrote:

} Frank,
}
} A full description of the standard, including example formats, can be
} found at:
} http://www.amc.anl.gov/ANLSoftwareLibrary/02-EMMPDL/Xeds/EMMFF/Emmff.Total
}
} David Vowles
} Electron Microscope Unit
} Dept of Materials Science and Metallurgy
} University of Cambridge
} Pembroke St Cambridge
} UK CB2 3QZ
} Tel: +44 (0)1223 334325
} Fax: +44 (0)1223 334567
} Email: djv23-at-cam.ac.uk
}
} On Wed, 10 Mar 2004, Frank Eggert wrote:
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 07:10:23 2004

Contents Retrieved from Microscopy Listserver Archives
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We just store ours in brown glass bottles. All we do in rinse the bottle out with distilled water and wrap parafilm around the lid. Osmium stored this way lasts for weeks without any problem.

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax

} } } by way of MicroscopyListserver {StAmourOwl-at-charter.net} 03/09/04 06:46PM } } }

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (StAmourOwl-at-charter.net) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 9, 2004 at 13:33:24
---------------------------------------------------------------------------

Email: StAmourOwl-at-charter.net
Name: Rick Dreiling

Organization: SIUE- Dental School

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am trying to purchase a bottle to store Osmium in. I am running into difficulty about how to clean the bottle. I have found recommendations of cleaning the glass with 5 % Hydrofluroic acid or 30% Nitric Acid. I am not too keen on either of these methods.

Has anyone been able to find a vendor that sells bottles already cleaned?

How do others deal with cleaning the bottles prior to storing Osmium in it? Is their another method I am unaware of?

If you forgo this cleaning step how long does your Osmium last?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 07:41:35 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

All I do is rinse out the jar with the buffer I'm going to use and then
make up my Osmium. I don't bother doing alot of cleaning and haven't had
any problems.

I did have a problem when I accidentally used a brown bottle that had been
used for osmium to make up a batch of uranyl acetate. I couldn't figure
out why the sections would jump off the grid (and run away for dear life!)
whenever I put them in my UA solution...live and learn!

Karen Bovard
EM Lab
Pathology
Creighton University Medical Center
Omaha, NE

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 07:54:09 2004

Contents Retrieved from Microscopy Listserver Archives
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Does anyone have any trick/tips that they would share about promoting
resin infiltration.

I work in a clinical pathology lab and time is of the essence.

I had read a small blurb in a book about someone putting their straight
resin and sections during infiltration under a 100 watt light bulb for the
heat to make the resin less viscous. Is this an OK thing to do? I crave
real life tips as to what others are doing!

Another question...What do most people feel is the most important step in
resin infiltration---the straight resin step vs the step with the resin
mixed with propylene oxide? Which step should I be placing the most
emphasis on to keep my time in the infiltration step as short as possible
and yet get the best possible results. I'm interested in hearing others
theories.

(I use EMBed 812 epoxy resin, PO, and process soft tissue for clinical
diagnosis--tumors, kidney, muscle, nerve, etc.)

Karen Bovard
EM Lab
Pathology
Creighton University Medical Center
Omaha, NE

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 08:05:35 2004

Contents Retrieved from Microscopy Listserver Archives
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Jodi:

Quite a bit of my work involves looking at inclusions
in steel using both metallography and SEM. Since
inclusions are small, you're sure to pick up the
surrounding steel matrix in the spectra from secondary
effects of the electron beam. I usually just ignore
it.

If you must determine the iron content within the
inclusion, there is an accepted technique I've read
about but not personally done. You can deeply etch
the surrounding metal matrix with dilute nital (4-10%
nitric acid in alcohol) so the inclusions stand proud.
Then apply softened replicating (acetate) tape. Let
harden, and remove the tape. This should hopefully
pull off the inclusions for EDS analysis without the
surrounding steel matrix. The inclusions should not
react to the nital.

Stu Smalinskas, P.E.
Sr. Metallurgist
SKF USA
Plymouth, Michigan
(734) 414-6862

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Jodi wrote:

Dear listers,

I am analysing polished sections containing small (3
-10µm), globular, calcium aluminium oxide inclusions
in a steel matrix. Naturally the analysis totals are
high as the surrounding steel influences my oxide
analysis. Is there a way/formula of determining how
much metallic steel is being measured and thus
removing it from the results (even though there may be
up to 4% iron oxide present)? I have noticed that the
amount of iron present is almost equal to the amount
that the total exceeds 100. Is it that simple? Does
the presence of metallic steel in the analysis affect
the ratio of oxides present?

Thank you,

Jodi Reynolds

ReynoldsJ-at-OneSteel.com

__________________________________
Do you Yahoo!?
Yahoo! Search - Find what you’re looking for faster
http://search.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 08:07:12 2004

Contents Retrieved from Microscopy Listserver Archives
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I always used soap and water, followed by several rinses with distilled
water. Why does a bottle for osmium need special cleaning? I certainly
would not use HF, it will etch the glass.

Geoff

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 08:16:24 2004

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Good morning, Karen,
When I worked in a Clinical EM Lab we found that placing our specimens,
in 100% resin, into a vacuum oven set at 37 degrees C for an hour helped
tremendously. The heat and vacuum together work much better than leaving the
vial on the rotator. Also, for large nerve pieces, you could leave them on
the rotator overnight in the 1:2 PO:resin then place them under vacuum the
next morning. That helped to prevent many of the holes in the axons.
As to which step is most important, the PO & resin or 100% resin, they
are equally important. The PO removes the alcohol or acetone, as well as
making the resin less viscous to pull it into the tissue. But the 100%
resin, especially under vacuum, draws out the remaining PO and further
infiltrates the tissues. If you have any PO left behind your blocks will not
polymerize properly nor cut well.
I hope this helps. Good luck! Feel free to write with any other
concerns.

Donna R. Clarkson
Northrop Grumman Information Technology
for U S Army Medical Research Detachment
at Brooks City-Base
Phone (210) 536-1416
FAX (210) 536-1449
e-mail donna.clarkson-at-brooks.af.mil
"Our Army at War--Relevant and Ready"

-----Original Message-----
} From: kbovard-at-creighton.edu [mailto:kbovard-at-creighton.edu]
Sent: Wednesday, March 10, 2004 8:10 AM
To: microscopy-at-ns.microscopy.com

Does anyone have any trick/tips that they would share about promoting
resin infiltration.

I work in a clinical pathology lab and time is of the essence.

I had read a small blurb in a book about someone putting their straight
resin and sections during infiltration under a 100 watt light bulb for the
heat to make the resin less viscous. Is this an OK thing to do? I crave
real life tips as to what others are doing!

Another question...What do most people feel is the most important step in
resin infiltration---the straight resin step vs the step with the resin
mixed with propylene oxide? Which step should I be placing the most
emphasis on to keep my time in the infiltration step as short as possible
and yet get the best possible results. I'm interested in hearing others
theories.

(I use EMBed 812 epoxy resin, PO, and process soft tissue for clinical
diagnosis--tumors, kidney, muscle, nerve, etc.)

Karen Bovard
EM Lab
Pathology
Creighton University Medical Center
Omaha, NE

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 08:26:20 2004

Contents Retrieved from Microscopy Listserver Archives
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Karen,

I think the fastest and easiest way to promote resin infiltration is to
use a microwave system, although it does require additional equipment.
Microwaves can take you from fresh tissue to polymerized blocks in 4-6
hours, with equal or sometimes better ultrastructure. They are ideal
for diagnostic work, because they make the procedure very fast, compared
to conventional processing methods, and do not (in my experience)
compromise quality. You can find details and protocols for these
systems on the websites of vendors selling them, such as Ted Pella and
Electron Microscopy Sciences and probably others.

Let me know if you have any questions. I have no financial interest in
any of these systems or companies, but our lab has been a very happy
user of microwave products.

Good luck.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

-----Original Message-----
} From: kbovard-at-creighton.edu [mailto:kbovard-at-creighton.edu]
Sent: Wednesday, March 10, 2004 8:10 AM
To: microscopy-at-ns.microscopy.com

Does anyone have any trick/tips that they would share about promoting
resin infiltration.

I work in a clinical pathology lab and time is of the essence.

I had read a small blurb in a book about someone putting their straight
resin and sections during infiltration under a 100 watt light bulb for
the heat to make the resin less viscous. Is this an OK thing to do? I
crave real life tips as to what others are doing!

Another question...What do most people feel is the most important step
in resin infiltration---the straight resin step vs the step with the
resin mixed with propylene oxide? Which step should I be placing the
most emphasis on to keep my time in the infiltration step as short as
possible and yet get the best possible results. I'm interested in
hearing others theories.

(I use EMBed 812 epoxy resin, PO, and process soft tissue for clinical
diagnosis--tumors, kidney, muscle, nerve, etc.)

Karen Bovard
EM Lab
Pathology
Creighton University Medical Center
Omaha, NE

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 08:40:18 2004

Contents Retrieved from Microscopy Listserver Archives
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I don't do a lot of high volume embedding, so I purchase the sealed vials of 4%
OsO4 fixative. I then make up small batches of 2% OsO4 (-at-20ml) at a time. I
use 20 ml scintillation vials and store it in the metal container that the vials
come in.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: StAmourOwl-at-charter.net [mailto:StAmourOwl-at-charter.net]
Sent: Tuesday, March 09, 2004 6:47 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by
(StAmourOwl-at-charter.net) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
March 9, 2004 at 13:33:24
---------------------------------------------------------------------------

Email: StAmourOwl-at-charter.net
Name: Rick Dreiling

Organization: SIUE- Dental School

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am trying to purchase a bottle to store Osmium in. I am running
into difficulty about how to clean the bottle. I have found recommendations of
cleaning the glass with 5 % Hydrofluroic acid or 30% Nitric Acid. I am not too
keen on either of these methods.

Has anyone been able to find a vendor that sells bottles already cleaned?

How do others deal with cleaning the bottles prior to storing Osmium in it? Is
their another method I am unaware of?

If you forgo this cleaning step how long does your Osmium last?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 08:42:28 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Sorry! I failed to mention that once we use up the OsO4, we rinse the
scint. vial and discard it in "hazardous" waste container. We don't bother
with cleaning and reusing the vials.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Paula Sicurello [mailto:patpxs-at-gwumc.edu]
Sent: Wednesday, March 10, 2004 8:24 AM
To: StAmourOwl-at-charter.net; microscopy-at-ns.microscopy.com

We just store ours in brown glass bottles. All we do in rinse the bottle
out with distilled water and wrap parafilm around the lid. Osmium stored
this way lasts for weeks without any problem.

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax

} } } by way of MicroscopyListserver {StAmourOwl-at-charter.net} 03/09/04 06:46PM
} } }

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (StAmourOwl-at-charter.net) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, March 9, 2004 at 13:33:24
---------------------------------------------------------------------------

Email: StAmourOwl-at-charter.net
Name: Rick Dreiling

Organization: SIUE- Dental School

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am trying to purchase a bottle to store Osmium in. I am running
into difficulty about how to clean the bottle. I have found recommendations
of cleaning the glass with 5 % Hydrofluroic acid or 30% Nitric Acid. I am
not too keen on either of these methods.

Has anyone been able to find a vendor that sells bottles already cleaned?

How do others deal with cleaning the bottles prior to storing Osmium in it?
Is their another method I am unaware of?

If you forgo this cleaning step how long does your Osmium last?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 09:09:40 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We use a standard glass bottle with a good plastic screw cap -
specifically, it is a Schott brand bottle that one can buy from most major
scientific supply houses. These bottles are the ones with blue or orange
caps. We start with a new clean bottle and rinse it well with distilled
water before using. We reuse the same bottle multiple times (} 1 year
usage per bottle) but the caps tend to become black with osmium so we
replace those about every 6 months. We keep this bottle in a plastic
secondary containment jar. The other jar is covered with aluminum foil to
minimize the osmium's exposure to light. We keep the whole assembly in a
fume hood at room temperature. Despite careful closing of the inner glass
jar, the inside of the plastic container goes black with time. This should
be a strong warning to those who keep their osmium in a refrigerator. They
are slowly leaking osmium into the refrigerator, the rest of its contents
and their lab air.

If the osmium stock goes bad (turns black prematurely), I would discard it
and probably the bottle rather than waste time cleaning it. If I had a
valuable piece of class contaminated with osmium, I would use hydrogen
peroxide (H2O2) to remove the osmium. This works great but it is very
reactive and significant quantities of osmium should not be mixed with
hydrogen peroxide or you may get a violent exothermic reaction.

} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by
} (StAmourOwl-at-charter.net) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
} March 9, 2004 at 13:33:24
} ---------------------------------------------------------------------------
}
} Email: StAmourOwl-at-charter.net
} Name: Rick Dreiling
}
} Organization: SIUE- Dental School
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: I am trying to purchase a bottle to store Osmium in. I am running
} into difficulty about how to clean the bottle. I have found
} recommendations of
} cleaning the glass with 5 % Hydrofluroic acid or 30% Nitric Acid. I am
} not too
} keen on either of these methods.
}
} Has anyone been able to find a vendor that sells bottles already cleaned?
}
} How do others deal with cleaning the bottles prior to storing Osmium in
} it? Is
} their another method I am unaware of?
}
} If you forgo this cleaning step how long does your Osmium last?
}
} ---------------------------------------------------------------------------

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 09:31:25 2004

Contents Retrieved from Microscopy Listserver Archives
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We have found that teflon bottles work well with osmium. There are some that are inert to nearly all chemicals, and they don't break if dropped. We wrap the top in parafilm for storage. I just rinse between refills and have no trouble with contamination.
Mary Gail Engle

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 09:46:12 2004

Contents Retrieved from Microscopy Listserver Archives
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Jodi:

I believe that your question is " how many of the x-rays are coming from
the steel matrix and not from the inclusion." There are some software
applications that address beam interaction area, including Electron
Flight Simulator (http://www.small-world.net/efs.htm) (no financial
interest, etc, etc.). These would help determine whether the volume of
x-ray emission is within a specific size of inclusion. You can also make
some estimates from simple nomographs that estimate electron penetration
depth as a function of accelerating voltage and sample density. These
nomographs can be found in texts and on periodic tables provided by some
EDS systems providers.

From my experience, there are other considerations that need to be made
on analyzing metallographically polished samples. The first is smearing
or carryover of matrix material into the inclusion. Inclusions are often
porous, so will capture polishing debris that is removed from the
surrounding matrix. Some of the iron that you detect could be polishing
residue if you are using mechanical polishing. Polishing compounds can
contaminate the inclusions in the same fashion, so you may detect higher
silicon or aluminum concentrations if you use silica or alumina
polishing compounds. I typically stick to diamond polishing for samples
where good EDS data is needed.

Be cautious if you are using a variable pressure SEM. VP is great for
analysis of nonconductive samples, but many operators are not aware
that the VP environment spreads the beam. The result is that you get
significant x-ray production from a much wider area than you would for
high vacuum operation. So, analysis of inclusion in steel would show
higher iron concentrations with VP than with high vac conditions.
Electron flight simulator can produce simulations of beam scatter for
various conditions.

Stu's suggestions on separating the inclusions from the matrix is a good
one, but you may still have some residue of steel matrix on the
inclusions pulled out on the replica.

Hope this helps.

--
Larry D. Hanke, P.E.
Materials Evaluation and Engineering, Inc.
Practical Solutions Through Technology and Innovation
http://www.mee-inc.com (763) 449-8870

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 09:50:40 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I store osmium in washed / rinsed scintillation vials with Parafilm wrapped
around the vial cap. The vials are stored in a larger jar along with
vegetable oil osmium traps. The lid of the outer jar is also sealed with
Paraflm. So far I have never had the outermost Parafilm darken since the
oil inside the second jar traps any osmium vapors that might get past the
Parafilm on the scintillation vial.

Lee Hadden, Ph. D.
Department of Biology
Wingate University
Wingate, NC 28174
704-233-8236

-----Original Message-----
} From: Geoff McAuliffe [mailto:mcauliff-at-umdnj.edu]
Sent: Wednesday, March 10, 2004 12:23 PM
To: by way of MicroscopyListserver
Cc: microscopy-at-ns.microscopy.com

I always used soap and water, followed by several rinses with distilled
water. Why does a bottle for osmium need special cleaning? I certainly
would not use HF, it will etch the glass.

Geoff

by way of MicroscopyListserver wrote:

} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

---
[This E-mail scanned for viruses by Declude Virus]

---
[This E-mail scanned for viruses by Declude Virus]

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 10:27:01 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

David Vowles already pointed you to the right place. While you are there, you might want to look at a couple of utilities that I wrote. The descriptions and the links are below:

EELS PLOT, A Windows-based electron energy loss spectroscopy and X-ray energy dispersive
spectroscopy plotting and processing program for EMSA formatted spectra that will smooth,
differentiate, re-color, re-scale, filter, plot, print, annotate, substract background, integrate intensities,
display, overlay, and do limited analysis.
http://www.amc.anl.gov/ANLSoftwareLibrary/02-EMMPDL/Eels/EELSPlot/

EM Periodic Table, A Windows-based electron energy loss spectroscopy and X-ray energy
dispersive spectroscopy program for displaying energy peak and edge values and for determining
possible spectral peak overlap lines.
http://www.amc.anl.gov/ANLSoftwareLibrary/02-EMMPDL/Xeds/EMPeriodicTable/

The second of these is included in the first program.

Let me know what you think.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Frank Eggert [mailto:Eggert-at-mikroanalytik.de]
Sent: Wednesday, March 10, 2004 5:23 AM
To: microscopy-at-MSA.Microscopy.com

Dear listers,

is there anybody who knows a web-based or other description of
EMSA-spectra file format standard?

Thanks in advance

Frank Eggert

===========================================
http://www.microanalyst.net
===========================================

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 11:07:26 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Larry -

You make a good point about the beam spread in a VP SEM. When I'm doing EDS
in our ESEM, I normally turn the chamber vapour pressure down to 0 (well,
it's not really 0, but it's substantially reduced) during the acquisition.
This causes the image to "fade to black", but that's not normally an issue.
At least it keeps the beam spread to a minimum.

F.C. Thomas
Geological Survey of Canada (Atlantic)
Dartmouth, Nova Scotia

-----Original Message-----
} From: Larry Hanke [mailto:hanke-at-mee-inc.com]
Sent: Wednesday, March 10, 2004 12:02 PM
To: MSA listserver
Cc: Reynolds, Jodi JI

Jodi:

I believe that your question is " how many of the x-rays are coming from
the steel matrix and not from the inclusion." There are some software
applications that address beam interaction area, including Electron
Flight Simulator (http://www.small-world.net/efs.htm) (no financial
interest, etc, etc.). These would help determine whether the volume of
x-ray emission is within a specific size of inclusion. You can also make
some estimates from simple nomographs that estimate electron penetration
depth as a function of accelerating voltage and sample density. These
nomographs can be found in texts and on periodic tables provided by some
EDS systems providers.

From my experience, there are other considerations that need to be made
on analyzing metallographically polished samples. The first is smearing
or carryover of matrix material into the inclusion. Inclusions are often
porous, so will capture polishing debris that is removed from the
surrounding matrix. Some of the iron that you detect could be polishing
residue if you are using mechanical polishing. Polishing compounds can
contaminate the inclusions in the same fashion, so you may detect higher
silicon or aluminum concentrations if you use silica or alumina
polishing compounds. I typically stick to diamond polishing for samples
where good EDS data is needed.

Be cautious if you are using a variable pressure SEM. VP is great for
analysis of nonconductive samples, but many operators are not aware
that the VP environment spreads the beam. The result is that you get
significant x-ray production from a much wider area than you would for
high vacuum operation. So, analysis of inclusion in steel would show
higher iron concentrations with VP than with high vac conditions.
Electron flight simulator can produce simulations of beam scatter for
various conditions.

Stu's suggestions on separating the inclusions from the matrix is a good
one, but you may still have some residue of steel matrix on the
inclusions pulled out on the replica.

Hope this helps.

--
Larry D. Hanke, P.E.
Materials Evaluation and Engineering, Inc.
Practical Solutions Through Technology and Innovation
http://www.mee-inc.com (763) 449-8870

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 11:19:33 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Jodi,
I had one student that dissolved the steel completely with bromine/ methanol and
filtered out the inclusions for analysis, but I agree with Stu that the acetate
replica technique is the one to use to separate the inclusions from the matrix
and look at them free of polishing artifacts and beam spread. I have done it and
it is quite simple.
1. Etch the sample with the appropriate etch. Fairly deep etch is best.
2. Soften cellulose acetate sheet ( 5 or 6 thou thick), cut into a 1cm by 2cm
strip, by placing it on a stack of filter papers moistened with acetone.
3. Put a small pool of acetone on the surface to be replicated and place the
acetate sheet on the pool of acetone. I find it helps handling if you bend 5 mm
of one end of the acetate up as a handle, before you start.
4. Wait half and hour for all the acetone to dry away and the acetate to go hard
and carefully pull the acetate away from the metal. Turn it over and fix to a
stub. Either gold or carbon coat or examine in variable pressure, since the
acetate is non-conductive. You should have nice inclusions sitting on a replica
of the etched metal, with only carbon and oxygen in the acetate to interfere.
Other considerations: how high is your x-ray take-off angle? High take-off angle
detectors see less of the rim of the inclusion, but it is not something you can
change in an existing setup. If you find a big inclusion (10 microns), how low
does the Fe content go? You might consider tilting the sample towards the EDS
detector to raise the take-off angle. I think that totals above 100% are more a
result of imprecision in the ZAF routines than an indication of metallic vs.
oxide iron. There is no way to tell them apart in EDS.
Good luck.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Reynolds, Jodi JI" {ReynoldsJ-at-onesteel.com}
To: {Microscopy-at-msa.microscopy.com}
Sent: Tuesday, March 09, 2004 7:26 PM

Dear listers,

I am analysing polished sections containing small (3 -10µm), globular, calcium
aluminium oxide inclusions in a steel matrix. Naturally the analysis totals are
high as the surrounding steel influences my oxide analysis. Is there a
way/formula of determining how much metallic steel is being measured and thus
removing it from the results (even though there may be up to 4% iron oxide
present)? I have noticed that the amount of iron present is almost equal to the
amount that the total exceeds 100. Is it that simple? Does the presence of
metallic steel in the analysis affect the ratio of oxides present?

Thank you,

Jodi Reynolds.

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 13:30:27 2004

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Karen,
To answer a few questions:
1. The heat of the lightbulb should not be a problem because I routinely put my
embedding dishes on top of my 60 degree oven overnight to warm and thin the
epon before putting the dishes into the oven. I remember when I started in TEM
(1971) that our procedure called for putting the molds into 2 ovens, the first
was maybe 35 degrees and the second at 60C the next morning.

2.Decades ago a fellow tech. was doing a fast sample prep of melanoma tumors. He
needed to section the day after receiving the tissue so he trimmed the samples
as small as possible and then used a magnetic stirrer - "flea" real small one,
in a scintillation vial to keep the solutions moving all the time. This worked
up to the complete epon exchange which was really too dense for the flea to
move in. Of course all the times were shortened so that the samples went into
the oven by the end of the day. If I remember correctly the oven that he used
was set at 70C.

For years I have put difficult samples on a rotating table instead of the table
top since I do not have one of those tissue rotators. The motion helps to mix
the small amount of solution that remains in the vials into the newly added
chemicals.

Can you purchase a microwave oven?

Pat Connelly
U of P
Biology Dept.
Philadelphia PA
psconnel-at-sas.upenn.edu
*
Quoting kbovard-at-creighton.edu:
------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
}
} Does anyone have any trick/tips that they would share about promoting
} resin infiltration.
}
} I work in a clinical pathology lab and time is of the essence.
}
} I had read a small blurb in a book about someone putting their straight
} resin and sections during infiltration under a 100 watt light bulb for the
} heat to make the resin less viscous. Is this an OK thing to do? I crave
} real life tips as to what others are doing!
}
} Another question...What do most people feel is the most important step in
} resin infiltration---the straight resin step vs the step with the resin
} mixed with propylene oxide? Which step should I be placing the most
} emphasis on to keep my time in the infiltration step as short as possible
} and yet get the best possible results. I'm interested in hearing others
} theories.
}
} (I use EMBed 812 epoxy resin, PO, and process soft tissue for clinical
} diagnosis--tumors, kidney, muscle, nerve, etc.)
}
} Karen Bovard
} EM Lab
} Pathology
} Creighton University Medical Center
} Omaha, NE

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 14:25:45 2004

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SPURR resin is much less dense than Epon. I do believe, you really could
short infiltration time with Spurr without compromising the quality. This
is total improvisation (never tried!!!!!!!!!!!!!!!!!!!!):
for really small pieces (0.5x0.5x0.5mmm)
30-50-70-95% Et-OH 10 min each
2x100% Et-OH - 20 min each
Prop Oxide (PO) - 20 min
PO:Spurr 1:1 - 40 min on rotator
Spurr - 1 h on rotator (tube should be open)
fresh Spurr - 1 h on rotator (tube should be open)
fresh Spurr in the mold, polymerization at 60oC (not higher), 24 h

Microwave is also good (possible best) idea.

Let me know if it works. Sergey

At 11:46 AM 3/10/2004, you wrote:

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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 15:19:09 2004

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Hello,

I'm searching for a preparation technology to make a grain size
determination with a SEM.
The grains should be distributed in a one-layer.
Gritting the powder is not satisfying, because the powders (about 1 to
30µm) agglomerates.
Does anyone have an idea how to make the preparation?
The SEM-picture should be evaluated with an image analysing software.

Thank you very much
Timo Junker

--
Timo Junker Holografie
Lindenstr. 10
97297 Waldbüttelbrunn
Tel: ++49 (0)931 4520655
Fax: ++49 (0)931 4520657
www.holografie.com

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 15:35:55 2004

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Hi Stu,

This is a great idea and I will definitely give it a go.

Cheers,

Jodi.

-----Original Message-----
} From: Kestutis Smalinskas [mailto:smalinskas-at-yahoo.com]
Sent: Thursday, 11 March 2004 1:22 AM
To: microscopy-at-sparc5.microscopy.com; Reynolds, Jodi JI

Hi Larry,

I generally, but not always, use an ultra sonic bath to clean the samples before analysis, do you think this is effective? I'd like to try the acetate tape method and pull the inclusions out, but you're right about the possibility of the incusions taking some of the steel with them. This would be obvious straight away I imagine and perhaps some of the inclusions would be free of steel matrix residue.

Thank you for your help,

Jodi.

-----Original Message-----
} From: Larry Hanke [mailto:hanke-at-mee-inc.com]
Sent: Thursday, 11 March 2004 3:02 AM
To: MSA listserver
Cc: Reynolds, Jodi JI

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (maloneyb-at-fiu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, March 10, 2004 at 09:40:19
---------------------------------------------------------------------------

Email: maloneyb-at-fiu.edu
Name: Barbara

Organization: FCAEM/FIU

Title-Subject: [Microscopy] [Filtered] TEM receipes for T4 bacteriophages

Question: Dear Group: would you please recommend the following:
1. buffers to use especially for T4 bacteriphages
2. what fixatives to use and postfixative
3. what negative stain works best
Let me know ASAP
thanks for your help
Barb

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 17:54:38 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Mukundan.Chakrapani-at-nrc.ca) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, March 10, 2004 at 13:00:34
---------------------------------------------------------------------------

Email: Mukundan.Chakrapani-at-nrc.ca
Name: Mukundan Chakrapani

Organization: National Research Council

Title-Subject: [Microscopy] [Filtered] AFM MAC mode imaging

Question: I have been using Molecular Imaging AFM in the MAC mode to image lipid bilayers under liquid. Everytime I change to a new tip, the images are okay to begin with but the quality deteriorates subsequently.
Can anyone comment on this phenomenon?

Thank you,

Mukundan

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 18:24:41 2004

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Richard Edelmann wrote:

} ......................could someone explain to me how using a higher
} accellerating voltage could/would/should decrease chromatic
} aberations in the EM? Particluarly in the TEM.

Richard,

It's as Dave Barnard wrote. The effective spread of focus in the TEM is the
chromatic aberration coefficient times the sum of (the relative energy spread in
the beam, the relative HT variation during the image acquisition time, and the
relative variation in the lens current during the image acquisition time).
Increasing the accelerating voltage lowers the relative energy spread term (the
deltaE/E term).

The focal length of the objective lens is proportional to the beam energy (higher
energy makes the electrons heavier and the lens less able to deflect them) and
inversely proportional to the square of the lens current (more current means
stronger lens with stronger focusing).

So a small variation in beam energy produces a small variation in the focal
length: delF/F is proportional to delE/E. Similarly, a small variation in lens
current produces a small variation in the focal length: delF/F is proportional to
-2 x delI/I (the 2 x comes from the square and the - comes from the inverse).
Where F, E and I are the focal length, beam energy, and lens current, and delF,
delE, and delI are their variations.

The constant of proportionality is Cc, the chromatic aberration coefficient. The
beam energy variations come from the beam energy spread plus variations in the
high-tension power supply. Beam energy spread can be as low as 0.7 eV FWHH for a
FEG TEM. HT variation can be 1 part per million root-mean-square. Converting the
0.7 eV full-width half-height to root-mean-square gives 0.7/2.355 = 0.3 eV. Then,
for 300kV the relative beam energy spread is 0.3 eV / 0.3 = 1.0 ppm rms. For a
200kV TEM, the relative beam energy spread would be 0.3 eV / 0.2 = 1.5 ppm rms.
However, the total 200kV beam variation is not 50% greater than the 300kV result
because the HT variation of 1 ppm rms must be added. Since the energy spread and
HT variation are independent* we add in quadrature to get sqrt [ 1.0**2 + 1.0**2 ]
= 1.4 for 300kV and sqrt [ 1.0**2 + 1.5**2 ] = 1.8 for 200kV. So going to 300kV
lowers the beam variation to about 80% of its 200kV value -- this 27% improvement
will of course vary depending on the actual beam energy spread and HT variation. .

We then need to add in the contribution coming from the lens current variation.
Then we multiply by Cc to get the spread of focus. Again we add in quadrature.
Assuming the lens variation is 0.8 ppm rms, and the Cc is 1.5 mm (typical values),
we get:
Spread of focus = Cc times sqrt [ (delE/E)**2 + (2 x delI/I)**2 ] = 1.5 x sqrt
[1.4**2 + 1.6**2] = 3.2 nm at 300kV, and 1.5 x sqrt [1.8**2 + 1.6**2] = 3.6 nm at
200kV. Now the improvement is only 13% on going from 200kV to 300kV. The amount
of improvement on increasing from 200 to 300 kV will vary depending on both the
relative HT variation and the relative lens current variation.

* "the energy spread and HT variation are independent" -- mostly, see “Estimation
of the Electron Beam Energy Spread for TEM Information Limit”, Michael A. O’Keefe,
Peter C. Tiemeijer and Maxim V. Sidorov, Microscopy and Microanalysis 8 (2002)
supplement 2: 480-481.

That is all.
Mike O'Keefe

David Barnard wrote:

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} -------------------------------------------------------------------------------
}
} I am thinking that the energy spread of the the source should be the
} same reguardless of accellerating voltage and the accellerator adds
} the exact same elctron volts to all electrons so the energy
} (chromatic) spread arriving at any lens should be the same no matter
} the accelerating voltage. Chromatic aberation, however, is a function
} of the relative energy spread compared to the final ev. The
} deflection error due to the spread at the source has a much smaller
} contribution to the total deflection in a higher voltage TEM lens.
}
} My 2 ev worth
}
} Dave
}
} --
} David Barnard
} Wadsworth Ctr
} NYS Dept Health
} Albany NY 12201-0509
} barnard-at-wadsworth.org
} 518 473-5299 voice
} 518 474-7992 fax

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 10 21:40:05 2004

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Hi All,

I'm posting this question on behalf of a colleague:

I would like to buy a PC (Mac or IBM clone) program for drawing stereograms that can show the relative orientation of two phases Eg matrix/precipitate relationships. I have been using Desktop Microscopist but it is an old version and not really compatible
with the current operating systems we use.

I would be most grateful of any advice/suggestions you would care to make.

Yours in hope

Kath

Mark Blackford
Materials and Engineering Science, ANSTO
PMB 1,
Menai, N.S.W., 2234
Australia

Phone 61 2 9717 3027
Fax 61 2 9543 7179

Disclaimer:
The views expressed in this E-mail message do not necessarily represent the official views of ANSTO from which this message was conveyed.

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 01:20:07 2004

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For disaggregation this would be helpful.
50 g aliquots of sample must be treated with about 100 ml dilute HCl for 5
min. in an ultrasonic bath. One liter of distilled water is added to further
dilute the acid and left 24 hours to let the particles settle. After
drainage of dilute acid, samples are dried overnight at 150 C.(Wohletz et
al. 1995- JVGR v. 67)

-----Original Message-----
} From: Timo Junker [mailto:timojunker-at-holografie.com]
Sent: 10 Mart 2004 Çarsamba 23:35
To: Microscopy-at-MSA.Microscopy.Com

Hi Timo,

I think some indication of the material it is you are trying to disperse
would be helpful. Otherwise, any offered solutions may be fruitless.

Regards,

David Bell
Scientist
Electron Microscopy Lab
Millipore Corporation
80 Ashby Road
Bedford, MA 01730
(781) 533-2108

"Orkun Ersoy" {oersoy-at-hacettepe.edu.tr}
03/11/2004 02:34 AM

To: {Microscopy-at-MSA.Microscopy.Com}
cc:
Subject: [Microscopy] RE: powder preparation technology for Grain size
determination (SEM) - need help

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

For disaggregation this would be helpful.
50 g aliquots of sample must be treated with about 100 ml dilute HCl for 5
min. in an ultrasonic bath. One liter of distilled water is added to
further
dilute the acid and left 24 hours to let the particles settle. After
drainage of dilute acid, samples are dried overnight at 150 C.(Wohletz et
al. 1995- JVGR v. 67)

-----Original Message-----
} From: Timo Junker [mailto:timojunker-at-holografie.com]
Sent: 10 Mart 2004 Çarsamba 23:35
To: Microscopy-at-MSA.Microscopy.Com

I use a technique developed by Millonig:

First, I use Spurr's, after dehydration with acetone, although I am sure
that po users culd also use the method. I infiltrate using specimens in
microcentrifuge tubes in an old desk-top clinical centrifuge (the one with
holders for 4 stnadard 15 ml tubes). Max speed is 2500 rpm (I have no
idea what the rcf is).

For each step, I centrifuge for 10 minutes:

5 drops Spurrs in 100 acetone
1:3 Spurr's:acetone
1:1 Spurr's:acetone
3:1 Spurr's acetone
2 changes of 100% acetone
Embed in fresh Spurr's.

Using .5 mm cubes of specimen, I can go from water to embedding oven in
less than 3 hours.

Best,

Don

______________________________________________________________________
Donald L. Lovett e-mail: lovett-at-tcnj.edu
Assoc. Professor, Dept. of Biology voice: (609) 771-2876
P.O. Box 7718 fax: (609) 637-5118
The College of New Jersey
Ewing, NJ 08628-0718

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 06:45:56 2004

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Hi Everybody,

We are studying the cells of SPUTUM with fluorescence (syto 25). we are
continuously having troble with the high autofluorescence of epithelial
cells (from mouth). We are using optilyse to treat the cells before
staining.

Does anybody know the cause for the autofluorescence and/or the treathent to
lower the autofluorescence.

Thanks

Ari Kuusisto
Research physicist

PerkinElmer Life and Analytical Sciences
tel. +358-2-2678 508
fax. +358-2-2578 357
E-mail: Ari.Kuusisto-at-PerkinElmer.com

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 09:55:23 2004

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A while back, someone on the list requested a spare holder for 3.5 x
4 in. film and I believe that it was for a Hitachi scope. I recently
found some in a box that had two labels on it, I thought that they
were for a Philips but they came from a Hitachi. If they are still
needed, I have a bunch of them but would like a good description of
the part you wish in case they are not a match.

Please contact me directly.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 10:09:38 2004

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Hi,

Our facility is in the process of acquiring an Arcturus LCM system. We
have been given a preview of both systems by an Arcturus
representative. But we are in need of some advice from investigators
who have used either the PixCell IIe and/or the AutoPix systems. Any
information regarding the advantages or disadvantages of each system
would be appreciated. Particular issues that concern us and would
appreciate any response on are:

Ease of use
Initial set up time for each of the systems
Resolution of each system
Sampling time for Proteomics and purity of samples for downstream
processing for ex. 50 to 500 samples
Can the template for the AutoPix be saved for future use?
Reliability of both hardware and software
Maintenance costs for each system.

Thank you in advance for your feedback.

aruna

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 11:37:57 2004

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Dear Microscopists,

I'm involved in a project working with gold and silver coins recovered
from a shipwreck. The ship went down in the 1800's. I am seeking advice
on how to clean some of the coins in a way that will not remove any of
the gold or silver from the coins. Some of the coins have coral on them,
some have iron oxide, some cupric cloride, and some have iron sulfide on
them. The sulfide is the real problem. Do any of you have suggestions as
to how to clean the coins chemically? I don't have the equipment to
clean them by electrolysis, and cannot polish them, for that would
decrease their value. Thank you in advance for your suggestions.

Edward Haller
Diagnostic Electron Microscopy Lab
University of South Florida
Pathology Department
Tampa, FL 33612
(813)974-9584

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 11:41:05 2004

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Immunogold Workshop Announcement

Dear Researcher:

      The Electron Microscopy Facility-Medical School at the University
of Wisconsin is hosting a three-day workshop on immunogold techniques
from May 24-26, 2004. Dr. Jan Luenissen from Aurion Immunogold Reagents
& Accessories, an internationally known expert in the field, will be
the instructor for the workshop. The workshop will include lectures,
hands-on training, round table discussions, and presentations on
applications. Also, participants of the workshop will be able to work
on their own samples during the workshop. The workshop main curriculum
is detailed below. If you are interested in attending or need more
information about the workshop, please contact the workshop technical
coordinator Hong Yi by phone (404-727-8692) or email (hyi-at-emory.edu).

MAIN CURRICULUM

The properties of gold particles and their protein conjugates.
Theories underlying immunogold labeling protocols.
Silver enhancement of gold particles
Immunogold labeling on a variety of sample preparations for LM.
Immunogold labeling for EM
a. Pre-embedding immunogold labeling using ultrasmall gold conjugates
and silver enhancement.
b. Post-embedding immunogold labeling using conventional colloidal gold
conjugates and   ultrasmalll gold conjugates.
Pre- and post-embedding double immunogold labeling.
Background minimization in immunogold labeling
Signal amplification in immunogold labeling.

Thanks and we hope to see you in Madison.

Randall Massey
Operations Manager
UW-Electron Microscope Facility
1300 University Ave.
Madison, WI 53706
voice (608)262-2993
Fax  (608)262-7306

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Hi Karen
We have a Pelco Microwave with a coolspot and a vaccum chamber. If we
have all the chemicals made up and ready to go (including the resin)
we can go from fixing and cutting in 2 hours. The results are as if
we had done it conventionally. The resin is an Epon-Spurr mix and
usually cuts easier than Epon alone.
Elaine

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--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 13:26:52 2004

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A grad student working with plant tissue in our labs wants to purchase
a diamond knife. Supplier catalogs indicate different specification
when you purchase a knife for TEM ultra-structure. When cutting plant
tissue I use a "knife angle" 4 degrees an obtain great results. My
question concerns the manufactures description of a 35 or 45 degree
knife. Is this the angle of the diamond mounted in the boat ?
Knowing we plan to cut plant tissues imbedded in spurr, what angle
knife would you suggest we select and why (35 or 45) ? If anyone can
also give me a good reference for diamond knives and cutting that would
be great.

If you wish you can forward your emails directly to
dufresne-at-ms.umanitoba.ca

Thanks,
André

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 13:39:52 2004

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Hello,

I have a customer that needs to section drilling mud core samples using a
cryostat. He is using a tungsten carbide knife and the sections are 30
microns thick. The problem is that no matter what we try, tape or plastic
tubing, the section falls apart. He needs to do some quantitative analysis
on the specimen.

We have been considering trying to embed it in a plastic resin and section
it on a microtome instead. I am not sure which plastic resin would be best
in this application. Also can we use plastic with 3 inch diameter cores or
would we have to divide the cores into quadrants.

I am hoping some of the materials people may be able to help me get on the
right path. Thanks for your help.

Cheryl Rehfeld
Meyer Instruments, Inc.
281-579-0342
e-mail csr-at-meyerinst.com

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 14:24:20 2004

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I agree with most of the posts presented so far. I did want to offer a few
more thoughts on quantitative analysis.

First, it seems like precious few people know how to do good quantitative
EDS these days. Or maybe I should say that few people are aware of the many
possible pitfalls. Most issues are rather common sense if one stops to
think about it; however, it is so darn easy to push the quantify button on
an EDS system without thinking about where the numbers come from and what
might have happened along the way.

Let me also say up front that I think most EDS manufacturers probably have
decent quantitative analysis routines. I don't think the problem is
necessarily in the software. It is usually a problem of not using it
correctly. Again, systems have become dreadfully easy to use and a novice
user can crank out results. Some of them might even be right.

Current PCs offer plenty of CPU storage and memory that allow for all kinds
of neat tricks. They can afford the new operator the benefit of a lot of
previous expertise. But I don't think that should absolve the new user of
the task of learning many of those principles themselves, such as properly
identifying the elements present.

You mentioned using "Oxford-type software". I have no idea what that means.
I am still using Oxford's ISIS suite of programs, but that doesn't mean
much to the EDAX or Noran users out there. You will have to describe what
you mean by that.

It seems one main question for your sample is where are the x-rays being
generated? You say you might have some Fe in your inclusion which
complicates the issue. I agree with the suggestion to use a program like
Electron Flight Simulator to model the interaction volume. You might
benefit from cutting back on your beam voltage. (You didn't tell us what
you were using.) Even if your beam only penetrates 1 um and your inclusion
is 3 um in diameter, you don't really know how thick a layer of inclusions
you have left on any given inclusion.

You also did not say if you were using spot mode on the center of the
inclusion or using a raster. Spot mode might be better in this case as the
raster will approach the edge of the inclusion and fluoresce more
neighboring Fe.

Your inclusion is definitely non-conductive. If left as is, the inclusion
will probably charge and deflect the beam onto the steel around it.
Variable pressure SEM was suggested as one possible remedy for dealing with
the charging problem and someone already stated that will lead to
scattering of the beam and fluorescence of the neighboring Fe. That is
probably not a good idea in your case unless you can collect data at a
variety of pressures and try to extrapolate back to 0 pressure. The
suggestion was also made to coat the sample with something conductive and
then ignore that element in the analysis. I have done that, but still you
must be careful. I use a layer of evaporated (not sputtered or flashed) C
on my standards. I have seen a measurable change in intensity as a result
of the C layer. If you are using your analysis total to judge the results,
you need to be aware that the coating will change the total.

You may wish to try the following exercise for sake of learning more about
your system. Try performing a linescan across a large inclusion. Our ISIS
software allows for a quick intensity linescan. A couple of minutes is
enough to produce a fairly good scan under our conditions. I make sure to
include a background window for reference. In this case, I would set one
close to Fe. You could also do point analyses across the interface, but
that would take longer. Then look to see how quickly and how much the Fe
level drops as you scan across the inclusion. If you reach a flat bottom on
the Fe scan then you might be sure that you have avoided influence from the
surrounding steel, if not, then you know your x-rays are not from the
inclusion only.

You said your totals do not equal 100%. That definitely requires more
information. I think most casual users simply select the normalize function
so their totals always come out to 100%. You have not done that, but what
does your system do for standards and for matrix corrections? If your
spectra were not collected under the same conditions (voltage, beam
current, coating, geometry, etc) as your standards, then the totals cannot
be expected to match. Then there is an issue of having a standard close in
composition to your unknown. Errors in the matrix correction can then
partially cancel out. However, I do not know the particulars of your system.

I will add that I was caught by surprise trying to analyze a sample which
had small Si inclusions in Al. I tried bending the rules to take an overall
analysis of the mixture at low magnification. The results were grossly in
error. It turned out that there is a strong linkage between Al and Si in
the matrix correction, but my sample had little interaction between the two
elements in practice. I basically had domains of pure Si and pure Al, yet
the matrix correction assumed a homogeneous mixture and calculated
accordingly, but in error. I had enabled normalization, but my total would
have been far off from 100% even if I was operating at the same beam
current. That could have tipped me off that something was wrong, in this
case, a lack of homogeneity.

I apologize for the long note, but I hope it is helpful.

Warren

At 09:26 PM 3/9/2004, you wrote:

} Dear listers,
}
} I am analysing polished sections containing small (3 -10µm), globular,
} calcium aluminium oxide inclusions in a steel matrix. Naturally the
} analysis totals are high as the surrounding steel influences my oxide
} analysis. Is there a way/formula of determining how much metallic steel
} is being measured and thus removing it from the results (even though there
} may be up to 4% iron oxide present)? I have noticed that the amount of
} iron present is almost equal to the amount that the total exceeds 100. Is
} it that simple? Does the presence of metallic steel in the analysis
} affect the ratio of oxides present?
}
} Thank you,
}
} Jodi Reynolds.

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You can find useful information on manufacturers sites,
for example
http://www.microstartech.com/
http://www.emsdiasum.com/Diatome/diamond_knives/default.htm

45 degrees knives are used for routine work.

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

} -----Original Message-----
} From: Andre Dufresne [mailto:dufresne-at-Ms.UManitoba.CA]
} Sent: Thursday, March 11, 2004 1:43 PM
} To: microscopy-at-ns.microscopy.com
} Subject: [Microscopy] Diamond Knife
}
}
}
}
} --------------------------------------------------------------
} ----------------
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} of America
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}
}
} A grad student working with plant tissue in our labs wants to
} purchase
} a diamond knife. Supplier catalogs indicate different specification
} when you purchase a knife for TEM ultra-structure. When
} cutting plant
} tissue I use a "knife angle" 4 degrees an obtain great results. My
} question concerns the manufactures description of a 35 or 45 degree
} knife. Is this the angle of the diamond mounted in the boat ?
} Knowing we plan to cut plant tissues imbedded in spurr, what angle
} knife would you suggest we select and why (35 or 45) ? If anyone can
} also give me a good reference for diamond knives and cutting
} that would
} be great.
}
} If you wish you can forward your emails directly to
} dufresne-at-ms.umanitoba.ca
}
} Thanks,
} André
}
}
}

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I would talk to at least two experts in the field before you try
anything. By expert I mean someone with real credentials who works in
the field, not some advice you get over the internet.
My understanding is that coins are not supposed to be cleaned, period.

Geoff

Edward Haller wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

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Your 4 degrees is the clearance angle...the angle at which the entire
knife sits in the stage (sets the "attack" angle of the knife edge
and that keeps the block from dragging down the back of the knife as
it passes). I was taught to set glass knives at 4 degrees, and most
of the diamond I've had over the years were designed to work best at
6. The manufacturer's 35 or 45 degrees refers to angle of the bevel
of the knife edge itself. I use an ultra-45 for animal-based
biological work. I don't know which would be better for plant
material.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 15:43:56 2004

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I second Geoff McAuliffe's opinion.

You are well advised to consult a maritime archaeological conservator before you do
anything to the coins.

The last thing archaeologists want is for them to be made bright and shiny.

cheers

rtch

Date sent: Thu, 11 Mar 2004 12:45:22 -0500
} From: Edward Haller {ehaller-at-hsc.usf.edu}
Send reply to: ehaller-at-hsc.usf.edu
To: microscopy-at-msa.microscopy.com

I have been seeing some of the comments on diamond knives and thought I
would share my recent experience with the new vibrating diamond knife from
Diatome (i am happy customer with no financial interest). This knife is
fantastic. It significantly reduces compression and i get a lot less
chatter in some of my hard to cut blocks (either plant seed material or
lymphoid tissue). I cut a mix of either Lowicryl K4M, LR Gold and epoxy
resin blocks. It works well with all of them. It is a little early to say
but I think I am getting less tearing and holes in sections that have
poorly infiltrated regions (e.g., starch grains in maize endosperm). The
concept of a diamond knife was first proposed by Daniel Studer and he has a
paper on it that was published about 3 years ago. So if you have the
bucks, consider one of these.

At 04:32 PM 3/11/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 17:40:34 2004

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André
Clearance angle of 4 deg indicates, your particular sample is quite hard to
cut. As smaller clearance angle or actual knife angle it's less
compression in your sections (better). From this point of view, 35 deg
knife should serve you better. From another hand, 35 deg diamond knife is
quite fragile: its easier to damage such knife, than "normal" 45 deg
knife. If the person, who is going to use knife is novice, I would suggest
45 deg. 35 deg knife is for "profi" in my opinion. I hope it may
help. Sergey

At 11:43 AM 3/11/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 11 23:03:38 2004

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André
Clearance angle of 4 deg indicates, your particular sample is quite hard to
cut. As smaller clearance angle or actual knife angle it's less
compression in your sections (better). From this point of view, 35 deg
knife should serve you better. From another hand, 35 deg diamond knife is
quite fragile: its easier to damage such knife, than "normal" 45 deg
knife. If the person, who is going to use knife is novice, I would suggest
45 deg. 35 deg knife is for "profi" in my opinion. I hope it may
help. Sergey

At 11:43 AM 3/11/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 00:18:33 2004

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A grad student working with plant tissue in our labs wants to purchase
a diamond knife. Supplier catalogs indicate different specification
when you purchase a knife for TEM ultra-structure. When cutting plant
tissue I use a "knife angle" 4 degrees an obtain great results. My
question concerns the manufactures description of a 35 or 45 degree
knife. Is this the angle of the diamond mounted in the boat ?
Knowing we plan to cut plant tissues imbedded in spurr, what angle
knife would you suggest we select and why (35 or 45) ? If anyone can
also give me a good reference for diamond knives and cutting that would
be great.

If you wish you can forward your emails directly to
dufresne-at-ms.umanitoba.ca

Thanks,
André

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 00:35:24 2004

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Hello,

I have a customer that needs to section drilling mud core samples using a
cryostat. He is using a tungsten carbide knife and the sections are 30
microns thick. The problem is that no matter what we try, tape or plastic
tubing, the section falls apart. He needs to do some quantitative analysis
on the specimen.

We have been considering trying to embed it in a plastic resin and section
it on a microtome instead. I am not sure which plastic resin would be best
in this application. Also can we use plastic with 3 inch diameter cores or
would we have to divide the cores into quadrants.

I am hoping some of the materials people may be able to help me get on the
right path. Thanks for your help.

Cheryl Rehfeld
Meyer Instruments, Inc.
281-579-0342
e-mail csr-at-meyerinst.com

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 03:24:31 2004

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Hi

Have you looked at any other LASER microdissection systems? We use a PALM
set-up and are very pleased with it. See

www.palm-microlaser.com

Note - I have no commercial connection with PALM or any of its associates.

} Our facility is in the process of acquiring an Arcturus LCM system. We
} have been given a preview of both systems by an Arcturus
} representative. But we are in need of some advice from investigators
} who have used either the PixCell IIe and/or the AutoPix systems. Any
} information regarding the advantages or disadvantages of each system
} would be appreciated. Particular issues that concern us and would
} appreciate any response on are:
}
} Ease of use
} Initial set up time for each of the systems
} Resolution of each system
} Sampling time for Proteomics and purity of samples for downstream
} processing for ex. 50 to 500 samples
} Can the template for the AutoPix be saved for future use?
} Reliability of both hardware and software
} Maintenance costs for each system.
}
} Thank you in advance for your feedback.
}
} aruna

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 07:09:02 2004

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We seem to be a bit hostile to this request. Before we get too upset, we
should remember there is a difference between cleaning coins and restoring
coins. I have recently rediscovered my childhood hobby of coin collecting
and from what I read cleaning coins is still (after more than 30 years of
not collecting) a hot topic.

Maybe the best advice this group can give is to provide referrals to
experts.

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 07:16:46 2004

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Hi all,
We had a superconductor named YBCO (Y1Ba2Cu3O7-x)(ceramic)with transition
temperature 91 K.
We put it on sem without coating and got good result below x17 000
magnifications. I coated it with carbon and now we get good results on x25
000 magnifications (I think the limit of our Sem-Cameca Su-30).

That was a superconductor but we had to coat it. The contamination on the
surface of material (which can not be seen with naked eye)may result that. I
just wanted to share my experience with you. All interpretations are
wellcome.

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
SEM Laboratory

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 14:25:33 2004

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Hi,

My two cents. I have worked with plant materials for many years. Using
standard 45 D-knife and UltraCut E Microtome$B!J(BReichert-Jung) I haven$B!G(Bt
had any problem with the standard 45 to cut Epon/standard, Epon/Araldit
mix, Spur and LR White plastics. I haven$B!G(Bt tried 35 Degree D-Knife and
have no right to say which one is better than the other.

Haixin Xu
Biological Sciences
Univ. of Maryland Baltimore County

white
-----Original Message-----
} From: Leona Cohen-Gould [mailto:lcgould-at-med.cornell.edu]
Sent: 2004$BG/(B3$B7n(B11$BF|(B 16:33
To: Andre Dufresne; microscopy-at-ns.microscopy.com

Your 4 degrees is the clearance angle...the angle at which the entire
knife sits in the stage (sets the "attack" angle of the knife edge
and that keeps the block from dragging down the back of the knife as
it passes). I was taught to set glass knives at 4 degrees, and most
of the diamond I've had over the years were designed to work best at
6. The manufacturer's 35 or 45 degrees refers to angle of the bevel
of the knife edge itself. I use an ultra-45 for animal-based
biological work. I don't know which would be better for plant
material.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 15:14:04 2004

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On Mar 11, 2004, at 9:45 AM, Edward Haller wrote:

} I'm involved in a project working with gold and silver coins recovered
} from a shipwreck. The ship went down in the 1800's. I am seeking advice
} on how to clean some of the coins in a way that will not remove any of
} the gold or silver from the coins. Some of the coins have coral on
} them,
} some have iron oxide, some cupric cloride, and some have iron sulfide
} on
} them. The sulfide is the real problem. Do any of you have suggestions
} as
} to how to clean the coins chemically? I don't have the equipment to
} clean them by electrolysis, and cannot polish them, for that would
} decrease their value. Thank you in advance for your suggestions.
}
Dear Edward,
You can wash the coins with a mild detergent without harming them, and
acetone or xylene can be used to get off grease. Do not use abrasives.
Gold is inert to many chemical treatments, but use them only if the
milder treatments do not work. Silver is more reactive than gold, so
chemical treatment would only be used as a last resort--it would
usually be right to leave a foreign material on the coins rather than
using chemical treatment to remove it. That said, some corrosion can
be dissolved with ammonia. Removing the sulfide is definitely not
recommended, since that would definitely decrease the value of the
coins. If you can reproduce the features of the contamination on some
silver coins of nominal value, you can test the effect of a proposed
treatment before using it on a much more valuable specimen. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 15:49:58 2004

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I have never used any diamond knives for semi-thin plastic sections:
0.5-0.75 microns thick, but I noticed them on the DIATOME web site today,
and I wondered what you folks might think of these knives. I really love
the idea of getting rid of glass knives once and for all, except perhaps to
rough in the blocks.

What do you people think of "histo" diamond knives for semi-thin sectioning?

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 17:27:21 2004

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My three cents (the Canadian dollar being chronically lower than the US
Greenback):

1. the 35 degree knife is an excellent knife IF USED WITH CARE. This can be
as simple as reducing the size of the block face as much as possible.

2. For soft materials, compression is indeed reduced.

3. Perhaps surprisingly, the 35 is much superior to higher knife angles at
sectioning 'hard' materials successfully, meaning useable pieces of
appropriate thickness. ('Shattering' of the section is common, but the
thickness is usually reasonably close to the set thickness, unless ultrathin
( {30 nm sections) are desired).

4. In the materials lab where I spent the greater part of my career, and
where we did a lot of contract work, our two 35's were in constant use. The
45s and a 55 collected dust.

Tom

Dr. Tom Malis
Scientist Advisor
Natural Resources Canada
Govt. of Canada
Phone: 613-995-7358
cell: 613-371-4577
FAX: 613-947-6606
malis-at-nrcan.gc.ca

-----Original Message-----
} From: Haixin Xu
To: 'Leona Cohen-Gould'; 'Andre Dufresne'; microscopy-at-ns.microscopy.com
Sent: 3/12/2004 10:16 AM

Hi,

My two cents. I have worked with plant materials for many years. Using
standard 45 D-knife and UltraCut E Microtome(Reichert-Jung) I haven?t
had any problem with the standard 45 to cut Epon/standard, Epon/Araldit
mix, Spur and LR White plastics. I haven?t tried 35 Degree D-Knife and
have no right to say which one is better than the other.

Haixin Xu
Biological Sciences
Univ. of Maryland Baltimore County

white
-----Original Message-----
} From: Leona Cohen-Gould [mailto:lcgould-at-med.cornell.edu]
Sent: 2004?3?11? 16:33
To: Andre Dufresne; microscopy-at-ns.microscopy.com

Your 4 degrees is the clearance angle...the angle at which the entire
knife sits in the stage (sets the "attack" angle of the knife edge
and that keeps the block from dragging down the back of the knife as
it passes). I was taught to set glass knives at 4 degrees, and most
of the diamond I've had over the years were designed to work best at
6. The manufacturer's 35 or 45 degrees refers to angle of the bevel
of the knife edge itself. I use an ultra-45 for animal-based
biological work. I don't know which would be better for plant
material.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 12 18:10:00 2004

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It's just simply great. I used to make huge 1.5 um semithin sections from
the whole mouse brain (coronal) and it was nightmare with glass. Then I
was trying tungsten carbide - sections were milky and did not stick well to
the glass slide (and yes, very scratchy). I think, histo-knife is great
for semithin. Sergey

At 02:05 PM 3/12/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Mar 13 10:40:27 2004

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Dear fellow microscopists

I have used "histology" diamond knives very successfully for many
years for semi-thin sectioning and for sectioning of hard (materials
science) specimens. That being said, such knives are manufactured by
several companies, and there can be substantial differences in
quality between "brands."

best regards,
Steven Slap

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Hi Karen
We have a Pelco Microwave with a coolspot and a vaccum chamber. If we
have all the chemicals made up and ready to go (including the resin)
we can go from fixing and cutting in 2 hours. The results are as if
we had done it conventionally. The resin is an Epon-Spurr mix and
usually cuts easier than Epon alone.
Elaine

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--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

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Hi

Have you looked at any other LASER microdissection systems? We use a PALM
set-up and are very pleased with it. See

www.palm-microlaser.com

Note - I have no commercial connection with PALM or any of its associates.

} Our facility is in the process of acquiring an Arcturus LCM system. We
} have been given a preview of both systems by an Arcturus
} representative. But we are in need of some advice from investigators
} who have used either the PixCell IIe and/or the AutoPix systems. Any
} information regarding the advantages or disadvantages of each system
} would be appreciated. Particular issues that concern us and would
} appreciate any response on are:
}
} Ease of use
} Initial set up time for each of the systems
} Resolution of each system
} Sampling time for Proteomics and purity of samples for downstream
} processing for ex. 50 to 500 samples
} Can the template for the AutoPix be saved for future use?
} Reliability of both hardware and software
} Maintenance costs for each system.
}
} Thank you in advance for your feedback.
}
} aruna

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Garry

We've used histoknives from both Diatome and Drukker with great success
cutting sections from 300 nm up to 2 microns thick and block faces
several mm wide. One reservation we had when we first started was the
life span of the edge. However this has not been a problem and we find
we can get a few years use out of a knife (mainly resin embedded plant
material)

Ian

} } } Garry Burgess {GBurgess-at-exchange.hsc.mb.ca} 13/03/2004 11:05:22
} } }

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I have never used any diamond knives for semi-thin plastic sections:
0.5-0.75 microns thick, but I noticed them on the DIATOME web site
today,
and I wondered what you folks might think of these knives. I really
love
the idea of getting rid of glass knives once and for all, except
perhaps to
rough in the blocks.

What do you people think of "histo" diamond knives for semi-thin
sectioning?

Ian Hallett
HortResearch
Mt Albert Research Centre, Private Bag 92 169
Auckland, New Zealand
Fax +64 9 815 4201
Telephone +64 9 815 4200
EMail ihallett-at-hortresearch.co.nz

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From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 02:32:40 2004

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I got a wide 'histo' diamond when starting a project involving lots of
mouse bone work. It is obviously much more forgiving to those in which
the decalcification was not quite complete. I roughly trim them all on
glass then pop the diamond in to take a good face off the whole batch. I
think histo diamonds are a real boon and well worth the money.

Gill Brown
Histopathology Group
GlaxoSmithKline Medicines Research Centre,
Gunnelswood Road,
STEVENAGE,
Hertfordshire.
SG1 2NY
tel. +44 (0)1438 764119
fax. +44 (0)1438 764782
email. gillian.2.brown-at-gsk.com

----- Forwarded by Gillian 2 Brown/PharmRD/GSK on 15-Mar-2004 08:37 -----

"Garry Burgess" {GBurgess-at-exchange.hsc.mb.ca}

12-Mar-2004 22:05

To: Microscopy

cc:
Subject: [Microscopy] Histo Diamond Knife for Semi-thin sections

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I have never used any diamond knives for semi-thin plastic sections:
0.5-0.75 microns thick, but I noticed them on the DIATOME web site today,
and I wondered what you folks might think of these knives. I really love
the idea of getting rid of glass knives once and for all, except perhaps
to
rough in the blocks.

What do you people think of "histo" diamond knives for semi-thin
sectioning?

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 07:23:37 2004

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I have used vinegar to dissolve calcium from sea cucumber and egg shell.
It can be used for cleaning coral on gold coin. For other coins, I don't
know. Good luck

Ann Fook

} } } Bill Tivol {tivol-at-caltech.edu} 03/12/04 02:29PM } } }

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On Mar 11, 2004, at 9:45 AM, Edward Haller wrote:

} I'm involved in a project working with gold and silver coins
recovered
} from a shipwreck. The ship went down in the 1800's. I am seeking
advice
} on how to clean some of the coins in a way that will not remove any
of
} the gold or silver from the coins. Some of the coins have coral on
} them,
} some have iron oxide, some cupric cloride, and some have iron sulfide

} on
} them. The sulfide is the real problem. Do any of you have suggestions

} as
} to how to clean the coins chemically? I don't have the equipment to
} clean them by electrolysis, and cannot polish them, for that would
} decrease their value. Thank you in advance for your suggestions.
}
Dear Edward,
You can wash the coins with a mild detergent without harming
them, and
acetone or xylene can be used to get off grease. Do not use abrasives.

Gold is inert to many chemical treatments, but use them only if the
milder treatments do not work. Silver is more reactive than gold, so
chemical treatment would only be used as a last resort--it would
usually be right to leave a foreign material on the coins rather than
using chemical treatment to remove it. That said, some corrosion can
be dissolved with ammonia. Removing the sulfide is definitely not
recommended, since that would definitely decrease the value of the
coins. If you can reproduce the features of the contamination on some

silver coins of nominal value, you can test the effect of a proposed
treatment before using it on a much more valuable specimen. Good
luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 08:01:55 2004

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Garry,
I haven't cut anything with glass in YEARS! (except when I'm teaching
someone how to section). I wouldn't be without a Histo knife.
Period.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 10:13:19 2004

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This is reckless, as copper that is part of the alloys will be attacked and in the
presence of salt (these are salt water archeological finds) may form
chloride-acetate double salts that later unduce further corrosion or efflorescence
problems. The long term results of various cleaning methods have been studied by
individuals with experience in handling archaeological finds and the benefits and
detriments are known. The cleaning of marine archaeological finds should be left
to a professional conservator with experience in dealing with salt contaminated
corrosion.

John Twilley
Conservation Scientist

Ann-Fook Yang wrote:

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} I have used vinegar to dissolve calcium from sea cucumber and egg shell.
} It can be used for cleaning coral on gold coin. For other coins, I don't
} know. Good luck
}
} Ann Fook
}
}
} On Mar 11, 2004, at 9:45 AM, Edward Haller wrote:
}
} } I'm involved in a project working with gold and silver coins
} recovered
} } from a shipwreck. The ship went down in the 1800's. I am seeking
} advice
} } on how to clean some of the coins in a way that will not remove any
} of
} } the gold or silver from the coins. Some of the coins have coral on
} } them,
} } some have iron oxide, some cupric cloride, and some have iron sulfide
}
} } on
} } them. The sulfide is the real problem. Do any of you have suggestions
}
} } as
} } to how to clean the coins chemically? I don't have the equipment to
} } clean them by electrolysis, and cannot polish them, for that would
} } decrease their value. Thank you in advance for your suggestions.
} }

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 11:29:28 2004

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I have been using DDk diamond knives to do cryo-ultra-thin cutting of
plastics for AFM phase imaging. I found knife damages developed as soon as
cut the first sample. I used 35-D first and then 45-D angle knives and saw
the same problem. I think I might need to try a Diatome knife now. Can
anybody comment on the qualities between DDK and Diatome knives?

Thank you very much.

Jiang Liu, PhD
Microscope Lab Supervisor
Atofina Petrochemicals
R&T Center.
La Porte, TX.

} From: Tom Phillips {phillipst-at-missouri.edu}
} To: Microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Re: Re: Diamond Knife
} Date: Thu, 11 Mar 2004 17:42:37 -0600
}
}
}
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_________________________________________________________________
Fast. Reliable. Get MSN 9 Dial-up - 3 months for the price of 1!
(Limited-time Offer) http://click.atdmt.com/AVE/go/onm00200361ave/direct/01/

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 11:33:22 2004

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John brings to mind a good point. We can't assume
that these coins are pure silver or pure gold. Given
1800's metallurgy, I'd be amazed if the coins were
"pure anything". The coins could easily contain
microinclusions and secondary intermetallic phases
which may react badly to any chemical cleaning
methods.

Stu Smalinskas
Metallurgist

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Edward Haller wrote:
I'm involved in a project working with gold and silver
coins recovered from a shipwreck. The ship went down
in the 1800's. I am seeking advice on how to clean
some of the coins in a way that will not remove any of
the gold or silver from the coins. Some of the coins
have coral on them, some have iron oxide, some cupric
chloride, and some have iron sulfide on them. The
sulfide is the real problem. Do any of you have
suggestions as to how to clean the coins chemically? I
don't have the equipment to clean them by
electrolysis, and cannot polish them, for that would
decrease their value. Thank you in advance for your
suggestions.

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Ann wrote:
I have used vinegar to dissolve calcium from sea
cucumber and egg shell. It can be used for cleaning
coral on gold coin. For other coins, I don't know.
Good luck

Ann Fook

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

John wrote:
This is reckless, as copper that is part of the alloys
will be attacked and in the presence of salt (these
are salt water archeological finds) may form
chloride-acetate double salts that later unduce
further orrosion or efflorescence problems. The long
term results of various cleaning methods have been
studied by individuals with experience in handling
archaeological finds and the benefits and detriments
are known. The cleaning of marine archaeological
finds should be left to a professional conservator
with experience in dealing with salt contaminated
corrosion.

John Twilley
Conservation Scientist

__________________________________
Do you Yahoo!?
Yahoo! Mail - More reliable, more storage, less spam
http://mail.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 13:31:01 2004

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When you take a picture of anatase particles distributed on a carbon film,
cells adhering to a substrate, or even crystals on Mars, the resulting
image is just the first step toward better understanding of the world. It
doesn't matter whether your "picture" is on photographic film, within a
digital file, or even presented as some other record of light, electrons,
x-rays, or other phenomena, it can and should be analyzed to extract
quantitative scientific facts. The picture is the art; the analysis is the
science.

The New England Society for Microscopy and the Connecticut Microscopy
Society announce that pre-registration has opened for the Image Processing
Workshop to be held Thursday April 29th. 2004, at Woods Hole, MA.

Details may be found at
{http://www.msa.microscopy.com/MSALAS/NESM/NESMHome.htm} http://www.msa.microscopy.com/MSALAS/NESM/NESMHome.htm

Navigate to "Future Meetings".

Initial details about the NESM/CMS Spring Symposium, to be held following
the Image Processing Workshop on April 30th. and May 1st., also at Woods
Hole, are also available on the same web site. Full details of the Spring
Symposium will be available before the end of March.

********************************************

Anthony J. Garratt-Reed, M.A., D.Phil.
Manager, Shared Experimental Facilities
Center for Materials Science and Engineering
Room #13-1027
Massachusetts Institute of Technology,
77 Massachusetts Avenue
Cambridge, Massachusetts 02139-4307
USA

Phone: 617-253-4622
Fax: 617-258-6478
********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 13:57:36 2004

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Steve is quite right. Some years ago, we evaluated a number of histos from
different companies on a variety of materials (Al alloy, Al-SiC composite,
etc) and found that some cut nearly as good as a conventional diamond knife,
while others performed poorly. Even the best of them left a lot of fine
knife marks, though, sometimes covering the entire section, leading us to
wonder if the knife edge was somehow serrated.

On the other hand, there were some pleasant surprises. A year or so later,
we had a request to section largish (10-20 micron) particles of an
amorphous Fe-Nd-B intermetallic used for magnets. It chewed up the edge of
all the conventional knives - 35. 45 and 55 - yet a histo (Diatome, if
memory serves) produced decent 30 nm thick sections with no edge damage!
Ever since, as Steve notes, we first use a histo on any 'hard' material with
which we are unfamiliar.

Finally, in another series of tests, we were able to cut 1 micron semithin
sections of Al alloy with no knife damage. Intriguingly, ultrathin
sectioning of the same alloy showed no 'curling' of the sections (due to
residual stress buildup) that can be such a headache when sectioning metals.
No idea why, unless the above hypothetical serrated edge somehow evened out
the strain buildup.

So, if one has a variety of materials to section, including many that are
'hard' in nature, investing in a histo might be wise so long as you are
prepared for the variability Steve mentions.

Tom

Dr. Tom Malis
Scientist Advisor
Natural Resources Canada
Govt. of Canada
Phone: 613-995-7358
cell: 613-371-4577
FAX: 613-947-6606
malis-at-nrcan.gc.ca

-----Original Message-----
} From: Steven E. Slap
To: Garry Burgess
Cc: Microscopy-at-sparc5.microscopy.com
Sent: 3/13/2004 11:56 AM

Dear fellow microscopists

I have used "histology" diamond knives very successfully for many
years for semi-thin sectioning and for sectioning of hard (materials
science) specimens. That being said, such knives are manufactured by
several companies, and there can be substantial differences in
quality between "brands."

best regards,
Steven Slap

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From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 14:17:14 2004

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Group,

I am looking for a hand tool that could press dry fine powder samples into a tablet with a surface that would be suitable for EDS analysis in an SEM. I have looked at things like KBr pellet makers but not sure that would work for this application. Any ideas would be appreciated.

Roy Beavers

Southern Methodist University
Department of Geological Sciences
P.O. Box 750395
Dallas, Tx 75275
Voice: 214-768-2756
Fax: 214-768-2701
Email: rbeavers-at-mail.smu.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 16:13:12 2004

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There are my 3 canadian cents to this thread (equivalent to 2 US cents).

There is a great FREE software for simulating the interactions "primary
electrons -matter" and subsequent XR emission.
The program can be downloaded from http://www.gel.usherb.ca/casino/ .
This software can simulate multilayered sample as well as bi-materials with
an interface perpendicular to the scanned surface. It might be vey useful
for studying inclusions in steel.

Good luck.

Jean-Paul Baďlon

++++++++++++++++++++++++++++++++++++++
Prof. Jean-Paul Baďlon jean-paul.bailon-at-polymtl.ca
Mathématiques Tél: +1(514) 340 4711, p. 4260
et Génie industriel Fax: +1(514) 340 4468
École Polytechnique
CP 6079, Succursale Centre-Ville
Montréal (QC) Canada H3C 3A7
++++++++++++++++++++++++++++++++++++++

-----Message d'origine-----
De : Reynolds, Jodi JI [mailto:ReynoldsJ-at-OneSteel.com]
Envoyé : 10 mars, 2004 16:59
Ŕ : Larry Hanke
Cc : Microscopy (E-mail)
Objet : RE: RE: SEM metallography

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Hi Larry,

I generally, but not always, use an ultra sonic bath to clean the samples
before analysis, do you think this is effective? I'd like to try the
acetate tape method and pull the inclusions out, but you're right about the
possibility of the incusions taking some of the steel with them. This would
be obvious straight away I imagine and perhaps some of the inclusions would
be free of steel matrix residue.

Thank you for your help,

Jodi.

-----Original Message-----
} From: Larry Hanke [mailto:hanke-at-mee-inc.com]
Sent: Thursday, 11 March 2004 3:02 AM
To: MSA listserver
Cc: Reynolds, Jodi JI

Yes, but the point is that by cleaning them you destroy all of the information about what
happens to coins in that marine environment.

An experienced marine archaelologist or archaeological conservator should be brought
into the project.

cheers

rtch

Date sent: Mon, 15 Mar 2004 09:52:16 -0800 (PST)
} From: Kestutis Smalinskas {smalinskas-at-yahoo.com}

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (dvanoekelen-at-omnilabo.be) from on Monday, March 15, 2004 at 01:30:08
---------------------------------------------------------------------------

Email: dvanoekelen-at-omnilabo.be
Name: Van Oekelen

Organization: Omnilabo

Title-Subject: [Microscopy] [Filtered] SEM from

Question: Dear Microscopists,

I know there are a lot of specialists regarding the use of SEM. Therefore, I was hoping that someone could help me finding a beautiful SEM image of a salt crystal.

Thank you very much for your time and help.

Best regards,
Dirk

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What kind of salt? I have marine salt, table
salt and Kosher salt. All look different.

What resolution and what useage?

gary g.

At 03:06 PM 3/15/2004, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 17:53:26 2004

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We recently removed the cover to do some maintenance on our MT2B microtomes. During the process I noticed that the set screw holding the knob to the pivot control screw was loose. When we reassembled the microtome and began cutting sections it became obvious that the upper thickness control was not in proper alignment. Previously we set the upper thickness at 10 to get silver sections. Not anymore. Does anyone know the procedure for realigning the upper thickness control knob? Or, does any one have a service manual that describes the procedure? You may email me directly or post on the list server.

Bob
Robert J. Schmitz
Department of Biology
University of Wisconsin Stevens Point
Stevens Point, WI 54481
715-346-2420 FAX 715-346-3624
Email: rschmitz-at-uwsp.edu
http://biology.uwsp.edu/faculty/RSchmitz/Default.htm

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 18:37:27 2004

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HB-501 for sale. If interested, please contact me off line.

John C. Wheatley
Lab Manager
Arizona State University
Center for Solid State Science
PSA-213
BOX 871704
Tempe, AZ 85287-1704

Phone: (480) 965-3831
FAX: (480) 965-9004
John.Wheatley-at-ASU.Edu

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 18:50:20 2004

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To all experts out there:
I was checking to see if anyone out there has been successful in
changing a freon insulated HV tank (ours is a 200 KV JEOL) to SF6 gas
(with or without outside assistance). If so, please let me about the
success of your experience and what internal/external components you may
changed and how it went...and if possible, please offer me any advice in
the process.
Thanks,
Michael Coveillo

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 15 19:35:58 2004

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Michael,
The National Center for Electron Microscopy {http://ncem.lbl.gov/} converted a JEOL
ARM-1000 from freon to SF6 several years ago. Someone there should be able to
answer your question.
Mike O'Keefe

coviello wrote:

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} To all experts out there:
} I was checking to see if anyone out there has been successful in
} changing a freon insulated HV tank (ours is a 200 KV JEOL) to SF6 gas
} (with or without outside assistance). If so, please let me about the
} success of your experience and what internal/external components you may
} changed and how it went...and if possible, please offer me any advice in
} the process.
} Thanks,
} Michael Coveillo

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 07:44:31 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 16, 2004 at 07:33:48
---------------------------------------------------------------------------

Email: kssim-at-mmu.edu.my
Name: ks

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear All,

Currently, I am trying to interface JEOL SEM 840A model with DT3152. I appreciate those who have experience to interface SEM with DT3152, on how to tap the signal scan x, sacn y and videos signal and connect to DT3152. Please kindly send email to me and supply me with information.

thanks
kok swee

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Hi all!

Someone asked me about how to assess the purity of a preparation of
yeast mitochondria on a sucrose gradient. As I have no experience of
this myself, I would be very glad if you could help me out. Should we
do it with EM or would an approach with fluorescent markers for
mitochondria do a better job?

Thanks,
Stefan

+++++++++++++++++++++++++++++++++++++++++++++++++++++++
Dr Stefan Gunnarsson
Evolutionsbiologiskt Centrum Evolutionary Biology Centre
Enheten för biologisk strukturanalys Microscopy and Imaging Unit
Norbyvägen 18A
SE75236 Uppsala, Sweden Tel & Fax: +46 - 18 471 2638
+++++++++++++++++++++++++++++++++++++++++++++++++++++++

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 09:07:19 2004

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Colleagues:

List members who have an interest in materials science are cordially invited to a free two-day "mini-workshop" on cryoultramicrotomy for the materials sciences. This topic is of special interest for those who work with polymers or other materials which could benefit from ultrathin sectioning or surface "polishing" at low temperatures (no embedding required).

This invitation is extended to persons who are located in the greater Philadelphia/Baltimore/Washington, D.C./New York City area. The workshop will be hosted by the Center for Advanced Scientific Imaging (CASI) at West Chester University of Pennsylvania.

The details are as follows:

**What**:
Mini-Workshop on Cryoultramicrotomy for Materials Science

**When**:
Tuesday, March 30, 2004, 11:00 am through Wednesday, March 31, 2004, 4:00 pm.

Visitors are invited to arrive early on Tuesday, March 30 for tours of the Center for Advanced Scientific Imaging. The lab will be open at 8:00 am on Tuesday.

**Where**:
West Chester University of Pennsylvania, Schmucker Science Center South, Room SSS017. Schmucker Science Center South is located on the corner of South Church Street and Rosedale Avenue in West Chester, PA. West Chester is located approximately 30 miles from Philadelphia.

**Format**:
A presentation on cryoultramicrotomy and its applications in the materials sciences will be given on the first day, as well as demonstrations on the preparation of cryotools (hair probes, large and small wire loops, etc.) and glass knife making and evaluation. The care and cleaning of diamond knives will also be discussed.

The demonstrations will be followed by open lab sessions for the attendees to prepare their own cryotools and glass knives.

Also on the first day an introduction to the cryoultramicrotome will be given, and attendees will have an opportunity for hands-on use of the instrument.

The second day will be reserved for attendees to sign up in small groups for additional time and training on the instrumentation, depending on the attendees' individual needs.

**Limited Space Available**:
The lectures and demonstrations on the first day are open to everyone, but space is limited to *10 persons* for the in-depth training and extended use of the instrumentation on the second day.

**Contacts**:
To RSVP or to reserve a seat for the second day's sessions, please contact any of the following people:

Dr. Fred Monson, CASI / West Chester University of Pennsylvania, 610.738.0437, {fmonson-at-wcupa.edu}

Dr. Robert Chiovetti, RMC Products / Boeckeler Instruments, Inc., 520.745.0001, {bob-at-boeckeler.com}

Ms. Kim Megaw, RMC Products / Boeckeler Instruments, Inc., 520.745.0001, {kim-at-boeckeler.com}

We hope to see you soon in West Chester!

Robert (Bob) Chiovetti
RMC Products
Boeckeler Instruments, Inc.
{bob-at-boeckeler.com}
{rchiovetti-at-aol.com}

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 09:28:14 2004

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I have recently encountered a problem I've not dealt with before. I'm
putting cover slips on thin sections of geode materials using Permount.
When first covered, they are fine, but within 24 hours they develop tiny
grains in the Permount, but only over certain mineral grains (usually quartz
grains that have inclusions of anhydrite). I'm stumped as to what may be
causing this. My only recourse at present is to clean off the cover slip,
re-mount and photograph while the Permount is fresh. Any suggestions as to
how to deal with this so it does not occur will be welcome.

Henry Barwood
Associate Professor of Science, Earth Science
Department of Math and Physics
MSCX 312G
Troy State University
Troy, Alabama 36082
hbarwood-at-troyst.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 12:00:31 2004

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This may be a stupid question, but there's no way that that an electron beam
of say, 15 or 20KeV can hurt a diamond in any way is there? I was checking
out a gemstone (unofficially - off the clock :-)for a colleague, which
turned out to be a cubic zirconium, but then I got thinking - if it had been
a diamond (carbon in crystal form)would that have been beam-sensitive in the
way that organic (carbon-based) things are? My hunch is no, but if somebody
ever asks me to check out their engagement ring to see if it's really
diamond (yes, I hear people sometimes do that ;-), I don't want to be the
guy that burns a hole in it.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: dvanoekelen-at-omnilabo.be [mailto:dvanoekelen-at-omnilabo.be]
Sent: Monday, March 15, 2004 7:07 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (dvanoekelen-at-omnilabo.be) from on Monday, March 15, 2004 at
01:30:08
---------------------------------------------------------------------------

Email: dvanoekelen-at-omnilabo.be
Name: Van Oekelen

Organization: Omnilabo

Title-Subject: [Microscopy] [Filtered] SEM from

Question: Dear Microscopists,

I know there are a lot of specialists regarding the use of SEM. Therefore, I
was hoping that someone could help me finding a beautiful SEM image of a
salt crystal.

Thank you very much for your time and help.

Best regards,
Dirk

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 12:38:13 2004

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Tom;

EDX will unlikely tell you anything about the difference between a synthetic diamond and a naturally occurring one, just in case you were thinking about going into the jewelry business. Zr is another matter, since it's elementally different than diamond, man made or natural. Regarding your question, I cannot imagine a beam current high enough in an SEM that would alter a diamond, especially with it's high thermal conductivity. Some new man-made gems are virtually indistinguishable from natural gems. It makes the diamond mining people very nervous.

I'm sure you'll hear from others on this subject.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Thomas, Frank [mailto:FThomas-at-NRCan.gc.ca]
Sent: Tuesday, March 16, 2004 1:19 PM
To: microscopy-at-ns.microscopy.com

This may be a stupid question, but there's no way that that an electron beam
of say, 15 or 20KeV can hurt a diamond in any way is there? I was checking
out a gemstone (unofficially - off the clock :-)for a colleague, which
turned out to be a cubic zirconium, but then I got thinking - if it had been
a diamond (carbon in crystal form)would that have been beam-sensitive in the
way that organic (carbon-based) things are? My hunch is no, but if somebody
ever asks me to check out their engagement ring to see if it's really
diamond (yes, I hear people sometimes do that ;-), I don't want to be the
guy that burns a hole in it.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: dvanoekelen-at-omnilabo.be [mailto:dvanoekelen-at-omnilabo.be]
Sent: Monday, March 15, 2004 7:07 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (dvanoekelen-at-omnilabo.be) from on Monday, March 15, 2004 at
01:30:08
---------------------------------------------------------------------------

Email: dvanoekelen-at-omnilabo.be
Name: Van Oekelen

Organization: Omnilabo

Title-Subject: [Microscopy] [Filtered] SEM from

Question: Dear Microscopists,

I know there are a lot of specialists regarding the use of SEM. Therefore, I
was hoping that someone could help me finding a beautiful SEM image of a
salt crystal.

Thank you very much for your time and help.

Best regards,
Dirk

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 13:38:11 2004

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Dear Frank,
I have looked at lots of diamonds, both industrial in cutting tools and our
hardness indenters. Some of them charge, but are otherwise unhurt by the beam. I
know a geologist who uses one as a substrate for WDS analysis on small grains.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Thomas, Frank" {FThomas-at-nrcan.gc.ca}
To: {microscopy-at-ns.microscopy.com}
Sent: Tuesday, March 16, 2004 10:19 AM

Hello Listers:

I have a question regarding mouse brain hippocampus which normally does not
contain any amount of IgG or IgM due to the blood/brain barrier. I am doing
immunoelectron microscopy with a gold secondary which would be silver
enhanced.

This experiment involves an injection/infection of a foreign protein
sequence attached to amplicons to induce cells from CA1 region of the
hippocampus to produce that protein. We see alot of cellular damage and the
presence of inflammatory cells at the injection site along the needle tract.
These lymphocytes and other cells involved in inflammation should produce
IgG in the area of injury.

My question is: Would the IgG present in the inflammatory cells diffuse out
into the neighboring CA1 to CA3 region? Could that cause a secondary
antibody such as gold tagged goat anti-mouse F(ab')2 IgG or IgM to also
label the surrounding normal cells(those which did not take up the foreign
protein/amplicons) some distance from the injury? I am using a mouse
monoclonal antibody to identify the infected cells which are producing this
new protein.

Thanks for your comments!

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 14:40:17 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Your local JEOL service people should be able to assist. In the UK I
think a good number of 120 kV and 200 kV TEMs have been converted.

Although I think SF6 is due to come under similar restrictions in 2-3
years. What happens then, I don't know.

I should declare an interest, as a JEOL employee.
--
Larry Stoter
NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 14:40:18 2004

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} ------------------------------------------------------------------------------
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Gallium FIB systems can certainly etch diamond (but then again, most
things can be etched in a FIB). A few years ago DeBeers were looking
at the possibility of using FIBs to put serial nos, etc on to gem
quality diamonds - a pity nothing ever came of it (too easy to remove
with a quick re-polish?) as SEM manufacturers were looking forward to
jewellers having to buy SEMs to check out diamonds :-))

I would also suggest that in some newer thermal FEG SEMs, the
electron probe current density can get very high, equivalent to
terawatts per square metre, the sort of energy densities achieved in
nuclear explosions. As has been pointed out, the thermal conductivity
of diamond is very high but I wouldn't want to be the one to discover
that this sort of energy density could damage gem quality diamonds :-)

I also recall many years ago looking at diamond in the TEM and that
it was possible, with small probes to cause damage in
electron-transparent diamond. This was thinned diamond crystals, as
opposed to DLC or any other sort of film.

I should declare an interest, as an employee of JEOL, in selling SEMs and FIBs.
--
Larry Stoter
NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 14:43:06 2004

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Frank writes ...

} This may be a stupid question, ...

That's what we're here for :o)

} but there's no way that that an electron beam of say,
} 15 or 20KeV can hurt a diamond in any way is there? ...

I am familiar with using diamond as a spectrum-free substrate for particle
analysis at typical keV and m'probe beam currents (cathodo-luminescence
being an aid over using polished vitreous carbon). They were commonly
reused, and as far as I am aware we never damaged them in any way. Still, I
believe you can feel 100% confident of using a defocused beam and lesser
beam currents. The only caveat would be respect to any possible difference
in altering the refractive index locally ... perhaps someone has possibly
noticed(?)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 15:08:34 2004

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I know that if you use the high voltage of a TEM and you have a poor vacuum with water vapor in it, you can drill holes in diamond when you focus the probe down. Don't know about SEM conditions.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Thomas, Frank [mailto:FThomas-at-nrcan.gc.ca]
Sent: Tuesday, March 16, 2004 1:19 PM
To: microscopy-at-ns.microscopy.com

This may be a stupid question, but there's no way that that an electron beam
of say, 15 or 20KeV can hurt a diamond in any way is there? I was checking
out a gemstone (unofficially - off the clock :-)for a colleague, which
turned out to be a cubic zirconium, but then I got thinking - if it had been
a diamond (carbon in crystal form)would that have been beam-sensitive in the
way that organic (carbon-based) things are? My hunch is no, but if somebody
ever asks me to check out their engagement ring to see if it's really
diamond (yes, I hear people sometimes do that ;-), I don't want to be the
guy that burns a hole in it.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: dvanoekelen-at-omnilabo.be [mailto:dvanoekelen-at-omnilabo.be]
Sent: Monday, March 15, 2004 7:07 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (dvanoekelen-at-omnilabo.be) from on Monday, March 15, 2004 at
01:30:08
---------------------------------------------------------------------------

Email: dvanoekelen-at-omnilabo.be
Name: Van Oekelen

Organization: Omnilabo

Title-Subject: [Microscopy] [Filtered] SEM from

Question: Dear Microscopists,

I know there are a lot of specialists regarding the use of SEM. Therefore, I
was hoping that someone could help me finding a beautiful SEM image of a
salt crystal.

Thank you very much for your time and help.

Best regards,
Dirk

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 15:14:23 2004

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For some years, I have been imaging electron-dense inclusion bodies in
various protozoal organisms by sticking them (unfixed, unsectioned) to
formvar and using a relatively high voltage.

Lately I have been trying to do similar imaging in fixed specimens,
because the fixation allows for the visualization of some membrane and
vacuolar structure. Unfortunately, it also adds a lot of contrast--so
much so that I often can't see the dense inclusions. I suspect this is
because the the cells shrink a bit in the fixative medium, which
renders them on the whole much more electron dense.

Any suggestions on alternative fixation procedures? I have tried
various concentrations of glutaraldehyde and paraformaldehyde both
alone and together with little luck. Or alternative TEM techniques? A
colleague mentioned in passing, for instance, trying to find a scope
with energy filtering capabilities, but I am not very familiar with
this approach.

_______________________________
Peter Rohloff, PhD
Laboratory of Molecular Parasitology
Medical Scholars Program
University of Illinois at Urbana-Champaign

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 15:24:35 2004

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Hello;

As a continuation of an earlier discussion last week; we are having a
few problems getting the resin to infiltrate into the Bundle Sheath
cells surronding vascular bundles in Ryegrass pseudostem.

We use an 812 resin and infiltrate overnight in 50/50 with Acetone and
then 100% resin; two lots at 6-12 hours each. When we cut 1 um sections
to view in LM looks OK; but then trim and polish the blockface for TEM
sections we can sometimes see minute "holes" in the face where the resin
has "fallen out" of the BS cells.

Any ideas on a possible solution to this annoying problem?

Thanks for your help

Raymond Bennett

______________________________________________________
The contents of this e-mail are privileged and/or confidential to the
named recipient and are not to be used by any other person and/or
organisation. If you have received this e-mail in error, please notify
the sender and delete all material pertaining to this e-mail.
______________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 15:51:10 2004

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Karen

unless they have changed everything in immunology over the past year,
the immunoglobulins are not going to diffuse out from the T cells, they
will be actively secreted. i suspect you knew that, however, and are
really interested in diffusion of antibodies within the surrounding
tissues. lymphocytes will perform their programmed functions, wherever
they happen to be. if they have crossed the blood brain barrier, or if
they are actually astrocytes already resident, they will still perform
their normal immunologic functions. you will get some interstitial
antibody in the neighborhood of the lymphocytes, whether in the brain or
any other tissue. if the foreign protein is to be trafficked to the
plasmalemma, then you will have a potential problem telling whether the
labelling is due to a reaction with primary mAb, or host produced
polyclonal antibodies to the foreign protein. if the foreign protein is
to be trafficked to the cell interior, then you should have less
trouble, but you still may have to deal with the question of whether the
reaction is due to the reaction of the primary mAb or host antibody
which has been taken into the cell.

having said this, all need not be lost. have your investigators
considered using human monoclonals produced in the Xenomouse model? the
mouse is transgenic and produces human immunoglobulins, not murine.
they could contact Abgenix about getting the antibody made. i do not
think they would simply sell the mice for use as models, i think they
would require you get the antibody from them or someone licensed by them
to do the work. for that matter, i do not know whether they have
actually licensed anyone, either.

no, i do not work for Abgenix, but i do know some people who wish to use
their model, and we have discussed using direct and indirect immunogold
EM with the project they wish to do.

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 16:47:42 2004

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On Mar 16, 2004, at 1:33 PM, Peter Rohloff wrote:

} For some years, I have been imaging electron-dense inclusion bodies in
} various protozoal organisms by sticking them (unfixed, unsectioned) to
} formvar and using a relatively high voltage.
}
} Lately I have been trying to do similar imaging in fixed specimens,
} because the fixation allows for the visualization of some membrane and
} vacuolar structure. Unfortunately, it also adds a lot of contrast--so
} much so that I often can't see the dense inclusions. I suspect this is
} because the the cells shrink a bit in the fixative medium, which
} renders them on the whole much more electron dense.
}
} Any suggestions on alternative fixation procedures? I have tried
} various concentrations of glutaraldehyde and paraformaldehyde both
} alone and together with little luck. Or alternative TEM techniques? A
} colleague mentioned in passing, for instance, trying to find a scope
} with energy filtering capabilities, but I am not very familiar with
} this approach.
}
Dear Peter,
Do you have the facilities for cryo-fixation? Depending on the
thickness(es) of the organisms you might have success either with
plunge-freezing--for ~ {1 um--or high-pressure-freezing followed by
cryo-substitution and sectioning or by cryo-sectioning.
Energy-filtered EM could be done either by taking a conventional image,
then acquiring spectra from areas of interest, or--probably more
usefully in your case--by acquiring an image using only elastically
scattered electrons (a zero-loss image) or electrons that have lost
energy in a window characteristic of a particular element (element
mapping). The first method will enhance contrast due to atoms heavier
than those predominant in biological molecules, and the second method
will show you where the amount of a particular element is high. A
disadvantage of element mapping is that it requires a high electron
dose, since electrons losing energies characteristic of a particular
element are a small fraction of the transmitted electrons. Energy
filtering is especially useful if the inclusions consist of element(s)
not present in large concentration(s) in the rest of the organism.
AFAIK, imaging filters are available only for scopes with HV {= 400 kV
(which may or may not include "relatively high voltage").
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 16:53:28 2004

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Cell walls can sometimes be difficult to infiltrate. We usually
dehydrate with propylene oxide after our last 100% ETOH and then use
~33% steps of resin:PO mixtures to infiltrate. A couple of hours in 33%
resin:66% PO, 4 hrs.to overnight in 66% resin : 33% PO, and the two or
three changes of 100% resin, the first overnight and the next two 6 -
12hrs. each. All infiltration steps are carried out on a sample rotator.
I do not remember, but do the BS cells have silica bodies? If so the
holes that you are seeing may be the silica bodies pulling out of the
block face. In this case you are on your own!

Raymond Bennett wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
(405)325-4391
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 18:57:10 2004

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Dear Karen
I am sorry if I don't understand you right. Many cells have Ig-like
receptors on their membranes including macrophages (I do believe). Brain
itself has a cells of macrophagal origin (glial cells for instance) and
your injury broke blood barrier, so more cells migrate to the brain (mostly
macrophages). At such background, it seems to me, you may not use
anti-mouse Ig-s as a secondary AB. It's common practice to use, for
instance, rabbit primary ABs and anti-rabbit secondary. You also need to do
negative control with secondary ABs only. Forgive me if I did not
understand your question. Sergey.

At 12:52 PM 3/16/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 16 21:07:27 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (nessonm-at-onid.orst.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 16, 2004 at 19:30:27
---------------------------------------------------------------------------

Email: nessonm-at-onid.orst.edu
Name: Michael Nesson

Organization: Oregon State University

Title-Subject: [Microscopy] [Filtered] MListserver: SiO grid films

Question: Can anyone provide a protocol for making SiO filmed gold grids? I'm planning some oxygen plasma-ashing experiments on some amorphous metal-rich biological materials. I know that I can obtain such grids from several of the EM supply houses, but I don't want to pay the prices, if I can make them myself. I have available an oil-diffusion pumped evaporator, tungsten baskets, and SiO granules.

---------------------------------------------------------------------------

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The last part of the letter listed below indicates damage to Nikon
lenses by the use of Zeiss immersion oil. Do you, Ralph, or anyone
else have instances where this has occurred? (I would suspect that
this would occur on inverted scopes most often and would be the
result of dissolving the seal between the lens and the outer case.)
If so was this the old Zeiss or the new Zeiss oil immersion medium?
I've got Nikon scopes and would like to post messages in the
appropriate rooms if this has proven to be a problem. I also have
Zeiss oil over 15 years old with no solidification problems that I've
kept hidden.

Also, does anyone know where to find small plastic 5-10 ml bottles
that would be suitable for dispensing oil immersion medium?

.. Jerry Calvin

listed 3-3-04
.. Also be aware that different types of immersion oil should never
be allowed to mix, and that some types of oil can damage the mounting
cement of some brands of lenses. Using Zeiss immersion oil with some
Nikon lenses, for example, can be disastrous.

Ralph Common
Electron Microscopist
Michigan State University
Division of Human Pathology
A608 East Fee Hall
East Lansing, MI 48824
517-355-7558; fax 517-432-1053
ralph.common-at-ht.msu.edu
--
****************************
Jerry G. Calvin
Science Support technician
Box 0731 Biology Department
Vassar College
124 Raymond Avenue
Poughkeepsie, NY 12604-0731

(845) 437-7423 - Office
(845) 437-7424 - Confocal Room
FAX: (845) 437-7315 - Biology Office
E-Mail: jecalvin-at-vassar.edu

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Second and Final Call for Papers
Michigan Microscopy &Microanalysis Society Spring Meeting in 2004

Bavarian Inn
Frankenmuth, MI
April 16, 2004

Revised Abstract Deadline: March 26, 2004

The Spring Meeting of the Michigan Microscopy and Microanalysis Society will
be held on Friday April 16, 2004 at Bavarian Inn in Frankenmuth, MI. In this
one-day conference, there will be two sessions. One is a platform session.
This session will have approximately 8-10 speakers representing industry,
academia, and research laboratories. The other one is a poster session newly
opened this year. Please encourage your colleagues who prefer to avoid a
platform presentation to submit abstracts for the poster presentations. In
addition to the speakers, vendors will exhibit a wide range of products and
services of interest to the microscopy community. Presentations are being
solicited from researchers in the Physical and Biological Sciences,
including one vendor presentation and two invited speakers. Student
participation is particularly encouraged. Also, vendors are encouraged to
contact the below address to reserve space for product display.

Abstract Submission
Please submit a 300 to 350 word abstract by March 26th indicating which
session you prefer to:

Ginam Kim (Ph.D) or email to
g.kim-at-dowcorning.com
Dow Corning Corp.
P.O. Box 994, C041D1
Midland, MI 48686
Tel) (989)-496-5077
Fax) (989)-496-5121

The poster format information will be provided to participants at a later
date.

Kevin Battjes
Impact Analytical Voice 989-832-5555, ext 556
Michigan Molecular Institute Fax 989-832-5560
1910 W. St Andrews Road e-mail: battjes-at-mmi.org
Midland MI 48640 battjes-at-impactanalytical.com

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 17 12:31:19 2004

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Greetings,
In connection to the thread, at one time in the past
different immersion oils from the different 'scope makers had
diferent refractive indices. Therefore, if they got mixed, the
results were really bad, and presumably the lens would have been
designed around a given index. I *think* that the oils from Zeiss,
Nikon, Olympus, Leica now have the same refractive index, but I am
not sure, and I would be interested to hear if anyone knows.

Tobias Baskin
}
}
} The last part of the letter listed below indicates damage to Nikon
} lenses by the use of Zeiss immersion oil. Do you, Ralph, or anyone
} else have instances where this has occurred? (I would suspect that
} this would occur on inverted scopes most often and would be the
} result of dissolving the seal between the lens and the outer case.)
} If so was this the old Zeiss or the new Zeiss oil immersion medium?
} I've got Nikon scopes and would like to post messages in the
} appropriate rooms if this has proven to be a problem. I also have
} Zeiss oil over 15 years old with no solidification problems that
} I've kept hidden.
}
} Also, does anyone know where to find small plastic 5-10 ml bottles
} that would be suitable for dispensing oil immersion medium?
}
} .. Jerry Calvin
}
} listed 3-3-04
} .. Also be aware that different types of immersion oil should never
} be allowed to mix, and that some types of oil can damage the
} mounting cement of some brands of lenses. Using Zeiss immersion oil
} with some Nikon lenses, for example, can be disastrous.

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 17 14:33:30 2004

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There is yet another issue: miscibility.

Some "oils" are not oils at all, at least not in the sense that they are derived from petroleum, or contain fully saturated long-carbon chain (aliphatics/alkanes, etc) compounds. Virtually any substance that has the correct RI, with useable physical properties will be suitable as an immersion "oil". Unfortunately, this leaves the door wide open for manufacturers to use anything from a "real" oil, to compounds like benzyl benzoate, or mixtures of a liquid with a dissolved solid component. The latter case is probably what has caused the infamous Zeiss crystallizing-oil problem. The Zeiss oil is probably saturated when it comes from the factory. When it experiences a drop in temperature, or a bit of evaporation, the solution becomes supersaturated and the crystals drop out. As has been mentioned, warming the mix redissolves the crystals. At that point, I would imagine the RI of the oil would be too high, and would create spherical aberration.

In any case, if you mix oils on the same microscope slide or objective lens without thorough cleaning, chances are you'll create a blurry liquid-liquid interface, and there goes the resolution! Since all the microscope manufacturers know that their oil might not be miscible with any other manufacturers oil, they always recommend that you pick one oil and use it exclusively.

Jim

-----Original Message-----
} From: Tobias Baskin [mailto:baskin-at-bio.umass.edu]
Sent: Wednesday, March 17, 2004 1:50 PM
To: microscopy-at-MSA.microscopy.com

Greetings,
In connection to the thread, at one time in the past
different immersion oils from the different 'scope makers had
diferent refractive indices. Therefore, if they got mixed, the
results were really bad, and presumably the lens would have been
designed around a given index. I *think* that the oils from Zeiss,
Nikon, Olympus, Leica now have the same refractive index, but I am
not sure, and I would be interested to hear if anyone knows.

Tobias Baskin
}
}
} The last part of the letter listed below indicates damage to Nikon
} lenses by the use of Zeiss immersion oil. Do you, Ralph, or anyone
} else have instances where this has occurred? (I would suspect that
} this would occur on inverted scopes most often and would be the
} result of dissolving the seal between the lens and the outer case.)
} If so was this the old Zeiss or the new Zeiss oil immersion medium?
} I've got Nikon scopes and would like to post messages in the
} appropriate rooms if this has proven to be a problem. I also have
} Zeiss oil over 15 years old with no solidification problems that
} I've kept hidden.
}
} Also, does anyone know where to find small plastic 5-10 ml bottles
} that would be suitable for dispensing oil immersion medium?
}
} .. Jerry Calvin
}
} listed 3-3-04
} .. Also be aware that different types of immersion oil should never
} be allowed to mix, and that some types of oil can damage the
} mounting cement of some brands of lenses. Using Zeiss immersion oil
} with some Nikon lenses, for example, can be disastrous.

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 17 15:44:11 2004

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First of all, I'd like to thank all of those helpful people who commented on
the histo-diamond knives by Diatome. I am very impressed with what I heard
and I will purchase one as soon as possible.

Still, I am wondering though how most people who use this knife for
semi-thin (0.5 microns)sectioning rough in their specimens. Do you people
still use glass knives, or do you just go very slowly with the histoknife.
I thought that it might be prudent to still use glass knives for this
purpose, if only to spare the histo diamond knife from rough treatment.

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 17 16:00:32 2004

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I trim with a blade and then rough the block face directly with the histo knife.
Works great.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Garry Burgess [mailto:GBurgess-at-exchange.hsc.mb.ca]
Sent: Wednesday, March 17, 2004 5:03 PM
To: Microscopy-at-sparc5.microscopy.com

First of all, I'd like to thank all of those helpful people who commented on
the histo-diamond knives by Diatome. I am very impressed with what I heard
and I will purchase one as soon as possible.

Still, I am wondering though how most people who use this knife for
semi-thin (0.5 microns)sectioning rough in their specimens. Do you people
still use glass knives, or do you just go very slowly with the histoknife.
I thought that it might be prudent to still use glass knives for this
purpose, if only to spare the histo diamond knife from rough treatment.

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 17 17:52:22 2004

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1. What is the most efficient material for electron diffraction? (I want
high flux in one diffraction order).

2. Has anybody seen electron diffraction from fabricated gratings?

3. How about evidence that diffracted electron-waves are phase coherent
with the incident beam?

4. I seek references for building a three-grating (Mach-Zhender style)
electron interferometer to study the Aharonov-Bohm effect.

- Alex Cronin

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 17 19:44:00 2004

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On Mar 17, 2004, at 4:11 PM, Alexander Cronin wrote:

Dear Alex,

} 1. What is the most efficient material for electron diffraction? (I
} want
} high flux in one diffraction order).

Since the scattering cross section increases with increasing Z, I'd
guess that the most efficient material reasonably available would be
uranium metal; however, the most practical efficient material is likely
to be gold (or maybe bismuth). In addition to the scattering cross
section, the crystal form would be important to give high intensity in
a single diffracted spot, so someone who knows more about
crystallography than I do can correct me if I'm off base.
}
} 2. Has anybody seen electron diffraction from fabricated gratings?

The wavelength of an electron typically used in TEM is very short, so
diffraction from a grating produced by making grooves on a substrate is
not likely to work, since the variations in groove spacings will be
larger than the wavelength; however, materials grown epitaxially, if
you consider them to be gratings, do show ED, and maybe low-angle
reflection ED has been seen from more conventional gratings--once
again, someone more expert than I should comment.
}
}
} 3. How about evidence that diffracted electron-waves are phase
} coherent
} with the incident beam?

I think that can be determined from holography; I'll let the experts
comment. The incident beam itself varies in coherence depending on the
source; a W filament is the least coherent of the usual sources, a LaB6
filament is more coherent and a field emission gun is the most
coherent. (There may be even more coherent non-conventional sources.)
}
} 4. I seek references for building a three-grating (Mach-Zhender style)
} electron interferometer to study the Aharonov-Bohm effect.

Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 08:12:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (verlaj-at-medicine.ufl.edu) from on Wednesday, March 17, 2004 at 12:38:29
---------------------------------------------------------------------------

Email: verlaj-at-medicine.ufl.edu
Name: Jill Verlander Reed

Organization: University of Florida College of Medicine

Title-Subject: [Microscopy] [Filtered] MListserver: seeking recommendations for a new carbon coater

Question: Dear Microscopy Listservers,
We are strongly considering replacing our old Denton evaporator with a new unit to carbon coat grids.
I would be grateful for the opinions of anyone who has purchased a new unit in the recent past.
I am particularly interested in the reliability of the unit and the quality of the coating. We are using the Denton almost exclusively to coat Formvar-coated grids for supporting and stabilizing Lowicryl thin sections. Ease of use and cost are other factors we will consider.
Vendors are more than welcome to contact me directly.

Thanks in advance for your time and the benefits of your experience.

Jill

Jill Verlander Reed, DVM
Director, College of Medicine Electron Microscopy Core Facility
University of Florida
P.O. Box 100215 Health Science Center
1600 SW Archer Road Room RB-167
Gainesville, FL 32610-0215
telephone (352) 846-0820
facsimile (352) 392-8996

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 08:12:00 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ptibbits-at-emerson-ept.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, March 17, 2004 at 12:19:44
---------------------------------------------------------------------------

Email: ptibbits-at-emerson-ept.com
Name: Patrick Tibbits

Organization: Emerson Power Transmission

Title-Subject: [Microscopy] [Filtered] MListserver: SEM Maintenance

Question: I would like to get suggestions for companies which carry maintenance contracts.

Also, I would like to learn of any third-party (not OEM) maintenance providers.

I have a Hitachi 2460N SEM and Oxford 300 ISIS EDS.

Patrick

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 08:13:06 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (hadden-at-wingate.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, March 17, 2004 at 13:50:41
---------------------------------------------------------------------------

Email: hadden-at-wingate.edu
Name: Lee Hadden

Organization: Wingate University

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: One of my SEM students is working with teeth. Can anyone recommend the best way to view the teeth in the SEM, i.e. hi vac SEI or low vac BEI [or any other suggestions for most effective imaging of enamel structure]? We are using a JEOL LV5600 SEM.

Thanks in advance.

Lee Hadden
Department of Biology
Wingate University
Wingate, NC 28174

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 08:46:26 2004

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Hi,

I have a question about lightsources in microscopy. For fluorescence
microscopy you can use Mercury or Xenon arcs and I am curious about the
level of even illumination you can achieve with this kind of
lightsources. If they would be pointsources the "radial" intensity would
diminish with 1/radius^3, but this doesn't seem to be the case ?

What is the residual uneven illumination below which it is not possible
to get with a traditional Xenon or Mercury Arc style illumination ?

Long ago I once read that there are fluorescent samples which you coud
use to make a background profiles for fluorescetce microscopy ? are
these pieces of plastic in which a fluorochorem is embedded ?

Has anyone ever measured the contribution of multiwell plate bottoms to
the illumination profile, due to the non-flat bottoms acting as a lens ?

Regards,

Peter Van Osta

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 12:37:09 2004

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On Mar 18, 2004, at 6:32 AM, Jill Verlander Reed wrote:

} We are strongly considering replacing our old Denton evaporator
} with a new unit to carbon coat grids.
} I would be grateful for the opinions of anyone who has purchased
} a new unit in the recent past.
} I am particularly interested in the reliability of the unit and
} the quality of the coating. We are using the Denton almost
} exclusively to coat Formvar-coated grids for supporting and
} stabilizing Lowicryl thin sections. Ease of use and cost are other
} factors we will consider.
} Vendors are more than welcome to contact me directly.
}
} Thanks in advance for your time and the benefits of your experience.
}
Dear Jill,
About a year ago we purchased a Cressington 208 evaporator, which has
a turbopump, to do both carbon and metal evaporation. The unit has
been completely reliable, and the coatings have been good. The best
coatings are obtained when the vacuum is around 10^-5, which takes a
fairly long time to achieve (depending on how much filter paper, etc.,
in put into the chamber). The instrument is very easy to use for
carbon evaporation, and slightly less so for metal evaporation when the
metal piece has to be loaded in a wire basket, and the cost was very
reasonable for a turbopump desktop system--~$20k if you only want the
carbon power supply, ~$25k with both carbon and metal power supplies.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 12:52:22 2004

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We have projects doing teeth and bone here. Since they are not
generally interested in soft tissues or cells, we just air dry the
teeth/bone, sputter coat and go look. Works well. This is in a
Hitachi S-570 with LaB6, or our S-900 FESEM, but I've also done this
in conventional tungsten-filament SEMs. High vacuum, SEI and BSE,
whole teeth or broken.
I've got a dinosaur tooth project that should be coming in, and he's
likely to do some acid-etching of the teeth to bring out the enamel,
but that's the only preparation step.
There's also this site from the American Museum of Natural History:
http://research.amnh.org/vertpaleo/enamel/index.html
It's on preparing tooth enamel for SEM.

Phil

} Email: hadden-at-wingate.edu
} Name: Lee Hadden
}
} Organization: Wingate University
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: One of my SEM students is working with teeth. Can anyone
} recommend the best way to view the teeth in the SEM, i.e. hi vac SEI
} or low vac BEI [or any other suggestions for most effective imaging
} of enamel structure]? We are using a JEOL LV5600 SEM.
}
} Thanks in advance.
}
} Lee Hadden
} Department of Biology
} Wingate University
} Wingate, NC 28174
}
} ---------------------------------------------------------------------------

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 13:42:02 2004

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I'm looking for a recipe or protocol for Fekete's Fixative.

please help!

Thanks

*********************************************************************
This message and any attachments are solely for the intended recipient. If you are not the intended recipient, disclosure, copying, use or distribution of the information included in this message is prohibited -- Please immediately and permanently delete.

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 14:01:44 2004

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} Larry;
}
} Just curious but doesn't Debeers laser mark their gems? I saw a
} program on TV about synthetic diamonds, gem quality, and they stated
} the difficulty in identification for fraud and authenticity, e.g.
} real or man-made.
}
} Is this a fact? I would imagine the laser marking could be polished off?
}
} Peter Tomic
}
I also seem to recall something on laser marking. As with FIB
marking, I guess is could be easily polished off. Although, if you
have a valuable gem-quality diamond with lots of facets, that may be
a much bigger job than most people would want to undertake,
especially as you would not want to devalue the stone.

I also seem to remember reading somewhere about a method for using
two laser beams - each on its own had no effect but where they
crossed, there was sufficient energy to damage the diamond. This then
makes it possible to put the serial number inside the diamond, so it
can't be polished out without seriously reducing the value.
--
Larry Stoter
NOTE - any message other than plain text will be automatically deleted :-)

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 14:36:15 2004

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Greetings,
I'm trying to find a good cocktail for non-specific digestion of tissue
from bone samples--only the mineralized bone needs to be left
unscathed. I'm looking for a relatively cheap solution that will yield
nice clean bones. I'm aware of a product from Fisher, but it costs
about $70/100ml. It seems to me that there must be a simple solution
that I'm just not aware of (aside from culturing maggots). Thanks in
advance for any suggestions.
Regards,
Karl G.

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 14:51:54 2004

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Household bleach, 1 part bleach to 4 parts water.
or
Adolph's meat tenderizer is papain, don't know the concentration needed.
You can get papain form Sigma, works well at 37C. I don't know any other
details.

Karl Garsha wrote:

} Greetings,
} I'm trying to find a good cocktail for non-specific digestion of
} tissue from bone samples--only the mineralized bone needs to be left
} unscathed. I'm looking for a relatively cheap solution that will
} yield nice clean bones. I'm aware of a product from Fisher, but it
} costs about $70/100ml. It seems to me that there must be a simple
} solution that I'm just not aware of (aside from culturing maggots).
} Thanks in advance for any suggestions.
} Regards,
} Karl G.
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 15:23:20 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (heather.eberhardt-at-frx.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, March 18, 2004 at 08:34:33
---------------------------------------------------------------------------

Email: heather.eberhardt-at-frx.com
Name: Heather Eberhardt

Organization: Forest Research Institute

Title-Subject: [Microscopy] [Filtered] Thin sectioning of tablets

Question: Hello everyone, Iím new here but learning a lot. I need to take thin sections of pharmaceutical tablets, and need several sections from a single tablet (Ideally 10+). They are for use with optical microscopy, ideally PLM. I am trying to figure out which type of epoxy compound I should be using since there are so many out there. Any help or suggestions from someone who has experience in this would be appreciated.

Thanks,

Heather Eberhardt

Heather Eberhardt
Materials Characterization Group
Forest Research Institute
Hauppauge, NY
631-436-2619

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From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 15:43:01 2004

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} I'm looking for a recipe or protocol for Fekete's Fixative.
}
} please help!
}
} Thanks

**********
Twice in one week? Wow. Here are some ref's:
Amer. Coll. of Vet Path. 2003 meeting abstract Poster T-6, Abst. 132
Toxocol. Path). Its an acid alcohol-formalin fix.
See also:
Am J Physiol Gastrointest Liver Physiol 274: G544-G551, 1998;
0193-1857/98 $5.00
Vol. 274, Issue 3, G544-G551, March 1998

Differential susceptibility of inbred mouse strains to dextran sulfate
sodium-induced colitis

Michael Mähler1, Ian J. Bristol1, Edward H. Leiter1, Aletha E.
Workman1, Edward H. Birkenmeier,1, Charles O.
Elson2, and John P. Sundberg1

--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 18 16:17:14 2004

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MR. TIBBITS,

WE DO IT ALL , WE ARE REASONABLE AND
WE ARE COMPETENT. PLEASE CALL IF
INTERESTED. WE ARE NOT TELEMARKETER
TYPES, SO WE DO NOT INUNDATE YOU WITH
ACCOLADES OF OUR SELVES.

IMAQUE IMAGING
BEN GHAFFARI
703-379-0027
571-437-6593
703-257-6321 FAX
----- Original Message -----
} From: "by way of MicroscopyListserver" {ptibbits-at-emerson-ept.com}
To: {microscopy-at-ns.microscopy.com}
Sent: Thursday, March 18, 2004 9:31 AM

Dear Larry,
I believe the diamonds mined in Canada are all marked with a laser-etched
symbol, some with a polar bear and some with a stylized maple leaf, to identify
them as non-conflict diamonds. They are advertised as such.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Larry Stoter" {larry-at-cymru.freewire.co.uk}
To: "Tomic, Peter (Peter)" {ptomic-at-agere.com} ; {Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, March 18, 2004 9:56 AM

Quick internet search found the following which appears to be good for
eyes.

Fekete's acid-alcohol-formalin fixative (3.2% formaldehyde, 0.7 M acetic
acid, 61% ethanol). After 24 h, the fixative was replaced with 70%
ethanol. Eyes were embedded in paraffin, sectioned (5 micron) and stained
with haematoxylin and eosin (H&E) using standard procedures.

Gill Brown

Histopathology Group
Asthma and Allergy Disease Biology
ri- CEDD.
GlaxoSmithKline Medicines Research Centre,

----- Forwarded by Gillian 2 Brown/PharmRD/GSK on 19-Mar-2004 08:39 -----

"Louro, Pedro" {pedro.louro-at-spcorp.com}

18-Mar-2004 20:00

To: Microscopy

cc:
Subject: [Microscopy] Fekete's Fixative

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I'm looking for a recipe or protocol for Fekete's Fixative.

please help!

Thanks

*********************************************************************
This message and any attachments are solely for the intended recipient. If
you are not the intended recipient, disclosure, copying, use or
distribution of the information included in this message is prohibited --
Please immediately and permanently delete.

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 08:53:24 2004

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Hello Peter,
Getting truly even illumination out of a conventional fluorescence arc
lamp isn't a trivial task. The illumination source doesn't really
approximate a point source very well--in a conventional lamp housing one
can adjust the position of the light bulb and mirror so there is an
image of the arc and a reflected image of the arc coming from behind,
this is defocused to provide quasi even illumination with the intensity
highest in the center of the field of view. Depending on the centration
of the objective and filters, the peak intensity can wander.
The most even illumination I've seen from an arc lamp is achieved by
fiber-coupling the lamp output to a fiber optic bent around a large
radius to homogenize the light-the fiber output provides a better
approximation of a point source and the output at the end of the fiber
is even. The Applied Precision Delta Vision takes this approach. It
isn't an easy task to couple an arc lamp to a fiber optic, though.
There are fluorescent plastic slides --I believe they can be
obtained from Chroma. On an inverted microscope, one can use dilution
series of fluorochromes to test things; I prefer this approach (I use
chambered coverslips from LabTek to hold the fresh solutions of
fluorochrome).
I haven't heard of anyone measuring the optical abberations
caused by multiwell plates, but it would seem that image arithmetic
could be used to quantify the difference in fluorescence intensity
across the field of view using such plates as opposed to using chambered
coverslips with a flat .17mm borosilicate glass bottom. The fluorescent
dilutions would be helpful in this context.
Regards,
Karl

Peter Van Osta wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hi,
}
} I have a question about lightsources in microscopy. For fluorescence
} microscopy you can use Mercury or Xenon arcs and I am curious about
} the level of even illumination you can achieve with this kind of
} lightsources. If they would be pointsources the "radial" intensity
} would diminish with 1/radius^3, but this doesn't seem to be the case ?
}
} What is the residual uneven illumination below which it is not
} possible to get with a traditional Xenon or Mercury Arc style
} illumination ?
}
} Long ago I once read that there are fluorescent samples which you coud
} use to make a background profiles for fluorescetce microscopy ? are
} these pieces of plastic in which a fluorochorem is embedded ?
}
} Has anyone ever measured the contribution of multiwell plate bottoms
} to the illumination profile, due to the non-flat bottoms acting as a
} lens ?
}
} Regards,
}
} Peter Van Osta
}
}

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 09:28:31 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I'm evaluating backscatter detectors, and am in need of this familiar test
material ... i.e., a difference in Z of 0.1 at Z=30. I see references to
this standard in the supplies catalogs, but it is not immediately available,
and the picture of it implies that it's not even polished ... which would
contribute a lot to broadening the image's histogram peaks. It would help a
lot if I could find a another source, and polish a sample of it next week.
Is anyone aware of a poor mans' source of inclusion-free alpha-beta (or
duplex) brass?

I don't even suppose it needs to be specifically AB brass, because all I
need do is polish it extremely well, that it have neighboring phases to
contrast, and have an average Z } 22 ... and make comparisons with the same
material. For example, I have "pure" FeS exsolved in pyrrhotite, but the
scale doesn't really allow me to select a relatively large area of each for
determining the noise.

Suggestions most welcome ..

tia & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 09:41:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Quoting "Louro, Pedro" {pedro.louro-at-spcorp.com} :
---------------------------------------------------------------
} I'm looking for a recipe or protocol for Fekete's Fixative

Pedro,

I believe that the original regerence is in AM. J. Path. 14:557, 1938.

This reference I found in Histopathologic Technic and Practical Histochemistry
by R.D. Lillie, 1954 in which the formula is stated as
10 cc. 37-40% formaldehyde
5 cc. Glacial acetic acid
100 cc. 70% alcohol

It states that it is a good glycogen preservative and suggests leaving the
tissue in 70% alcohol rather than in the fixative if it is necessary to store
the tissue for any length of time after fixation.

I love reading old histology books!
Pat Connelly psconnel-at-sas.upenn.edu
Research Specialist
Dept. of Biology
Univ. of Pennsylvania
Philadelphia, PA 19104

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 10:13:19 2004

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Hi Peter,
i totally agree with Karl....
the fibercoupling is a way, for certain (blue) wavelengths you want to use liquid
wave guides - but you will get a new problem once you bring your fibers/LWG`s in a
different position. so you have definitively to fixate them somewhere on your scope!
maybe you could make a "flatness" around 10%! if that`s not enough, you will have to
correct the images anyways. just in case:
correctedimage=(rawimage-rawdark)/(flatimage-flatdark) ["dark" are the darkcounts
with ccd... the "dark" image you get with light turned off]
propably you want to make a new flatfield image from time to time, since the lamp
changes the properties in terms of resulting flatness incredibly over the time! we
did at least once a week with our (Zeiss) HBO100.
i wouldn`t suggest using bulk plastic slides, since these will homogenize your
illumination quite a bit. you will see that clearly if you try to stitch the
resulting images together to create a bigger image. The way Karl is describing seems
much better, especially because you would be able to control the resulting intensity
by concentration.
we had the best results with a thin (1..3µm) fluorescent layer e.g. fluorophore-doped

polyimide on borosilicate-glass for flatfielding. its the same idea, just in a so.lid

phase. these are just easier to handle, store and use as dilutions... especially if
you want to use the same thing different times.

cheers
thomas

Karl Garsha schrieb:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hello Peter,
} Getting truly even illumination out of a conventional fluorescence arc
} lamp isn't a trivial task. The illumination source doesn't really
} approximate a point source very well--in a conventional lamp housing one
} can adjust the position of the light bulb and mirror so there is an
} image of the arc and a reflected image of the arc coming from behind,
} this is defocused to provide quasi even illumination with the intensity
} highest in the center of the field of view. Depending on the centration
} of the objective and filters, the peak intensity can wander.
} The most even illumination I've seen from an arc lamp is achieved by
} fiber-coupling the lamp output to a fiber optic bent around a large
} radius to homogenize the light-the fiber output provides a better
} approximation of a point source and the output at the end of the fiber
} is even. The Applied Precision Delta Vision takes this approach. It
} isn't an easy task to couple an arc lamp to a fiber optic, though.
} There are fluorescent plastic slides --I believe they can be
} obtained from Chroma. On an inverted microscope, one can use dilution
} series of fluorochromes to test things; I prefer this approach (I use
} chambered coverslips from LabTek to hold the fresh solutions of
} fluorochrome).
} I haven't heard of anyone measuring the optical abberations
} caused by multiwell plates, but it would seem that image arithmetic
} could be used to quantify the difference in fluorescence intensity
} across the field of view using such plates as opposed to using chambered
} coverslips with a flat .17mm borosilicate glass bottom. The fluorescent
} dilutions would be helpful in this context.
} Regards,
} Karl
}
} Peter Van Osta wrote:
}
} }
} }
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } Hi,
} }
} } I have a question about lightsources in microscopy. For fluorescence
} } microscopy you can use Mercury or Xenon arcs and I am curious about
} } the level of even illumination you can achieve with this kind of
} } lightsources. If they would be pointsources the "radial" intensity
} } would diminish with 1/radius^3, but this doesn't seem to be the case ?
} }
} } What is the residual uneven illumination below which it is not
} } possible to get with a traditional Xenon or Mercury Arc style
} } illumination ?
} }
} } Long ago I once read that there are fluorescent samples which you coud
} } use to make a background profiles for fluorescetce microscopy ? are
} } these pieces of plastic in which a fluorochorem is embedded ?
} }
} } Has anyone ever measured the contribution of multiwell plate bottoms
} } to the illumination profile, due to the non-flat bottoms acting as a
} } lens ?
} }
} } Regards,
} }
} } Peter Van Osta
} }
} }
}
} --
} Karl Garsha
} Light Microscopy Specialist
} Imaging Technology Group
} Beckman Institute for Advanced Science and Technology
} University of Illinois at Urbana-Champaign
} 405 North Mathews Avenue
} Urbana, IL 61801
} Office: B650J
} Phone: 217.244.6292
} Fax: 217.244.6219
} Mobile: 217.390.1874
} www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 10:33:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all,

We have a new SEM/EDS system at NSAC. This is the
first electron microscope in our College. The
College administration has asked me to develop a
policy for usage, funding, prioritization and data
collection of the SEM/EDS unit. The
administration could not provide a technical
support for the unit.
I will be the major user of the system, I would
assume there will be between 10 and 15 other users
from the College. The system has been purchased
with CFI funding to support research programs.

I would appreciate your comments and suggestions
on how to develop user fees, how much of my time
should be dedicated to the unit as teaching
others, managing the lab, and simple maintenance.
Perhaps I can ask the administration that 30-40%
of my time to be dedicated to the unit..

Kind regards
Valtcho Jeliazkov

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 12:05:16 2004

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Valtcho;

Although I am not in a university environment, I would strongly urge you to develop a thorough training program with specific instructions on how not to break things. Where people get in trouble, in my experience, is in areas like crashing the stage into the EDX nosepiece and lens, as well as putting in samples that are not thoroughly dry, [except for ESEMS], sample exchange and/or inappropriate samples for vacuum environments. The more you have written down in terms of instruction, the less likely it will be that your 30-40% of SEM time will be with wrench in hand. This will also help when you need to exile someone from the lab. since you will have documented procedures to point to. It also impresses upper management. In your case upper faculty and admins.

With regard to EDX, make them calibrate before using. It's a good habit to have.

Hope this is of some value.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Valtcho Jeliazkov (Zheljazkov) Ph.D.
[mailto:vjeliazkov-at-nsac.ns.ca]
Sent: Friday, March 19, 2004 11:52 AM
To: Microscopy-at-MSA.Microscopy.Com

Hi all,

We have a new SEM/EDS system at NSAC. This is the
first electron microscope in our College. The
College administration has asked me to develop a
policy for usage, funding, prioritization and data
collection of the SEM/EDS unit. The
administration could not provide a technical
support for the unit.
I will be the major user of the system, I would
assume there will be between 10 and 15 other users
from the College. The system has been purchased
with CFI funding to support research programs.

I would appreciate your comments and suggestions
on how to develop user fees, how much of my time
should be dedicated to the unit as teaching
others, managing the lab, and simple maintenance.
Perhaps I can ask the administration that 30-40%
of my time to be dedicated to the unit..

Kind regards
Valtcho Jeliazkov

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 12:27:31 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Do you have a maintenance contract ? The policy specifics and your time
allotment may hinge on this factor.

Regards,
Ed

----- Original Message -----
} From: "Valtcho Jeliazkov (Zheljazkov) Ph.D." {vjeliazkov-at-nsac.ns.ca}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Friday, March 19, 2004 8:52 AM

PS to Peters comments -

Very Important also..keep an ongoing log near the system to record all
maintenance and 'problems'...this is invaluable for troubleshooting
thoughout the life of the system.

Also, in the training process, cover the 'artifact' issues (SEM as well as
EDS). Never rely on the automation!

} From: "Tomic, Peter (Peter)" {ptomic-at-agere.com}
} Date: Fri, 19 Mar 2004 13:23:39 -0500
} To: "Valtcho Jeliazkov (Zheljazkov) Ph.D." {vjeliazkov-at-nsac.ns.ca} ,
} {Microscopy-at-MSA.Microscopy.Com}
} Subject: [Microscopy] RE: SEM/EDS system policy for usage
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Valtcho;
}
} Although I am not in a university environment, I would strongly urge you to
} develop a thorough training program with specific instructions on how not to
} break things. Where people get in trouble, in my experience, is in areas like
} crashing the stage into the EDX nosepiece and lens, as well as putting in
} samples that are not thoroughly dry, [except for ESEMS], sample exchange
} and/or inappropriate samples for vacuum environments. The more you have
} written down in terms of instruction, the less likely it will be that your
} 30-40% of SEM time will be with wrench in hand. This will also help when you
} need to exile someone from the lab. since you will have documented procedures
} to point to. It also impresses upper management. In your case upper faculty
} and admins.
}
} With regard to EDX, make them calibrate before using. It's a good habit to
} have.
}
} Hope this is of some value.
}
} Peter Tomic
} Agere Systems
}
} -----Original Message-----
} } From: Valtcho Jeliazkov (Zheljazkov) Ph.D.
} [mailto:vjeliazkov-at-nsac.ns.ca]
} Sent: Friday, March 19, 2004 11:52 AM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] SEM/EDS system policy for usage
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Hi all,
}
} We have a new SEM/EDS system at NSAC. This is the
} first electron microscope in our College. The
} College administration has asked me to develop a
} policy for usage, funding, prioritization and data
} collection of the SEM/EDS unit. The
} administration could not provide a technical
} support for the unit.
} I will be the major user of the system, I would
} assume there will be between 10 and 15 other users
} from the College. The system has been purchased
} with CFI funding to support research programs.
}
} I would appreciate your comments and suggestions
} on how to develop user fees, how much of my time
} should be dedicated to the unit as teaching
} others, managing the lab, and simple maintenance.
} Perhaps I can ask the administration that 30-40%
} of my time to be dedicated to the unit..
}
} Kind regards
} Valtcho Jeliazkov
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 13:37:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Valtcho,
I inherited the system in our University to manage the SEMs and TEM in our lab,
but it has worked out well for me.
1. Because my department pays my expenses, users from my department do not pay
for use. I have money available from a Shared Services account that all
researchers in our department contribute to, to buy consumables like apertures
and filaments. These users must still sign up on the calendar to reserve the
instrument for themselves.
2. Other users from our university and other universities are charged a low
hourly fee for use of all the instruments. I charge them $25 per hour for SEM
and an additional $10 per hour if they use EDX. I also charge for gold coatings,
film or other things that cost me money.
3. Commercial companies that want to use the instruments are charged commercial
rates ( I charge $200 per hour). You need to find a commercial test firm that
does SEM/EDX and see what their hourly charge is. Do not undercut them with a
CFI grant-supplied instrument.
I also set a priority system that spells out who has priority on the available
time on the instrument. As an example: you would be first, researchers that
supported your CFI application would be next, other researchers, Graduate
Students, Undergraduate laboratories and projects would be defined. Commercial
use is usually last, only if there is unused time available. All my instruments
have a sign-up calendar so people can reserve them for a specified time. Some of
my instruments are open time, so people can sign up for as much time as they
want, when they want. The most popular (newest) instrument has a strict schedule
where each day has four two-hour time slots and each user can only sign up for
one slot. When they use that slot they can sign up for the next available slot.
This gives everyone a chance.
I hope this example gives you some ideas.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca} -----Original Message-----
} } From: Valtcho Jeliazkov (Zheljazkov) Ph.D.
} [mailto:vjeliazkov-at-nsac.ns.ca]
} Sent: Friday, March 19, 2004 11:52 AM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] SEM/EDS system policy for usage
}
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ------------------------------------------------------------------------------
-
}
} Hi all,
}
} We have a new SEM/EDS system at NSAC. This is the
} first electron microscope in our College. The
} College administration has asked me to develop a
} policy for usage, funding, prioritization and data
} collection of the SEM/EDS unit. The
} administration could not provide a technical
} support for the unit.
} I will be the major user of the system, I would
} assume there will be between 10 and 15 other users
} from the College. The system has been purchased
} with CFI funding to support research programs.
}
} I would appreciate your comments and suggestions
} on how to develop user fees, how much of my time
} should be dedicated to the unit as teaching
} others, managing the lab, and simple maintenance.
} Perhaps I can ask the administration that 30-40%
} of my time to be dedicated to the unit..
}
} Kind regards
} Valtcho Jeliazkov
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 14:56:42 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Shaf,

I have some. I got it from out machine shop - when we had one. It is a
(for SEM) large chunk and I can cut you a piece from it if nothing else
easier turns up.

IMHO, The surface *must* be polished or the topo-contrast will swamp the
Z-contrast. My GW Electronics, Type 47 system, "sees" the phases fine (No
affiliation).

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: michael shaffer [mailto:michael-at-shaffer.net]
Sent: Friday, March 19, 2004 10:47 AM
To: Microscopy list; Sx50-Users

I'm evaluating backscatter detectors, and am in need of this familiar test
material ... i.e., a difference in Z of 0.1 at Z=30. I see references to
this standard in the supplies catalogs, but it is not immediately available,
and the picture of it implies that it's not even polished ... which would
contribute a lot to broadening the image's histogram peaks. It would help a
lot if I could find a another source, and polish a sample of it next week.
Is anyone aware of a poor mans' source of inclusion-free alpha-beta (or
duplex) brass?

I don't even suppose it needs to be specifically AB brass, because all I
need do is polish it extremely well, that it have neighboring phases to
contrast, and have an average Z } 22 ... and make comparisons with the same
material. For example, I have "pure" FeS exsolved in pyrrhotite, but the
scale doesn't really allow me to select a relatively large area of each for
determining the noise.

Suggestions most welcome ..

tia & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 19 16:26:53 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Colleagues,

This is a second announcement for the workshop entitled
“Multidimensional data presentation techniques” which will take place on
April 4 from 12:30 to 4:30 just before the opening of the “Focus on
Microscopy 2004” Conference in Philadelphia. Please hurry with your
registration! There are only a few spots left.

For more information about the workshop please point you Internet
browsers to:

http://www.cyto.purdue.edu/FOM2004/ - workshop web page
or
http://www.focusonmicroscopy.org/ - FOM2004 web page

This workshop will include an interactive tutorial on the use of a
variety of techniques for multidimensional microscopy data presentation.
Many advanced visualization packages for microscopists are commercially
available. Similarly, plenty of applications for video processing and
presentations can be found on the market. However, transforming complex
data sets into the actual presentation for use in lectures or in web
sites is not as easy as it seems. There are a variety of
tricks-of-the-trade, useful suggestions, and some very nice inexpensive
or free software obtainable. We would like to share our experiences and
tell you about them!

You will learn how to present static 2D images as well as 3D datasets in
the most efficient way. We will show you how to produce short animations
using data from confocal/MP systems in highly compressed MPEG4-based
formats. You will receive a handout and CD-ROM containing key materials
presented in the workshop as well as a significant number of really
valuable free utility software packages.

We will demonstrate:
* How to compress microscopy data. What are the pros and cons of
compression? Does it affect final results? What about lossy and lossless
compression?
* How you should present your 3D data. How to prepare 3D image
reconstruction? How to create anaglyphs? How to protect the data in an
anaglyph when you compress it? How to make a movie anaglyph/animation?
* How to create an animation from a 3D construction.
* How to create movies that are playable in PowerPoint, on web pages,
or with other media.
* How to understand codecs and their associated problems.
* How to edit animations/movies using high-speed command line processing.
* How to you add your name, logo of your institution, or other info
into the movie.
* How to deal with sound overlays.
* How to reproduce a movie-making process. You will learn simple
command line macros that are really fast!

If you are registered for the workshop, please take some time to take
our pre-workshop survey. Your participation will help us greatly with
the workshop preparation. We would like to know about your expectations,
your level of experience in multimedia multidimensional data
presentation techniques, and the issues you consider to be important.
The link to the survey is present on the workshop web page.

Bartek Rajwa (rajwa at flowcyt.cyto.purdue.edu)
Jennie Sturgis (jennie at flowcyt.cyto.purdue.edu)
J. Paul Robinson (jpr at flowcyt.cyto.purdue.edu)

Purdue University Cytometry Laboratories
Hansen Research Building
201 S. University Street
West Lafayette, IN 47907
Telephone: (765) 494-0757
Fax: (765) 494-0517
Web: http://www.cyto.purdue.edu/

----------------------------------------------------------------------
The organizers of the workshop gratefully acknowledge the assistance of
Media Cybernetics Corporation, the producer of Image-Pro Plus - an image
analysis software package for fluorescence imaging, quality assurance,
materials imaging, and various other scientific, medical, and industrial
applications.

From MicroscopyL-request-at-ns.microscopy.com Sat Mar 20 08:48:56 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Elliotluke-at-yahoo.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, March 19, 2004 at 18:04:47
---------------------------------------------------------------------------

Email: Elliotluke-at-yahoo.com
Name: Elliott Morrow

Organization: none

Title-Subject: [Microscopy] [Filtered] Adventures in Amateur Micrography

Question: Dear Forum,
I am a recent college graduate. I have a BS in Biology and
hope to acquire my MS in microbiology in a few years. I enjoy microscopy and can not wait for graduate school to afford me the opportunities to stretch my microscopy muscles.
I am looking to buy a microscope/microscopy setup for home use. I spend hours on the Internet looking at micrographs and associated photos. I would love to start taking my own photos and preparing slides in-house. I know that many seasoned microscopists share my passion for micrography.
If you have any ideas on what sort of setup I should buy or ideas on how to approach amateur micrography on a budget please mail me.
Thank you, Elliott

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Mar 20 08:47:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (cynthia.green-at-njmoldinspection.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, March 20, 2004 at 06:44:14
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Email: cynthia.green-at-njmoldinspection.com
Name: Cindy Green

Education: Graduate College

Location: City, State, Country

Question: I'm trying to locate a objective extender of about 10mm in length for a Wild DIN lens. Do you know of a good microscope parts source?

Thank you,

Cindy Green

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From MicroscopyL-request-at-ns.microscopy.com Sun Mar 21 18:48:59 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (zachary_carr-at-eku.edu) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Sunday, March 21, 2004 at 14:41:54
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Email: zachary_carr-at-eku.edu
Name: Zachary Carr

Organization: Eastern Kentucky University

Education: Undergraduate College

Location: Richmond, Ky, USA

Question: On a comparison microscope, how does the optical bridge split the image by means of mirrors?

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From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 01:33:27 2004

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Hi,

Does anyone know how to accomplish a batch export of images from Autobeam in
ISIS? I have 3000 odd images that need to be exported for processing on
software that was written inhouse. Currently I have to open each image
individually in Autobeam and then type/copy in a filename to export as tif.

Any help would be GREATLY appreciated.

Regards
George

George Theodossiou
Physicist / Electron Microscopist

AMCOR Research and Technology
Ph: +61 3 9490 6135
Fax: +61 3 9499 4295
Mobile: 0409 568 840
email: George.Theodossiou-at-amcor.com.au

************************************************************************
CAUTION - This message may contain privileged and confidential
information intended only for the use of the addressee named above.
If you are not the intended recipient of this message you are hereby
notified that any use, dissemination, distribution or reproduction of
this message is prohibited. If you have received this message in error
please notify AMCOR immediately.
Any views expressed in this message are those of the individual sender
and may not necessarily reflect the views of AMCOR.
************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 07:27:05 2004

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hello all, looking for dee bergers email address. let
me know.
thanks
john hoffpauir

__________________________________
Do you Yahoo!?
Yahoo! Finance Tax Center - File online. File on time.
http://taxes.yahoo.com/filing.html

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 08:58:11 2004

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As with any material there are several ways of specimen
preparation for observation of tooth structure.
Specimens could be fractured or polished, they could be
etched with acids. For observation of an enamel hi vac
mode is usually better.

It is difficult to advise you without knowing the
specifics of the research. You are welcome to contact
me off line for more discussion.

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

} Email: hadden-at-wingate.edu
} Name: Lee Hadden
}
} Organization: Wingate University
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: One of my SEM students is working with teeth. Can
} anyone recommend the best way to view the teeth in the SEM,
} i.e. hi vac SEI or low vac BEI [or any other suggestions for
} most effective imaging of enamel structure]? We are using a
} JEOL LV5600 SEM.
}
} Thanks in advance.
}
} Lee Hadden
} Department of Biology
} Wingate University
} Wingate, NC 28174
}
} --------------------------------------------------------------
} -------------
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 12:03:00 2004

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Zachary,
Here is a very quick explanation of the light path of the comparison microscope.
As light comes up through the objective lens above each of the two stages it enters a set of prisms that erect the image and redirect it toward the center of the bridge. You could think of this set of prisms as a mirror set at 45 degrees to reflect the image at a right angle toward the center of the bridge, the prisms do more, but this will give you an idea of what is happening. At the center of the bridge is another set of prisms that reflect the image up to the eye pieces. You could think of this prism set as two mirrors set back to back at 45 degrees each, with the tops of the mirrors meeting at a very sharp edge, they redirect both fields (one from each objective) 90 degrees upward to the eye pieces. In some scopes this center prism set is on a moveable mount that lets you move this set of prisms into position to allow 50% of the field from each objective, all of one field and none of the second, or any percent of each that makes up 100%, for example 70% of one field and 30% of the other. Here is a very rough diagram of the light path. If you want a better one I think I have a photo of a part of a Leica poster with a diagram of the UFM 4's optical path, I could send it off the list but don't want to clutter the list with attachments. Drop me a note if you need this, I'll see if I can find it or snap another.

|
/------/\------\
| |
_ _

Jim

James L. Roberts
Forensic Scientist / Firearm and Toolmark Examiner
Ventura County Sheriff's Forensic Science Laboratory
800 S. Victoria Ave.
Ventura, CA. 93009

(805) 654-2308
James.Roberts-at-mail.co.ventura.ca.us

} } } {zachary_carr-at-eku.edu} 03/21/04 05:10PM } } }

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (zachary_carr-at-eku.edu) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Sunday, March 21, 2004 at 14:41:54
---------------------------------------------------------------------------

Email: zachary_carr-at-eku.edu
Name: Zachary Carr

Organization: Eastern Kentucky University

Education: Undergraduate College

Location: Richmond, Ky, USA

Question: On a comparison microscope, how does the optical bridge split the image by means of mirrors?

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From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 12:11:47 2004

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M&M 2004 Attendees there will be two additional short courses offered
at M&M2004 this year that were not listed in the call for papers.
Their descriptions are listed below. You can sign up for these courses
at the meeting or online.

Short Course X18

Title: Microspectroscopy - Raman, FT-IR and EDXRF Microscopy

9:00am to 5:00pm

Instructors: Fran Adar, John Reffner, Paul Dinh

Today more and more laboratories are combining microscopy with the
power of spectroscopy to provide a detailed characterization of their
samples.   This short course will show how laboratories are using
Raman, FT-IR and EDXRF Microspectroscopy to their benefit.  These three
techniques provide molecular and/or elemental information with a
spatial resolution at the micron level. They can also be used for
hyperspectral imaging to show how the molecular and elemental
structure changes throughout a sample.  Attendees will leave the course
with a knowledge of the varied uses of the instrumentation and the
applicability of these methods to their particular materials.
Examples from biological, pharmaceutical, polymer, semiconductor and
forensic applications will be used to illustrate the power of these
techniques. The course will offer lectures, hands on instrumentation
and a chance for questions. Participants are welcome to bring samples.

Short Course X19

Title: Application Pathways- Native sample to Immunolabeling via
Tokayasu and High Pressure Freezing

9:00am to 5:00pm

Instructors: Kent McDonald & Jan Slot

High pressure freezing is the way to localize or characterize
organelles, subcellular components and gene products in electron
microscopy. This single-day short course will discuss the process of
sample preparation using cryo techniques.

The course will review methods for cryopreparation of biological
samples. High pressure freezing, why,? the advantages of HPF over
chemical and or microwave fixation. After HPF what techniques or
methods of tissue examination can be used, such as cryo planing,
cryosectioning, freeze substitution, freeze fracture and
immunolabeling. The course will offer lectures, hands on of related
instrumentation and roundtable discussions.

--
John Mansfield PhD MInstP
North Campus Electron Microbeam Analysis Laboratory
417 SRB, University of Michigan
2455 Hayward, Ann Arbor MI 48109-2143 USA
Phone: (734) 936-3352
FAX (734) 763-2282
Cell. Phone: (734) 834-3913
(Leaving a phone message at 936-3352 is preferable to 834-3913)
Email: jfmjfm-at-engin.umich.edu
URL: http://emalwww.engin.umich.edu/people/jfmjfm/jfmjfm.html
Location: Lat. 42° 16' 48" Long. 83° 43' 48"
AIM: thejfmjfm

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 13:32:56 2004

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We (an hourly under my direction) wrote a utility to export batches of ISIS
Autobeam images to TIFF format. We have used it on hundreds of images. I
don't think we are up to the thousands yet. You can download the package
from ftp://www.marl.iastate.edu/Utilities/ISIS-TIFF/. Documentation is
included with the executable files.

I think we had some problems where the last image of the selected set might
not get converted. If so, you may need to convert it after the larger
batch. But I think it has been working okay of late, especially when I
convert the entire job.

As long as you remember you get what you pay for, you may drop me a line if
you have detailed questions about its use.

At 01:44 AM 3/22/2004, George Theodossiou wrote:

} Hi,
}
} Does anyone know how to accomplish a batch export of images from Autobeam in
} ISIS? I have 3000 odd images that need to be exported for processing on
} software that was written inhouse. Currently I have to open each image
} individually in Autobeam and then type/copy in a filename to export as tif.
}
}
} Any help would be GREATLY appreciated.
}
} Regards
} George
}
} George Theodossiou
} Physicist / Electron Microscopist
}
} AMCOR Research and Technology
} Ph: +61 3 9490 6135
} Fax: +61 3 9499 4295
} Mobile: 0409 568 840
} email: George.Theodossiou-at-amcor.com.au

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 16:12:00 2004

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Dear Colleagues

I have used an AGFA Duoscan 1200 for some years for TEM negatives.
Recently it stopped working and it seems that it is easier to buy a new
one than repair the old machine.

Can anyone recomend a suitable (inexpensive) machine?
As far as my experience goes, the low end scanners do not give acceptable
results with dense negatives. The Duoscan was acceptable perhaps due to better
sensitivity. More sensitive scanners may become too expensive for our lab.
So, I'm looking for a suitable compromise: enough sensitivity v. lowest price

Thanks in advance

A.P. Alves de Matos
Biologist
Electron Microscopy Unit
Curry Cabral Hospital, Lisbon

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 22 22:20:46 2004

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Colleagues:

This is the second announcement for the upcoming free, 2-day "miniworkshop"
in Cryoultramicrotomy for Materials Sciences that will be held at West Chester
University of Pennsylvania.

If you have not yet sent your RSVP, please do so to any of the people listed
below. We need an accurate count of attendees for meals and refreshments.

The details are as follows:

Members who have an interest in materials science are cordially invited to a
free two-day "mini-workshop" on cryoultramicrotomy for the materials sciences.
This topic is of special interest for those who work with polymers or other
materials which could benefit from ultrathin sectioning or surface "polishing"
at low temperatures (no embedding required).

This invitation is extended to persons who are located in the greater
Philadelphia/Baltimore/Washington, D.C./New York City area. The workshop will be
hosted by the Center for Advanced Scientific Imaging (CASI) at West Chester
University of Pennsylvania.

**What**:
Mini-Workshop on Cryoultramicrotomy for Materials Science

**When**:
Tuesday, March 30, 2004, 11:00 am through Wednesday, March 31, 2004, 4:00 pm.

Visitors are invited to arrive early on Tuesday, March 30 for tours of the
Center for Advanced Scientific Imaging. The lab will be open at 8:00 am on
Tuesday.

**Where**:
West Chester University of Pennsylvania, Schmucker Science Center South, Room
SSS017. Schmucker Science Center South is located on the corner of South
Church Street and Rosedale Avenue in West Chester, PA. West Chester is located
approximately 30 miles from Philadelphia.

**Format**:
A presentation on cryoultramicrotomy and its applications in the materials
sciences will be given on the first day, as well as demonstrations on the
preparation of cryotools (hair probes, large and small wire loops, etc.) and glass
knife making and evaluation. The care and cleaning of diamond knives will also
be discussed.

The demonstrations will be followed by open lab sessions for the attendees to
prepare their own cryotools and glass knives.

Also on the first day an introduction to the cryoultramicrotome will be
given, and attendees will have an opportunity for hands-on use of the instrument.

The second day will be reserved for attendees to sign up in small groups for
additional time and training on the instrumentation, depending on the
attendees' individual needs.

**Limited Space Available**:
The lectures and demonstrations on the first day are open to everyone, but
space is limited to *10 persons* for the in-depth training and extended use of
the instrumentation on the second day.

**Contacts**:
To RSVP or to reserve a seat for the second day's sessions, please contact
any of the following people:

Dr. Fred Monson, CASI / West Chester University of Pennsylvania,
610.738.0437, {fmonson-at-wcupa.edu}

Ms. Kim Megaw, RMC Products / Boeckeler Instruments, Inc., 520.745.0001,
{kim-at-boeckeler.com}

Dr. Robert Chiovetti, RMC Products / Boeckeler Instruments, Inc.,
520.745.0001, {bob-at-boeckeler.com}

See you soon in West Chester!

Robert (Bob) Chiovetti
RMC Products
Boeckeler Instruments, Inc.
{bob-at-boeckeler.com}
{rchiovetti-at-aol.com}

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 07:08:42 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jrobson-at-rdg.boehringer-ingelheim.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Tuesday, March 23, 2004 at 06:41:11
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Email: jrobson-at-rdg.boehringer-ingelheim.com
Name: John Robson

Organization: Boehringer Ingelheim

Education: Undergraduate College

Location: Danbury, CT

Question: I've been asked to perform several measurements on a polyethylene part. I need to determine the length and diameter (at several points) of a channel that is roughly 0.3mm wide X ~2.0mm long. Years ago we had worked with latex casting materials for this purpose unfortunately shrinkage was a constant issue. I would appreciate any recommendations on alternative casting materials that would allow us to accurately reproduce an impression of the part with minimal shrinkage. Thank You, John.

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From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 07:24:10 2004

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O.k., folks the radiation safety people here are looking at re-classifying
*ALL* the uranyl compounds on campus as lisenced materials (i.e.
radioisotopes) with all the requirments and certifications that go along. As
careful dropwise users of Uranyl acetate I am trying to avoid unneeded
headaches, and trying to get low concentration low quantity Uac to be
considered separately from the high quantity chemistry users. To that end I
am collecting info on how other institutions handle it.

So folks how does your institution classify Uac: Radioisotope or not. And
how is it disposed of?

Especially Ohio folks appreciated! Thank you.

(Note: I have searched the listserv archive 2001-2004 before posting this, and
we've only discussed it a little in early Jan 2004)

==============

Since some folks may ask: How we currently use and handle UA:

The EM Facility does use Uranyl Acetate on a regular basis for
heavy metal "staining" of transmission electron microscope (TEM) samples.
We work with 0.5% & 2.0% aqueous solutions (approximately 80-85% of the
work uses 0.5% UAc), and we use ~ 0.3-0.6g total per year. The EM grade
Uranyl acetate for staining is sold as a "depleated" Uranyl acetate (since
we need the heavey metal and not the radiation), and is difficult to
detect above back ground radiation. We use 10ul drops at a time, these
droplets are collected and stored in lable waste containers, and rinse
water is also collected in the waste containers (Containers only contain
Uac and water). Transfer pipettes are rinsed before disposal. Waste
containers are collected by EHS regularly. We treat the Uac as a serious
heavy metal toxin as we do our other heavy metal stains (Pb, Os, W, Cr,
Ag, etc.).

If the decision is made to consider *ALL* Uranyl compunds licensed
material, the this will have a serious impact on the facility to meet the
licensing requirments, for very little increased safety. One of our
standing polcies at present is *NOT* to allow radioisotopes in the
facility as we are not certified to handling them. We would need radiation
training of all TEM users. We would need locked storage of stocks,
working solutions, and wastes (since locking the facility would not be
practical), then users would be facing moving solutions from the locked
location to the application site, and back again. Whereas at present the
working solution and wasters containers used are not moved they are simply
opened and closed. In this case I think licensing would increase the risk
(due to dropping and spillage) rather than decrease.

I would just ask that the radiation safety committee perhaps consider
subcategories of Uranyl compounds and/or quanities used.

=====================

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 08:03:57 2004

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hi,

Struers from Denmark made a special latex resin for this research !
I used this resin "RepliSet 3 - D Replicas for Non-Destructive Testing"

best regards for all

chris hübner

Foundry Research Institute
Kraków - Poland

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 08:10:00 2004

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I too, had a limited budget and a need for a scanner. A few years
ago, I bought an Epson Expression 1600 Professional scanner with
trans-illumination. I've been pretty happy with it. It comes with
holders for negatives, but for the 3.25 x 4 inch negs I have. I
place my negatives directly on the glass and use the focus setting
for contact and I haven't had problems. (OK everyone, a collective
gasp of horror here...but really, its been OK).
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 08:30:49 2004

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Greetings all,

Does anyone know where I can buy Loctite 460 superglue? How about the
softer black wax (Apeizon brand?).

I've been looking around online and I cannot find either of these sample
prep items. Any help would be great.

Have a good week,

William Stratton

-------------------
William G. Stratton
Research Assistant
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu
http://www.cae.wisc.edu/~stratton/

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 08:31:51 2004

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We bought the Epson Perfection 3200 Photo and it works well. We also have
to put our TEM negs directly on the glass, but we have had no problem with
it.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: AP Alves de Matos [mailto:apamatos-at-oninet.pt]
Sent: Monday, March 22, 2004 5:34 PM
To: Microscopy-at-MSA.Microscopy.Com

Dear Colleagues

I have used an AGFA Duoscan 1200 for some years for TEM negatives.
Recently it stopped working and it seems that it is easier to buy a new
one than repair the old machine.

Can anyone recomend a suitable (inexpensive) machine?
As far as my experience goes, the low end scanners do not give acceptable
results with dense negatives. The Duoscan was acceptable perhaps due to
better
sensitivity. More sensitive scanners may become too expensive for our lab.
So, I'm looking for a suitable compromise: enough sensitivity v. lowest
price

Thanks in advance

A.P. Alves de Matos
Biologist
Electron Microscopy Unit
Curry Cabral Hospital, Lisbon

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 08:52:20 2004

Contents Retrieved from Microscopy Listserver Archives
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We also use the EPSON 3200 Photo, with great results. If better scans (for
enlargements) need to be performed, we use the NIKON SuperCoolScan 8000 ED which
gives 4000 ppi images to work with. The slowness is the reason for only using the
NIKON for specific negatives, BUT as for the resolution, and the contrast depth -
it is unsurpassed.
Stan

"Sherwood, Margaret" wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} We bought the Epson Perfection 3200 Photo and it works well. We also have
} to put our TEM negs directly on the glass, but we have had no problem with
} it.
}
} Peggy Sherwood
} Lab Associate, Photopathology
} Wellman Laboratories of Photomedicine (W224)
} Massachusetts General Hospital
} 55 Fruit Street
} Boston, MA 02114
} 617-724-4839 (voice mail)
} 617-726-6983 (lab)
} 617-726-3192 (fax)
} msherwood-at-partners.org
}
} -----Original Message-----
} } From: AP Alves de Matos [mailto:apamatos-at-oninet.pt]
} Sent: Monday, March 22, 2004 5:34 PM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] TEM Acquiring new scanner for negatives
}
} ----------------------------------------------------------------------------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ----------------------------------------------------------------------------
} ---
}
} Dear Colleagues
}
} I have used an AGFA Duoscan 1200 for some years for TEM negatives.
} Recently it stopped working and it seems that it is easier to buy a new
} one than repair the old machine.
}
} Can anyone recomend a suitable (inexpensive) machine?
} As far as my experience goes, the low end scanners do not give acceptable
} results with dense negatives. The Duoscan was acceptable perhaps due to
} better
} sensitivity. More sensitive scanners may become too expensive for our lab.
} So, I'm looking for a suitable compromise: enough sensitivity v. lowest
} price
}
} Thanks in advance
}
} A.P. Alves de Matos
} Biologist
} Electron Microscopy Unit
} Curry Cabral Hospital, Lisbon

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 09:16:09 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

William Stratton wrote:
================================================
Does anyone know where I can buy Loctite 460 superglue? How about the
softer black wax (Apeizon brand?).

I've been looking around online and I cannot find either of these sample
prep items. Any help would be great.
================================================
All three of the Apiezon waxes, all black, can be found on URL
http://www.2spi.com/catalog/vac/apiezon-waxes.html

We offer the Duro brand cyanoacrylate "super glue" on URL
http://www.2spi.com/catalog/spec_prep/superglue.shtml

Disclaimer: SPI Supplies offers for sale the above mentioned products.

Chuck

PS: Remember that we are striving to be 100% paperless, therefore there
are no paper copies kept of this correspondence. Please be sure to always
reply by way of "reply" on your software so that the entire string of
correspondence can be kept in one place.
============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
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Cust.Service: spi2spi-at-2spi.com

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From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 10:21:58 2004

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William:

The Black Wax is available from South Bay Technology under part no.
MWM100. Please request information on our entire range of mounting
waxes as you may find something else that would be equally suitable.
I'll be happy to send you samples.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

William Stratton wrote:

} ------------------------------------------------------------------------------
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David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
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TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
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email: henriks-at-southbaytech.com

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Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 10:48:08 2004

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Dental impression materials work well for this type of purpose; they should
be available from any dental supplier. There are several different types,
but the most commonly used is the polyvinyl siloxane type, sold under
various brand names. Ask for the light body version of whichever brand you
choose.

Lesley Weston.

on 23/03/2004 5:30 AM, by way of Ask-A-Microscopist at
jrobson-at-rdg.boehringer-ingelheim.com wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted
} by (jrobson-at-rdg.boehringer-ingelheim.com) from
} http://www.msa.microscopy.org/Ask-A-Microscopist.html on Tuesday, March 23,
} 2004 at 06:41:11
} ---------------------------------------------------------------------------
}
} Email: jrobson-at-rdg.boehringer-ingelheim.com
} Name: John Robson
}
} Organization: Boehringer Ingelheim
}
} Education: Undergraduate College
}
} Location: Danbury, CT
}
} Question: I've been asked to perform several measurements on a polyethylene
} part. I need to determine the length and diameter (at several points) of a
} channel that is roughly 0.3mm wide X ~2.0mm long. Years ago we had worked
} with latex casting materials for this purpose unfortunately shrinkage was a
} constant issue. I would appreciate any recommendations on alternative casting
} materials that would allow us to accurately reproduce an impression of the
} part with minimal shrinkage. Thank You, John.
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 11:20:17 2004

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Hi,

About the Loctite 460, you can find it in hardware stores.

On Tue, 23 Mar 2004, William Stratton wrote:

}
} Greetings all,
}
} Does anyone know where I can buy Loctite 460 superglue? How about the
} softer black wax (Apeizon brand?).
}
} I've been looking around online and I cannot find either of these sample
} prep items. Any help would be great.
}
} Have a good week,
}
} William Stratton
}
} -------------------
} William G. Stratton
} Research Assistant
} University of Wisconsin - Madison

o-------------------------------------------------------o
| Carlos Kazuo Inoki |
| Department of Physics - University at Albany |
| 1400 Washington Ave.- Albany - NY - 12222 |
o-------------------------------------------------------o

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 11:30:38 2004

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Hi,

Sorry for the last message. My fingers slip and hit the send. :)
As I said you can buy Loctite 460 superglue em hardware stores. We found
one close to us by checking the Loctite webpage, that carries the list of
distribuitors (www.loctite.com). Another place we used to by was EMS, but
last time I did check they didn't have it.

Now, the last batch of Loctite 460 we bought, it came from HMC
Electronics (www.hmcelectronics.com). You can check under
Adhesives & Sealants/Instant Adhesives. Hope this helps.

Regards,

Carlos

On Tue, 23 Mar 2004, William Stratton wrote:

}
} Greetings all,
}
} Does anyone know where I can buy Loctite 460 superglue? How about the
} softer black wax (Apeizon brand?).
}
} I've been looking around online and I cannot find either of these sample
} prep items. Any help would be great.
}
} Have a good week,
}
} William Stratton
}
} -------------------
} William G. Stratton
} Research Assistant
} University of Wisconsin - Madison
}

o-------------------------------------------------------o
| Carlos Kazuo Inoki |
| Department of Physics - University at Albany |
| 1400 Washington Ave.- Albany - NY - 12222 |
o-------------------------------------------------------o

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 13:11:35 2004

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Hi,

I'd suggest you contact Dr. Gina Semprebon at Bay Path College in Longmeadow (gsempreb-at-baypath.edu P: 413-565-1366). She did her PhD dissertation on the study of teeth of prehistoric animals and found a great way of making replicas to use in the SEM.

Also interesting: we have looked at teeth in the confocal. They are autofluorescence and present a very SEM-like view without all the vacuum and sample prep.

Good Hunting!
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

~-at-~-at-~~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
At 09:19 AM 3/22/04 -0600, Dusevich, Vladimir wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 16:24:17 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (stephan.reineke-at-gmx.de) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 23, 2004 at 13:59:52
---------------------------------------------------------------------------

Email: stephan.reineke-at-gmx.de
Name: Stephan Reineke

Organization: University of Osnabrueck, Department of Animal Physiology

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello,

does anybody know why OsO4 binds only to the hydrophilic part of plasma membranes to arouse the lamellar structure in electron microscopy pictures? Especially when itĄs known that OsO4 reacts with double bonds as in fatty acids.

Thanks a lot for the response

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 16:23:32 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rcasillas-at-techinst.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 23, 2004 at 12:15:06
---------------------------------------------------------------------------

Email: rcasillas-at-techinst.com
Name: Roberto Casillas

Title-Subject: [Microscopy] [Filtered] FRET

Question: Hello all,

My question today is with respect to the RM-FRET Sytems from Photon Technology International.

I have an application where I would like to determin if FRET is occuring between Alexa Fluor 568 and Alexa fluor 647 as one pair and the second pair is cy3.5 and cy5.5.

The main question is am I better off with the Photon systems device with its PMT and software or with an Optical Insights Dual View properly outfitted with the apropriate filters, simple PCI software and a nice camera like a Coolsnap HQ?

Thanks for any asistance and best regards,

Roberto

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 19:54:14 2004

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Stephan,
I am not sure if I know but as you stated OsO4 reacts with double bonds
in lipids. If I remember correctly (it's been a while!) lower Osmium
oxides result from these reactions and these oxides are bound to the
hydrophobic fatty acid chains which as a result become more
hydrophilic. Next the more hydrophilic lipid tails are thought to bend
away from the hydrophobic interior of the membrane towards the
polarized heads of the lipids which in terms of energy would be a more
favoured situation. So the Osmium signal only occurs in the hydrophilic
area as a the result of a secondary process, not by directly binding
there.

Jan

} Question: Hello,
}
} does anybody know why OsO4 binds only to the hydrophilic part of
} plasma membranes to arouse the lamellar structure in electron
} microscopy pictures? Especially when itĄs known that OsO4 reacts with
} double bonds as in fatty acids.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 23 21:31:28 2004

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Richard
Consider this: you may buy UA from any EM supplier using your own credit
card (I think so, never tried). So, you don't need to provide
"authorization number" or number of your licence to use radioactive
materials to buy UA. I could not imagine, how your authorities could
dictate you what to buy (and use) on your credit card etc. There is a lot
of controversy here. I went through that nightmare when decided to try
uranium for shadowing. It took almost two years to go through. They are
so concerned about 75 g of depleted uranium that they just don't care about
UA... You have to see how they jump out when I demonstrate to them U (that
I did not use it to make nuclear bomb, I guess) and they disappeared very
quickly ... untill next year. There is some benefit from having metal
uranium in your drawer. Sergey.

At 05:45 AM 3/23/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 08:18:28 2004

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Hi, all,

I am posting this on behalf of a mycologist colleague who does not
subscribe to the list.

She would like to know of any vital stains that exist for heavily
melanized fungal spores. The spores she's studying are very dark in
colour and so present a unique problem. She is concerned that any
treatment which removes the melanin would damage the spore structure,
and add another variable.

If you can help, please reply to me and I'll forward the replies to
her.

Thanks in advance.

Paula.

Paula M. Allan-Wojtas
Research Scientist - Food Microstructure / Chercheur scientique -
microstructure des aliments
Food Safety and Quality Team / Salubrité et qualité des aliments
Agriculture and Agri-Food Canada /Agriculture et Agroalimentaire
Canada
Telephone / Téléphone: 902-679-5566
Facsimile / Télécopieur: 902-679-2311
32 Main Street / 32 rue Main
Kentville, Nova Scotia / Kentville (Nouvelle-Écosse)
B4N 1J5
allanwojtasp-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 08:41:37 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all,
I need some advice.
A professor in my dept. would like to "go digital". For many years he
has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
photographs of small seeds (about 0.5 mm). He's been working in Costa
Rica and Ecuador so I haven't actually seen the set-up. His description
of it makes it sound similar to a slide copier set-up rather than a
copy stand.
Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
camera coupled to a dissecting scope.
Any other suggestions are greatly appreciated...he's writing a grant
and wants this info by tomorrow...of course! ;-)
thanks,
Beth
**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 09:42:40 2004

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Hi Paula:

I think the place to start is with "traditional" vital stains like
janus green, neutral red, etc and see what sort of results can be
acquired. Another possibility is phase contrast microscopy or Nomarski
DIC. If the spores are so heavily melanized she can't see much then
bleaching out the melanin is an obvious step. She could use phase or
Nomarski to compare structure before and after bleaching. Saying that
the spores are too dark but not wanting to bleach them seems
counter-productive. As always, what does the literature say on this topic?

Geoff

Paula Allan-Wojtas wrote:

} Hi, all,
}
} I am posting this on behalf of a mycologist colleague who does not
} subscribe to the list.
}
} She would like to know of any vital stains that exist for heavily
} melanized fungal spores. The spores she's studying are very dark in
} colour and so present a unique problem. She is concerned that any
} treatment which removes the melanin would damage the spore structure,
} and add another variable.
}
} If you can help, please reply to me and I'll forward the replies to
} her.
}
} Thanks in advance.
}
} Paula.
}
}
}
} Paula M. Allan-Wojtas
} Research Scientist - Food Microstructure / Chercheur scientique -
} microstructure des aliments
} Food Safety and Quality Team / Salubrité et qualité des aliments
} Agriculture and Agri-Food Canada /Agriculture et Agroalimentaire
} Canada
} Telephone / Téléphone: 902-679-5566
} Facsimile / Télécopieur: 902-679-2311
} 32 Main Street / 32 rue Main
} Kentville, Nova Scotia / Kentville (Nouvelle-Écosse)
} B4N 1J5
} allanwojtasp-at-agr.gc.ca
}
}
}
}
}
}
}
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 10:20:57 2004

Contents Retrieved from Microscopy Listserver Archives
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Beth, I've used both setups, a 35mm camera with
bellows and digital camera with stereobinoculars. The
35mm/bellows went to 50X magnification and gave
wonderful resolution on a 4"x6" print.

In my opinion the 35mm camera gives superior pictures
for presentation. If the 35mm prints will be
subsequently scanned before presentation, they
probably lose all benefit over digital cameras.

Digital cameras are getting considerably better. The
Nikon Coolpix 4500 (I'm not familiar with the 990/995)
gives good pictures, and is considered by some as the
standard digital workhorse in microscopic imaging
labs. It's hard to beat the convenience of a digital
camera. The images can always be tweaked by image
handling software to enhance presentation.

One caveat with stereobinoculars is that the proper
coupling must be used to marry the camera to the
stereobinoculars. There is a source for the coupler,
but I lost the link to that source. Using a homemade
or improper coupler can give all kinds of undesirable
optical artifacts such as barreling, pincushion, and
streaky images.

There are sources that sell complete packages (camera
& scope), where everything is engineered for optimal
performance. One such source is Mager Scientific in
Dexter, Michigan. They specialize in digital
microscopy imaging.

(Disclaimer: I have no interest in Mager Scientific,
Inc., I'm just a satisfied customer.)

Stu Smalinskas, P.E.
Sr. Metallurgist
SKF
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Beth wrote:
Hi all,
I need some advice. A professor in my dept. would
like to "go digital". For many years he has been using
a Nikon 35mm camera, bellows, and an AIS lens to shoot
photographs of small seeds (about 0.5 mm). He's been
working in Costa Rica and Ecuador so I haven't
actually seen the set-up. His description of it makes
it sound similar to a slide copier set-up rather than
a copy stand.

Anyway, my solution would be to use a Nikon Coolpix
990/995/or 4500 camera coupled to a dissecting scope.
Any other suggestions are greatly appreciated...he's
writing a grant and wants this info by tomorrow...of
course! ;-)
thanks,
Beth

Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

__________________________________
Do you Yahoo!?
Yahoo! Finance Tax Center - File online. File on time.
http://taxes.yahoo.com/filing.html

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 11:15:15 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We used a Nikon Coolpix 5000 to connect to our Nikon stereoscope. In my
opinion, it works really well. If your stereoscope has the proper
connections for a camera already present, you can use the same attachment
that we used. It was from MVIA Inc (http://www.mvia.com).

Also Nikon.com sometimes sells repaired Coolpix cameras (good place to look
for a cheap high quality camera).

Best of luck,

William Stratton

-------------------
William G. Stratton
Research Assistant
Voyles Research Group
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu
http://www.cae.wisc.edu/~stratton/

-----Original Message-----
} From: Beth Richardson [mailto:beth-at-plantbio.uga.edu]
Sent: Wednesday, March 24, 2004 9:03 AM
To: microscopy

Hi all,
I need some advice.
A professor in my dept. would like to "go digital". For many years he
has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
photographs of small seeds (about 0.5 mm). He's been working in Costa
Rica and Ecuador so I haven't actually seen the set-up. His description
of it makes it sound similar to a slide copier set-up rather than a
copy stand.
Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
camera coupled to a dissecting scope.
Any other suggestions are greatly appreciated...he's writing a grant
and wants this info by tomorrow...of course! ;-)
thanks,
Beth
**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 12:06:44 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Beth:

Better solution is to go Nikon digital SLR (i.e. 35mm replacment) like the
Nikon D70 ($1000), Nikon D2H ($3100), Nikon D100 ($1600).

Why? He can just replace the camera body and use the rest of his
bellows, lenses, etc. He knows how to use a Nikon SLR, why change? Why
suddenly use a dissecting scope if he can get what he needs with his 35mm
Nikon? Since its for a grant pick a price, list a camera at that price, and then
he can get the best camera he can for the funds when the grant is funded
(Digital world changes to fast.)

The Foveon's X3 sensor cameras are even better in terms of scientific
imaging (they are NOT mosaic filter sensors) like the Sigma SD10 ($1600), or
SD9 - but the the lens mounts are different and he'd need new bellows, lenses
etc.

} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ************************************************************************
} ***
}
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 12:06:01 2004

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If you are not pinched for money and want a digital image
with a standard camera body (easy to interface via
existing optics) look at the recent announcement below.
The performance on this system finally has me thinking
about getting a digital camera. I have no connection with
this vendor but they often have very good prices as well
as used equipment.

Kodak introduced an updated version of the Pro 14N at PMA
- the Pro SLR/n,
AND now their full frame camera is available in a CANON
version! These cameras
will begin shipping in May - so order your camera now!!

Kodak Pro SLR/c features:

* Canon EF Lens compatible
* 14MP file size
* Highest Resolution and ISO Range of ANY camera on the
market
* ISO Range from 0-1600
* Full Size 35mm allows for wide angle capture benefits
* New CMOS Imager with HPLN Technology (High Performance,
Low Noise)
* Image Burst up to 19 frames
* FREE Firmware and Software Updates at any time

In addition to the newly upgraded CMOS Chip, the DCS Pro
SLR/c Digital
Camera also features a "longer" exposure mode, enabling
exposures up to
30 seconds at lower ISO settings with an integrated 512MB
RAM buffer; and a
"sleep mode," which conserves battery life. Go to
http://www.promarketinc.com/
for additional formation. Our Introductory Price for
preorders on the Pro SLR/c is
just $4,749! We also have a demo Pro SLR/n in stock!

Larry Ackerman
Keck Advanced Microscopy Lab
Dept. of Biochemistry & Biophysics
University of California San Francisco
600-16th Street, Room S101, Box 2140
San Francisco, CA 94158 (for postal mail use 94143)

415-476-4441 FAX 415-514-4142

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 12:55:35 2004

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Beth,

We use a Nikon Coolpix 5000 on a trinocular dissecting scope and it is working
very well. We bought the whole package from a used microscope co. in
Pennsylvania, Conneaut Lake Scientific http://www.conneautlakesci.com/.

No financial interest in the co. just a happy customer.

Soumitra

Quoting Beth Richardson {beth-at-plantbio.uga.edu} :

}
}
} -----------------------------------------------------------------------------
-
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------------
--
}
} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ************************************************************************
} ***
}
}
}
}

Soumitra Ghoshroy Ph.D
College Associate Professor, Biology
Director, Electron Microscopy Lab
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office)
505-646-3283 (lab)
Fax: 505-646-3282

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 13:20:29 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I can definatly recommend the Nikon D100, or the upcoming, much cheaper,
D70. Since I bought a D100 for our lab, everyone is stunned with it's
performances. Easy-to-use, nice colors, sharpness. The only negative mark
is the shuttertime delay of 1/2 second or something about that (which is
actually normal with digital photography until now, but it's being said to
be resolved in the D70).

The Nikon D100 can be used with old and new lenses from Nikon (the Nikkor
series), Vivtar etc. and I must admit that the 105mm Macro is a very nice
lens (hence not cheap!). But! Attachment to stereomicroscopes or
fluorescencemicroscopes is very simple if they are provided with a C-mount.
Just like in the old days, where you attached an analogue SLR, you now
attach the digital camera.

For it's price, a very good camera with many capabilities, photos with a
resolution up to 6 Megs (make that computer crash, yeah!), comparable to the
previous SLR analogs.

And now the bad news...well, bad: I'm a fan of analogue photographhy since a
digital camera still ain't capable of doing what an analogue camera can.
Unless the high speed with which your photos are available with a digital,
another plus for digitals, colors still aren't the same, high speed of
shuttertime might be important and you don't get it, and last but not least,
how high the quality of pixels is, the old negatives, and especially the
dias, still can provide you better resolution when scanning them. But,
that's my opinion. And I must say, I also really enjoy a lot to see a photo
appearing on paper while developping...from white paper where slowly a foggy
image appears as if it's a revelation of the paper trying to tell you
something by images...but I'm getting too nostalgic now... ;-)

In these days of progression, speed and fast results, I would recommend the
Nikon D100 or D70 (but if you have more time, a good negative scanner and an
old camera). And no, I do not have any deal with Nikon. You like what you
use and you use what you like, that's common knowledge.

Best regards,

Sven Terclavers

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOHIO.EDU]
Sent: Wednesday, March 24, 2004 19:28 PM
To: Beth Richardson
Cc: microscopy-at-MSA.Microscopy.com

Beth:

Better solution is to go Nikon digital SLR (i.e. 35mm replacment) like the
Nikon D70 ($1000), Nikon D2H ($3100), Nikon D100 ($1600).

Why? He can just replace the camera body and use the rest of his
bellows, lenses, etc. He knows how to use a Nikon SLR, why change? Why
suddenly use a dissecting scope if he can get what he needs with his 35mm
Nikon? Since its for a grant pick a price, list a camera at that price, and
then
he can get the best camera he can for the funds when the grant is funded
(Digital world changes to fast.)

The Foveon's X3 sensor cameras are even better in terms of scientific
imaging (they are NOT mosaic filter sensors) like the Sigma SD10 ($1600), or
SD9 - but the the lens mounts are different and he'd need new bellows,
lenses
etc.

} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ************************************************************************
} ***
}
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 13:22:22 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

if you need a digital camera coupler let me know. We have a
list of digital cameras, SLR cameras, C-Mount cameras which
we all can connect to a C-Mount coupler or to an eyepiece.
You even could add a camcorder to a microscope.

If you would like to receive our list of cameras we can
connect to a microscope, please let me know, I can send it
to you by email.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

WS} ------------------------------------------------------------------------------
WS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
WS} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
WS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
WS} -------------------------------------------------------------------------------

WS} We used a Nikon Coolpix 5000 to connect to our Nikon stereoscope. In my
WS} opinion, it works really well. If your stereoscope has the proper
WS} connections for a camera already present, you can use the same attachment
WS} that we used. It was from MVIA Inc (http://www.mvia.com).

WS} Also Nikon.com sometimes sells repaired Coolpix cameras (good place to look
WS} for a cheap high quality camera).

WS} Best of luck,

WS} William Stratton

WS} -------------------
WS} William G. Stratton
WS} Research Assistant
WS} Voyles Research Group
WS} University of Wisconsin - Madison

WS} 1509 University Avenue
WS} Madison, WI 53706
WS} Office: 608-265-6391
WS} Fax: 608-262-8353
WS} wgstratton-at-wisc.edu
WS} http://www.cae.wisc.edu/~stratton/

WS} -----Original Message-----
} } From: Beth Richardson [mailto:beth-at-plantbio.uga.edu]
WS} Sent: Wednesday, March 24, 2004 9:03 AM
WS} To: microscopy
WS} Subject: [Microscopy] camera set-up

WS} ----------------------------------------------------------------------------
WS} --
WS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
WS} To Subscribe/Unsubscribe --
WS} http://www.msa.microscopy.com/MicroscopyListserver
WS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
WS} ----------------------------------------------------------------------------
WS} ---

WS} Hi all,
WS} I need some advice.
WS} A professor in my dept. would like to "go digital". For many years he
WS} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
WS} photographs of small seeds (about 0.5 mm). He's been working in Costa
WS} Rica and Ecuador so I haven't actually seen the set-up. His description
WS} of it makes it sound similar to a slide copier set-up rather than a
WS} copy stand.
WS} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
WS} camera coupled to a dissecting scope.
WS} Any other suggestions are greatly appreciated...he's writing a grant
WS} and wants this info by tomorrow...of course! ;-)
WS} thanks,
WS} Beth
WS} **********************************************************************
WS} Beth Richardson
WS} EM Lab Coordinator
WS} Plant Biology Department
WS} University of Georgia
WS} Athens, GA 30602-7271

WS} Phone - (706) 542-1790 & FAX - (706) 542-1805

WS} "Between the two evils,
WS} I always pick the one I never tried before". Mae West (1893-1980)
WS} *******************************************************************

WS} "And it's only the giving that makes you what you are".
WS} Wond'ring Aloud, Jethro Tull (Aqualung)

WS} ************************************************************************
WS} ***

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 14:00:54 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I can definatly recommend the Nikon D100, or the upcoming, much cheaper,
D70. Since I bought a D100 for our lab, everyone is stunned with it's
performances. Easy-to-use, nice colors, sharpness. The only negative mark
is the shuttertime delay of 1/2 second or something about that (which is
actually normal with digital photography until now, but it's being said to
be resolved in the D70).

The Nikon D100 can be used with old and new lenses from Nikon (the Nikkor
series), Vivtar etc. and I must admit that the 105mm Macro is a very nice
lens (hence not cheap!). But! Attachment to stereomicroscopes or
fluorescencemicroscopes is very simple if they are provided with a C-mount.
Just like in the old days, where you attached an analogue SLR, you now
attach the digital camera.

For it's price, a very good camera with many capabilities, photos with a
resolution up to 6 Megs (make that computer crash, yeah!), comparable to the
previous SLR analogs.

And now the bad news...well, bad: I'm a fan of analogue photographhy since a
digital camera still ain't capable of doing what an analogue camera can.
Unless the high speed with which your photos are available with a digital,
another plus for digitals, colors still aren't the same, high speed of
shuttertime might be important and you don't get it, and last but not least,
how high the quality of pixels is, the old negatives, and especially the
dias, still can provide you better resolution when scanning them. But,
that's my opinion. And I must say, I also really enjoy a lot to see a photo
appearing on paper while developping...from white paper where slowly a foggy
image appears as if it's a revelation of the paper trying to tell you
something by images...but I'm getting too nostalgic now... ;-)

In these days of progression, speed and fast results, I would recommend the
Nikon D100 or D70 (but if you have more time, a good negative scanner and an
old camera). And no, I do not have any deal with Nikon. You like what you
use and you use what you like, that's common knowledge.

Best regards,

Sven Terclavers

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOHIO.EDU]
Sent: Wednesday, March 24, 2004 19:28 PM
To: Beth Richardson
Cc: microscopy-at-MSA.Microscopy.com

Beth:

Better solution is to go Nikon digital SLR (i.e. 35mm replacment) like the
Nikon D70 ($1000), Nikon D2H ($3100), Nikon D100 ($1600).

Why? He can just replace the camera body and use the rest of his
bellows, lenses, etc. He knows how to use a Nikon SLR, why change? Why
suddenly use a dissecting scope if he can get what he needs with his 35mm
Nikon? Since its for a grant pick a price, list a camera at that price, and
then
he can get the best camera he can for the funds when the grant is funded
(Digital world changes to fast.)

The Foveon's X3 sensor cameras are even better in terms of scientific
imaging (they are NOT mosaic filter sensors) like the Sigma SD10 ($1600), or
SD9 - but the the lens mounts are different and he'd need new bellows,
lenses
etc.

} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ************************************************************************
} ***
}
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 14:00:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi,

if you need a digital camera coupler let me know. We have a
list of digital cameras, SLR cameras, C-Mount cameras which
we all can connect to a C-Mount coupler or to an eyepiece.
You even could add a camcorder to a microscope.

If you would like to receive our list of cameras we can
connect to a microscope, please let me know, I can send it
to you by email.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

WS} ------------------------------------------------------------------------------
WS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
WS} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
WS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
WS} -------------------------------------------------------------------------------

WS} We used a Nikon Coolpix 5000 to connect to our Nikon stereoscope. In my
WS} opinion, it works really well. If your stereoscope has the proper
WS} connections for a camera already present, you can use the same attachment
WS} that we used. It was from MVIA Inc (http://www.mvia.com).

WS} Also Nikon.com sometimes sells repaired Coolpix cameras (good place to look
WS} for a cheap high quality camera).

WS} Best of luck,

WS} William Stratton

WS} -------------------
WS} William G. Stratton
WS} Research Assistant
WS} Voyles Research Group
WS} University of Wisconsin - Madison

WS} 1509 University Avenue
WS} Madison, WI 53706
WS} Office: 608-265-6391
WS} Fax: 608-262-8353
WS} wgstratton-at-wisc.edu
WS} http://www.cae.wisc.edu/~stratton/

WS} -----Original Message-----
} } From: Beth Richardson [mailto:beth-at-plantbio.uga.edu]
WS} Sent: Wednesday, March 24, 2004 9:03 AM
WS} To: microscopy
WS} Subject: [Microscopy] camera set-up

WS} ----------------------------------------------------------------------------
WS} --
WS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
WS} To Subscribe/Unsubscribe --
WS} http://www.msa.microscopy.com/MicroscopyListserver
WS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
WS} ----------------------------------------------------------------------------
WS} ---

WS} Hi all,
WS} I need some advice.
WS} A professor in my dept. would like to "go digital". For many years he
WS} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
WS} photographs of small seeds (about 0.5 mm). He's been working in Costa
WS} Rica and Ecuador so I haven't actually seen the set-up. His description
WS} of it makes it sound similar to a slide copier set-up rather than a
WS} copy stand.
WS} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
WS} camera coupled to a dissecting scope.
WS} Any other suggestions are greatly appreciated...he's writing a grant
WS} and wants this info by tomorrow...of course! ;-)
WS} thanks,
WS} Beth
WS} **********************************************************************
WS} Beth Richardson
WS} EM Lab Coordinator
WS} Plant Biology Department
WS} University of Georgia
WS} Athens, GA 30602-7271

WS} Phone - (706) 542-1790 & FAX - (706) 542-1805

WS} "Between the two evils,
WS} I always pick the one I never tried before". Mae West (1893-1980)
WS} *******************************************************************

WS} "And it's only the giving that makes you what you are".
WS} Wond'ring Aloud, Jethro Tull (Aqualung)

WS} ************************************************************************
WS} ***

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 14:23:02 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We are currently imaging several haloarchaea using TEM and we have been
getting nice images of whole cells using both negative and UA/LC enbloc
staining. Our next step is to follow the attachment and movement of halocins
onto and through their membranes. However we are having difficulty locating
specific references in the recent literature that describe applicable
protocols utilizing gold labeling techniques to follow the halocin over time
and so we have turned to the well of knowledge that is the microscopy list
serve. We would appreciate any suggestions, citations or links from those that
have expertise in this area. Thanks in advance.
Pete

Peter J. Polsgrove, R.A. Microbiology
Shand Lab at Northern Arizona University Flagstaff, AZ.
H-928-214-9446_Cell-928-600-1004_Lab-928-523-6145
pjp6-at-dana.ucc.nau.edu
micro2001p-at-netscape.net

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 14:48:22 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

As a commercial photographer of 25 years and one who now shoots all digital
for the last 2 years I've had extensive experience with several of the high
end professional digital cameras. I've owned a Nikon D1, D1X and a Fuji S2.
The Nikons are solid very well built, but heavy pro cameras. The Fuji
produces a higher resolution image but is hampered by a mediocre user
interface and poor battery design.

In light of those experiences, I looked at Kodak's new Pro SLR/n at the
industry show in Las Vegas last month. It's has an 8 Megapixel full-frame
sensor which produces large files. It has a well designed interface based on
Kodak's long experience producing pro digital cameras. Unfortunately the
camera has some noticeable problems with the images it produces. There are
green/magenta fringes along the edge of images depending on the lens one
uses. Many pros who have bought this camera are tearing their hair out
waiting for Kodak to fix the problem with changes to the cameras firmware.
The dialog among these photographers can be read at the user forums at
www.robgalbraith.com, a pro photo site.

For any of you contemplating the purchase of the newest Kodak SLR/n camera I
would suggest two things: Wait until Kodak has fixed the color problem in
firmware V5 (currently at 4.5.5) and make sure your dealer has a reasonable
test period and a return policy if the camera does not perform to your
needs. The previous 14n model is best suited to studio situations with
plenty of light or used out-of-doors in sunlight with a low ISO setting as
it produces excessive noise at higher ISOs.

Regards,
Doug Baldwin
Baldwin Photography
Scottsdale, Arizona
(neophyte microscope user)

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 15:00:56 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi,

if you need a digital camera coupler let me know. We have a
list of digital cameras, SLR cameras, C-Mount cameras which
we all can connect to a C-Mount coupler or to an eyepiece.
You even could add a camcorder to a microscope.

If you would like to receive our list of cameras we can
connect to a microscope, please let me know, I can send it
to you by email.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

WS} ------------------------------------------------------------------------------
WS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
WS} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
WS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
WS} -------------------------------------------------------------------------------

WS} We used a Nikon Coolpix 5000 to connect to our Nikon stereoscope. In my
WS} opinion, it works really well. If your stereoscope has the proper
WS} connections for a camera already present, you can use the same attachment
WS} that we used. It was from MVIA Inc (http://www.mvia.com).

WS} Also Nikon.com sometimes sells repaired Coolpix cameras (good place to look
WS} for a cheap high quality camera).

WS} Best of luck,

WS} William Stratton

WS} -------------------
WS} William G. Stratton
WS} Research Assistant
WS} Voyles Research Group
WS} University of Wisconsin - Madison

WS} 1509 University Avenue
WS} Madison, WI 53706
WS} Office: 608-265-6391
WS} Fax: 608-262-8353
WS} wgstratton-at-wisc.edu
WS} http://www.cae.wisc.edu/~stratton/

WS} -----Original Message-----
} } From: Beth Richardson [mailto:beth-at-plantbio.uga.edu]
WS} Sent: Wednesday, March 24, 2004 9:03 AM
WS} To: microscopy
WS} Subject: [Microscopy] camera set-up

WS} ----------------------------------------------------------------------------
WS} --
WS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
WS} To Subscribe/Unsubscribe --
WS} http://www.msa.microscopy.com/MicroscopyListserver
WS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
WS} ----------------------------------------------------------------------------
WS} ---

WS} Hi all,
WS} I need some advice.
WS} A professor in my dept. would like to "go digital". For many years he
WS} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
WS} photographs of small seeds (about 0.5 mm). He's been working in Costa
WS} Rica and Ecuador so I haven't actually seen the set-up. His description
WS} of it makes it sound similar to a slide copier set-up rather than a
WS} copy stand.
WS} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
WS} camera coupled to a dissecting scope.
WS} Any other suggestions are greatly appreciated...he's writing a grant
WS} and wants this info by tomorrow...of course! ;-)
WS} thanks,
WS} Beth
WS} **********************************************************************
WS} Beth Richardson
WS} EM Lab Coordinator
WS} Plant Biology Department
WS} University of Georgia
WS} Athens, GA 30602-7271

WS} Phone - (706) 542-1790 & FAX - (706) 542-1805

WS} "Between the two evils,
WS} I always pick the one I never tried before". Mae West (1893-1980)
WS} *******************************************************************

WS} "And it's only the giving that makes you what you are".
WS} Wond'ring Aloud, Jethro Tull (Aqualung)

WS} ************************************************************************
WS} ***

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 15:00:55 2004

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------------------------------------------------------------------------------
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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I can definatly recommend the Nikon D100, or the upcoming, much cheaper,
D70. Since I bought a D100 for our lab, everyone is stunned with it's
performances. Easy-to-use, nice colors, sharpness. The only negative mark
is the shuttertime delay of 1/2 second or something about that (which is
actually normal with digital photography until now, but it's being said to
be resolved in the D70).

The Nikon D100 can be used with old and new lenses from Nikon (the Nikkor
series), Vivtar etc. and I must admit that the 105mm Macro is a very nice
lens (hence not cheap!). But! Attachment to stereomicroscopes or
fluorescencemicroscopes is very simple if they are provided with a C-mount.
Just like in the old days, where you attached an analogue SLR, you now
attach the digital camera.

For it's price, a very good camera with many capabilities, photos with a
resolution up to 6 Megs (make that computer crash, yeah!), comparable to the
previous SLR analogs.

And now the bad news...well, bad: I'm a fan of analogue photographhy since a
digital camera still ain't capable of doing what an analogue camera can.
Unless the high speed with which your photos are available with a digital,
another plus for digitals, colors still aren't the same, high speed of
shuttertime might be important and you don't get it, and last but not least,
how high the quality of pixels is, the old negatives, and especially the
dias, still can provide you better resolution when scanning them. But,
that's my opinion. And I must say, I also really enjoy a lot to see a photo
appearing on paper while developping...from white paper where slowly a foggy
image appears as if it's a revelation of the paper trying to tell you
something by images...but I'm getting too nostalgic now... ;-)

In these days of progression, speed and fast results, I would recommend the
Nikon D100 or D70 (but if you have more time, a good negative scanner and an
old camera). And no, I do not have any deal with Nikon. You like what you
use and you use what you like, that's common knowledge.

Best regards,

Sven Terclavers

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOHIO.EDU]
Sent: Wednesday, March 24, 2004 19:28 PM
To: Beth Richardson
Cc: microscopy-at-MSA.Microscopy.com

Beth:

Better solution is to go Nikon digital SLR (i.e. 35mm replacment) like the
Nikon D70 ($1000), Nikon D2H ($3100), Nikon D100 ($1600).

Why? He can just replace the camera body and use the rest of his
bellows, lenses, etc. He knows how to use a Nikon SLR, why change? Why
suddenly use a dissecting scope if he can get what he needs with his 35mm
Nikon? Since its for a grant pick a price, list a camera at that price, and
then
he can get the best camera he can for the funds when the grant is funded
(Digital world changes to fast.)

The Foveon's X3 sensor cameras are even better in terms of scientific
imaging (they are NOT mosaic filter sensors) like the Sigma SD10 ($1600), or
SD9 - but the the lens mounts are different and he'd need new bellows,
lenses
etc.

} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ************************************************************************
} ***
}
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 15:49:24 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Colleagues:

List members in the Pittsburgh, PA area who have an interest in materials science are cordially invited to a free two-day "mini-workshop" on Cryoultramicrotomy for The Materials Sciences.

This topic is of special interest for those who work with polymers or other materials which could benefit from ultrathin sectioning or surface "polishing" at low temperatures (no embedding required).

The workshop will be hosted by the RJ Lee Group, Inc. in Monroeville, PA. The invitation is open to everyone in the Pittsburgh, PA / Youngstown, OH / Akron, OH area.

The details are as follows:

**What**:
Mini-Workshop on Cryoultramicrotomy for Materials Science

**When**:
Tuesday, April 6th, 2004, 9:00 am through Wednesday, April 7th, 2004, 4:00 pm.

A tour of the facilities at RJ Lee Group will be given at the beginning of the workshop.

**Where**:
RJ Lee Group,Inc., 350 Hochberg Rd., Monroeville, PA.

**Format**:
A presentation on cryoultramicrotomy and its applications in the materials sciences will be given on the first day, as well as demonstrations on the preparation of cryotools (hair probes, large and small wire loops, etc.) and glass knife making and evaluation. The care and cleaning of diamond knives will also be discussed.

The demonstrations will be followed by open lab sessions for the attendees to prepare their own cryotools and glass knives.

Also on the first day an introduction to the cryoultramicrotome will be given, and attendees will have an opportunity for hands-on use of the Instrument.

The second day will be reserved for attendees to sign up in small groups for additional time and training on the instrumentation, depending on the attendees' individual needs.

**Limited Space Available**:
The lectures and demonstrations on the first day are open to everyone, but space is limited to *10 persons* for the in-depth training and extended use of the instrumentation on the second day.

**Contacts**:
To RSVP and to reserve a seat for the second day's sessions, please contact any of the following people:

Ms. Kim Megaw, RMC Products / Boeckeler Instruments, Inc.,
800.552.2262
{kim-at-boeckeler.com}

Mr. Hank Beebe, RJ Lee Group
724-325-1776
{hbeebe-at-rjlg.com}

Dr. Robert Chiovetti, RMC Products / Boeckeler Instruments, Inc.,
800.552.2262
{bob-at-boeckeler.com}

We hope to see you soon in Monroeville!

Robert (Bob) Chiovetti, Ph.D.
RMC Products
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 17:50:25 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mmckillip-at-smurfitlcom) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, March 24, 2004 at 12:25:08
---------------------------------------------------------------------------

Email: mmckillip-at-smurfitlcom
Name: M McKillip

Organization: Smurfit Stone Container Corp

Title-Subject: [Microscopy] [Filtered] MListserver:Embedding polymer films

Question: Is there a method to enhance polymer film bonding to a Poly/Bed 812 embedding medium. Frequently the thin films release from the embedding medium during microtoming.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 18:23:09 2004

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Beth,

Any Nikon Coolpix will do well, but Nikon D100 with one of standard macro lenses and add-on lenses is a much better solution. It
will produce great images up to mag. about 50X. Or, remove the lens, and install camera body on any microscope with 35 mm camera
port. F-mount fits directly, any other requires inexpensive adapter. Most cameras in this class (low end professional/high end
consumer) can be fully controlled by computer with optional software. De-tachable lens and sensor area equal to 35mm negative makes
microscope coupling much simpler.

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "Beth Richardson" {beth-at-plantbio.uga.edu}
To: "microscopy" {microscopy-at-msa.microscopy.com}
Sent: Wednesday, March 24, 2004 10:02 AM

There are several options for this sort of work.

If the past tasks were performed using 35mm film SLR,
a digital SLR may be a viable option. Keep in mind
that the high end digital SLRs use CCDs. The low end,
but not necessarily high quality, ones use CMOS sensors.
Nikon only uses CCDs. Regardless, the magnification
factor is 1.5 rather than 1:1. Thus, a 100mm macro lens
is actually 150mm. This may matter to him or not. Nikon
makes 60mm/105mm/200mm Micro-Nikkor lenses. Each one
has their own idiosyncrasies. Not bad, just different.
But all work with Nikon macro flash. Sort of.

That said, the digital bodies do not do TTL flash.
It is all manual. If using flash, one must get an
SB-80 regular flash or SB-29s macro in order to be
able to manually adjust the amount of flash. Film
SLRs will do TTL off of the film. Digital SLRs don't
do this. Fill flash is terrible. If the lighting is
solid halogen or other continuous source, not much
problem.

For Nikon mount, my personal and collective experience
puts Sigma at the bottom. Up from that is Fovea, D100,
then D1h, D2h and finally D1x. I do not personally consider
Kodak SLRs to be industrial strength. D1x in RAW mode
will do 10.5M pixels.

When I go on assignment, I take two D1x bodies, five
512MB Lexar USB CF modules, notebook computer and one
N-90s body. I will return with saleable pictures.

If a prosumer camera like CP990/995 or CP 5000 will
work, then clearly, chromatic aberration, spherical
aberration and non-flat field issues do not exist.
Go for the cheap prosumer digicam. A cheap $375
adapter will do the mating. Caveat emptor. The
other serious options are twice as costly. Even so,
they may not be viable in his environmental situation.

gary g.

At 07:02 AM 3/24/2004, you wrote:

} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ************************************************************************ ***
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 19:40:22 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Is anyone really truly 100% certain that a Nikon digital SLR body can be a
drop-in replacement for a Nikon 35mm SLR body?

We have a Nikon setup, with the Nikon FX-35WA body (essentially it's a
35mm camera body w/o metering or a mirror) which mounts onto the
microscope tube with a bayonet fitting that looks to me identical to that on
standard Nikon 35mm SLRs.

But when I've tried to put the D 1 (the early Nikon digital SLR) onto the
microscope tube, it doesn't want to fit. I've not liked to force it, and
concluded that there may be a subtle difference between the Nikon
bayonet mount on digital SLRs and that on 35mm SLRs.

Does anyone know what the story is here?

I gave up on thinking about it and bought a Coolpix plus the WPI interface,
which works well, and means that the D 1 isn't tied up on the microscope.

cheers

rtch

----------------------------------------------------
} ---------
}
} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His
} description of it makes it sound similar to a slide copier set-up
} rather than a copy stand. Anyway, my solution would be to use a Nikon
} Coolpix 990/995/or 4500 camera coupled to a dissecting scope. Any
} other suggestions are greatly appreciated...he's writing a grant and
} wants this info by tomorrow...of course! ;-) thanks, Beth
} **********************************************************************
} Beth Richardson EM Lab Coordinator Plant Biology Department University
} of Georgia Athens, GA 30602-7271
}

--
Ritchie Sims Ph D Phone : 64 9 3737599
ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 24 19:56:58 2004

Contents Retrieved from Microscopy Listserver Archives
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Yes, they can...with proper adapters.

I have, and have used, a Diagnostic Instrument PA1-10A
SLR adapter for Nikon F mount SLRs. It works fine
but lacks a locking click. Nevertheless, it works.
It works with F, F2, F3, F4, F5, N-xx Dxx.

That said, when you do this, the camera must be
in aperture preferred mode. Not all bodies like
this. So, YMMV.

gary g.

At 06:05 PM 3/24/2004, you wrote:

} Is anyone really truly 100% certain that a Nikon digital SLR body can be a
} drop-in replacement for a Nikon 35mm SLR body?
}
} We have a Nikon setup, with the Nikon FX-35WA body (essentially it's a
} 35mm camera body w/o metering or a mirror) which mounts onto the
} microscope tube with a bayonet fitting that looks to me identical to that on
} standard Nikon 35mm SLRs.
}
} But when I've tried to put the D 1 (the early Nikon digital SLR) onto the
} microscope tube, it doesn't want to fit. I've not liked to force it, and
} concluded that there may be a subtle difference between the Nikon
} bayonet mount on digital SLRs and that on 35mm SLRs.
}
} Does anyone know what the story is here?
}
} I gave up on thinking about it and bought a Coolpix plus the WPI interface,
} which works well, and means that the D 1 isn't tied up on the microscope.
}
} cheers
}
} rtch
}
}
} ----------------------------------------------------
} } ---------
} }
} } Hi all,
} } I need some advice.
} } A professor in my dept. would like to "go digital". For many years he
} } has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} } photographs of small seeds (about 0.5 mm). He's been working in Costa
} } Rica and Ecuador so I haven't actually seen the set-up. His
} } description of it makes it sound similar to a slide copier set-up
} } rather than a copy stand. Anyway, my solution would be to use a Nikon
} } Coolpix 990/995/or 4500 camera coupled to a dissecting scope. Any
} } other suggestions are greatly appreciated...he's writing a grant and
} } wants this info by tomorrow...of course! ;-) thanks, Beth
} } **********************************************************************
} } Beth Richardson EM Lab Coordinator Plant Biology Department University
} } of Georgia Athens, GA 30602-7271
} }
}
} --
} Ritchie Sims Ph D Phone : 64 9 3737599
} ext 87713
} Microanalyst Fax : 64 9 3737435
} Department of Geology email :
} r.sims-at-auckland.ac.nz
} The University of Auckland
} Private Bag 92019
} Auckland
} New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 07:44:22 2004

Contents Retrieved from Microscopy Listserver Archives
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Yes, the Standard Nikon F-mount is standard. The regularly swicth lenes,
microscope mounts between two older nikon 35mm film and our digital F-4
body (its a kodak DCS760 but built on the Nikon F-4).

The ONLY exceptions are: Autofocus features obviously will not work with non-
autofocus lenses (i.e. microscopes), and some extreme lenses project back
into the camera body signifcantly far. The digital cameras often have an IR
filter in front of the SLR mirror which may interfere with some lenses. The
filters are removeable on some Digitals but not all. (Which lenses? Extremes:
8mm Fisheye mostly, my camera lists a couple odd 20mm and one odd
45mm, but I've never seen anything in a microscope mount which projects
past the mounting flange itself.)

Perhaps someone else has some thing else to add?

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America To

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 07:46:44 2004

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Dear fellow microscopists,

Phil Swab teaches a technique at the RMC/Boeckeler materials
microtomy workshops which involves adding Z-6040 silane
(g-glycidoxypropyltrimethoxysilane), an epoxy primer, to a Spurrs
resin mixture to enhance adhesion. I haven't tried it with Poly/Bed
812, but it works wonders with thin film coatings in Spurrs.

best regards,
Steven Slap

At 6:12 PM -0600 3/24/04, by way of MicroscopyListserver wrote:
} Email: mmckillip-at-smurfitlcom
} Name: M McKillip
}
} Organization: Smurfit Stone Container Corp
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Embedding polymer films
}
} Question: Is there a method to enhance polymer film bonding to a
} Poly/Bed 812 embedding medium. Frequently the thin films release
} from the embedding medium during microtoming.

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 08:46:10 2004

Contents Retrieved from Microscopy Listserver Archives
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The Kodak DCS 5xx/6xx/7xx series cameras(and their Canon twins
D2000/D6000)
had either an Anti-Aliasing filter or an Infrared Blocking Filter mounted
in front of the mirror.
Currently all of the manufacturers, including Kodak, mount these
filters directly on
top of the image sensor behind the mirror. Except for lenses or devices
that require "mirror lockup",
you should have few mounting issues with current models.
"Professional" level digital SLR cameras such as the Nikon D1x/h,
D2h, Canon
EOS-1D and EOS-1DS will provide almost complete functionality when mounted
to a microscope.
Some of the lower level cameras such as the Nikon D100/D70, and Fuji S2 Pro
will only provide
limited functionality if they are not mounted with an AF lens.
Kodak, Fuji, and Canon include software with their cameras that
will run them while tethered
to a computer. Nikon offers their Capture software as an option.
Another consideration when replacing a 35mm body with a digital SLR
is that the sensor
in most digital SLR cameras is smaller than the 35mm frame. Currently the
Canon EOS-1DS,
and the Kodak DCS Pro SLR/n(Nikon mount) and Pro SLR/c (Canon EF mount) are
the only
"full frame" digital SLR cameras available. For the non full frame cameras
a change in the camera
mount optics will generally correct the magnification mismatch.

George

George Laing
National Graphic Supply
ph 800.223.7130 x3109
f 800.832.2205
email scisales-at-ngscorp.com

} The ONLY exceptions are: Autofocus features obviously will not work with
non- autofocus lenses (i.e. microscopes), and some extreme lenses project
back
} into the camera body signifcantly far. The digital cameras often have an
IR
} filter in front of the SLR mirror which may interfere with some lenses.
The
} filters are removeable on some Digitals but not all. (Which lenses?
Extremes:
} 8mm Fisheye mostly, my camera lists a couple odd 20mm and one odd
} 45mm, but I've never seen anything in a microscope mount which projects
} past the mounting flange itself.)
}
} Perhaps someone else has some thing else to add?

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 11:03:59 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Gary;
I think you have been mislead about the type of sensors on high
end cameras. The Cannon high end cameras like the 1Ds (11MP), the D10
and D60 (6MP), the Digital Rebel(6MP), and the old D30(3MP) all used
CMOS sensors. Only the 1D (4MP) which was intended for high repletion
rate shooting used CCD's. Also the Kodak DCS 14 series (14MP) all use
CMOS sensors. Nikon and Fuji, on the other hand, have used primarily
CCD's.
Also, for TTL flash, these digital bodies all use through the
lens TTL. No, the light does not bounce of the film-it bounces off the
CCD that is right where the film would be if it was not digital. You can
read more at
http://www.dpreview.com.

John Mardinly
Intel

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Wednesday, March 24, 2004 5:10 PM
To: Beth Richardson
Cc: MSA listserver

There are several options for this sort of work.

If the past tasks were performed using 35mm film SLR,
a digital SLR may be a viable option. Keep in mind
that the high end digital SLRs use CCDs. The low end,
but not necessarily high quality, ones use CMOS sensors.
Nikon only uses CCDs. Regardless, the magnification
factor is 1.5 rather than 1:1. Thus, a 100mm macro lens
is actually 150mm. This may matter to him or not. Nikon
makes 60mm/105mm/200mm Micro-Nikkor lenses. Each one
has their own idiosyncrasies. Not bad, just different.
But all work with Nikon macro flash. Sort of.

That said, the digital bodies do not do TTL flash.
It is all manual. If using flash, one must get an
SB-80 regular flash or SB-29s macro in order to be
able to manually adjust the amount of flash. Film
SLRs will do TTL off of the film. Digital SLRs don't
do this. Fill flash is terrible. If the lighting is
solid halogen or other continuous source, not much
problem.

For Nikon mount, my personal and collective experience
puts Sigma at the bottom. Up from that is Fovea, D100,
then D1h, D2h and finally D1x. I do not personally consider
Kodak SLRs to be industrial strength. D1x in RAW mode
will do 10.5M pixels.

When I go on assignment, I take two D1x bodies, five
512MB Lexar USB CF modules, notebook computer and one
N-90s body. I will return with saleable pictures.

If a prosumer camera like CP990/995 or CP 5000 will
work, then clearly, chromatic aberration, spherical
aberration and non-flat field issues do not exist.
Go for the cheap prosumer digicam. A cheap $375
adapter will do the mating. Caveat emptor. The
other serious options are twice as costly. Even so,
they may not be viable in his environmental situation.

gary g.

At 07:02 AM 3/24/2004, you wrote:

} Hi all,
} I need some advice.
} A professor in my dept. would like to "go digital". For many years he
} has been using a Nikon 35mm camera, bellows, and an AIS lens to shoot
} photographs of small seeds (about 0.5 mm). He's been working in Costa
} Rica and Ecuador so I haven't actually seen the set-up. His description
} of it makes it sound similar to a slide copier set-up rather than a
} copy stand.
} Anyway, my solution would be to use a Nikon Coolpix 990/995/or 4500
} camera coupled to a dissecting scope.
} Any other suggestions are greatly appreciated...he's writing a grant
} and wants this info by tomorrow...of course! ;-)
} thanks,
} Beth
} **********************************************************************
} Beth Richardson
} EM Lab Coordinator
} Plant Biology Department
} University of Georgia
} Athens, GA 30602-7271
}
} Phone - (706) 542-1790 & FAX - (706) 542-1805
}
} "Between the two evils,
} I always pick the one I never tried before". Mae West (1893-1980)
} *******************************************************************
}
} "And it's only the giving that makes you what you are".
} Wond'ring Aloud, Jethro Tull (Aqualung)
}
} ***********************************************************************
* ***
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 11:26:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I don't consider Canon or Kodak as high end cameras. Not
only do I hate the Canon bodies but I dislike Kodak's
implementation overall. Kodak DCS bodies are notorious
for failing. CMOS imagers are cheap. This
makes them popular. However, they are noisy and bin
saturate very quickly. Nikon has stuck with CCDs throughout.
Many folks will argue the attributes and disadvantages
of each model and each sensor. I know from use that
the Nikon CCD systems work best for all of the types of
shooting I do with them. There are lots of choices.

People coming from Canon film background tend to stick
with Canon digicams. Likewise for Nikon film bodies
and lenses. So what happens is that whatever lens
legacy the user has, this dictates their digicam. Then,
they praise its attributes...right or wrongly.

The D1x is supposed to have matrix TTL flash. It does,
but does not work worth a hoot. Even with the new SB80
and SB50DX flash, fill flash must be done in manual mode. Same
for macro. The SB29s macro flash has a manual adjustment
of amount of light output. This has to be used to get
proper exposure. I have yet to get true TTL fill flash
to work with either of my D1x bodies. When the shots are
done correctly, the results are stunning.

gary g.

At 09:24 AM 3/25/2004, you wrote:
} Gary;
} I think you have been mislead about the type of sensors on high
} end cameras. The Cannon high end cameras like the 1Ds (11MP), the D10
} and D60 (6MP), the Digital Rebel(6MP), and the old D30(3MP) all used
} CMOS sensors. Only the 1D (4MP) which was intended for high repletion
} rate shooting used CCD's. Also the Kodak DCS 14 series (14MP) all use
} CMOS sensors. Nikon and Fuji, on the other hand, have used primarily
} CCD's.
} Also, for TTL flash, these digital bodies all use through the
} lens TTL. No, the light does not bounce of the film-it bounces off the
} CCD that is right where the film would be if it was not digital. You can
} read more at
} http://www.dpreview.com.
}
} John Mardinly
} Intel
}
} -----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
} Sent: Wednesday, March 24, 2004 5:10 PM
} To: Beth Richardson
} Cc: MSA listserver
} Subject: [Microscopy] Re: camera set-up
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 14:44:33 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I just wanted to thank everyone for their suggestions and information
on a digital camera set-up. This is a great listserv!

again, thank you!
Beth
**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 15:10:57 2004

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I am trying to deliver light for fluorescence to a Zeiss Axiovert 200 via a
SMA fiber optic. The Zeiss lamps connect to the microscope with a dovetail
that is ~53 mm in diam. Is there some sort of adapter or connector I can
use. Any ideas? Thanks!

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 15:46:02 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Steve Slap wrote:
===============================================================
Phil Swab teaches a technique at the RMC/Boeckeler materials microtomy
workshops which involves adding Z-6040 silane (g-
glycidoxypropyltrimethoxysilane), an epoxy primer, to a Spurrs resin
mixture to enhance adhesion. I haven't tried it with Poly/Bed 812, but it
works wonders with thin film coatings in Spurrs.
=================================================================
Steve is right, this is an excellent way to enhance adhesion. Our SPI-Chem
brand of this same material is described on URL
http://www.2spi.com/catalog/chem/trimethoxysilane.shtml

It is available in small laboratory quantities for EM use. It is known also
as "3GTMO" generically. CAS#: 2530-83-8 From what we have seen, several
brands of the material, including Z-6040, work equivalently in this kind of
application. It is my understanding (if I remember correctly) that the
technique was originally designed for use with "Epon" type epoxy systems and
was later found to work also with Spurr-type formulations.

My perception is that a) more than a few people are using this material for
this application and b) one small bottle will last a long time.

Disclaimer: SPI Supplies offers this product commercially as an adhesion
promoter as described by Steve's posting.

Chuck

============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 16:45:39 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

M. McKIillip wrote:
=======================================================
Question: Is there a method to enhance polymer film bonding to a Poly/Bed
812 embedding medium. Frequently the thin films release from the embedding
medium during microtoming.
=======================================================
In an earlier posting, I think I was answering the wrong question, and I
apologize for that.

The problem with embedding polymer films is that if the embedding resin
really does "wet" the film surface (necessary for good adhesion), it will
likely start to swell the polymer film and cause artifacts in the final
images. Over the years we have developed an approach where we metallize the
film surfaces, Pt is preferred but Au will do if that is all you have
available (Pt is less soft than Au will be more resistant to smearing), and
after both sides are metallized, you then do the embedding. My perception
is that most of the commercially available "Epon subsitutes", be it our own
SPI-Pon™ 812 or others, behave in much the same way. Our experience has
been mainly with the SPI-Pon epoxy embedding resin, and generally speaking,
the interface does remain intact. But if things are not "just right", the
gold/epoxy interface will be the first to come apart. For example, if your
diamond knife is not in good shape, it is hard to keep the interface from
coming apart under any circumstances.

One other comment: If there are any surface release agents (such as from an
extrusion aid or lubricant) on the film surface, this is another reason for
poor adhesion. This problem can be "cured" by brief exposure in the a
plasma cleaner such as the SPI Plasma Prep Plasma Cleaner operating at 10
watts to remove the release agent which then will result in a greatly
improved adhesion situation.

In any case, these approaches do not require the use of 3GTMO, to which I
referred in my earlier posting.

Disclaimer: In our analytical services business, we do this kind of
sectioning for clients routinely and is the basis of our experience for
these kinds of samples.

Chuck

============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 16:47:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (gfuente-at-arqueologia.edu.ar) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, March 25, 2004 at 08:44:26
---------------------------------------------------------------------------

Email: gfuente-at-arqueologia.edu.ar
Name: Guillermo A. De La Fuente

Organization: School of Archaeology, Univ. of Catamarca, Argentina

Title-Subject: [Microscopy] [Filtered] SEM-EDAX chemical data adquisition

Question: Dear Co-Listers,

I am starting to work with SEM-EDAX analysis in archaeological
ceramics, especifically with the paintings covering the external
surface.
My question is: can I get quantitative chemical data (in % for each
element present in the area under analysis) apart from the spectras
-with the peaks of the elemenets- for each area analysed?
Thanks for your help,
Guillermo

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 16:47:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (swatkins-at-pitt.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, March 25, 2004 at 10:21:33
---------------------------------------------------------------------------

Email: swatkins-at-pitt.edu
Name: simon watkins

Organization: University of Pittsburgh

Title-Subject: [Microscopy] [Filtered] Lynx processor recipes

Question: FOlks, I am looking for a couple of things, 1: lynx
processor recipes. I know there are loads of machines out there, and
perhaps a little recipe sharing would be of common interest.
Also any critical comments on care and maintenance would also be welcome
Thanks

simon

-----------------------------------------------------------
Simon C. Watkins Ph.D. FRC Path.
Professor, Cell Biology and Physiology
Director Center for Biologic Imaging
BSTS 225
University of Pittsburgh
3500 Terrace St.
Pittsburgh PA 15261
Tel:412-648-3051
Fax:412-648-2797
URL: http://www.cbi.pitt.edu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 16:58:28 2004

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Gary;
If you don't consider a camera that costs $8,000 for just the
body to be high end, I don't know what would be. I can't vouch for your
experience, and there is no disputing that Nikons are GREAT cameras, but
independent testing organizations have found the noise in Cannon CMOS
sensors to be measurably consistently lower than in Nikon CCD sensors.
Even Nikon's new JFET (Junction Field Effect Transistor) LBCAST (Lateral
Buried Charge Accumulator and Sensing Transistor array) sensor in the
D2H, which appears to be similar to CMOS technology, shows slightly more
noise than the Cannon sensors. I follow three sites that evaluate
digital cameras and recommend them to anyone interested in digital
photography:
http://www.dpreview.com
http://www.imaging-resource.com/
http://www.steves-digicams.com/

John Mardinly

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Thursday, March 25, 2004 9:48 AM
To: Mardinly, John
Cc: MSA listserver

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 18:08:40 2004

Contents Retrieved from Microscopy Listserver Archives
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Surely it's the performance that qualifies something as 'high-end', isn't it,
not the price?

There's usually a good correlation (and I'm not saying that there isn't in
this case) but not always.

cheers

rtch

ps it's 'Canon', not 'Cannon'

} If you don't consider a camera that costs $8,000 for just the
} body to be high end, I don't know what would be. }

--
Ritchie Sims Ph D Phone : 64 9 3737599
ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu Mar 25 20:21:57 2004

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Guillermo,

The short answer is no, the beam penetration is too much influenced by variations
of topography and porosity. Beam probe methods are also too much influenced by
diagenetic changes in the paint layer (involving the loss of certain ingredients,
or the uptake of new ones from the surroundings) that are not uniform and therefore
create differences between formerly identical objects. Secondary mineral deposits
will tend to coat the original paint components, giving rise to larger differences
in surface analysis techniques.

If your purpose is to group or differentiate the ceramics and if you have a SEM
with an X-ray spectrometer and lack other types of instruments (such as X-ray
fluorescence or AA or ICP) you might consider looking at fracture sections across
the paint layer for other kinds of distinguishing features that don't require
quantification. You might find, for example, that certain minor minerals accompany
a pigment from one source but not the same pigment from another source. Making the
distinction one of trace occurrence/non-occurrence instead of a question of bulk
chemistry might work for you.

John Twilley
Art Conservation Scientist

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (gfuente-at-arqueologia.edu.ar) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Thursday, March 25, 2004 at 08:44:26
} ---------------------------------------------------------------------------
}
} Email: gfuente-at-arqueologia.edu.ar
} Name: Guillermo A. De La Fuente
}
} Organization: School of Archaeology, Univ. of Catamarca, Argentina
}
} Title-Subject: [Microscopy] [Filtered] SEM-EDAX chemical data adquisition
}
} Question: Dear Co-Listers,
}
} I am starting to work with SEM-EDAX analysis in archaeological
} ceramics, especifically with the paintings covering the external
} surface.
} My question is: can I get quantitative chemical data (in % for each
} element present in the area under analysis) apart from the spectras
} -with the peaks of the elemenets- for each area analysed?
} Thanks for your help,
} Guillermo
}
} ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 02:16:59 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

Thank you all for your help and suggestions concerning uneven
illumination in fluorescence. The liquid wave guides seem a good
solution to look at to reduce the background variation caused by the
lightsource.

The background pattern doesn't cause problems for our image analysis, as
it is based on local geometric operators which detect objects locally,
regardless of the background pattern. For spatial feature
quantification, the impact of the backgroundremains limited too.

My main concern is on quantitative densitometry, as an uneven background
wil cause different results depending on the position of the object in
the image. If the S/N ratio is high, then the error caused by a small
amount of radial/local background variation is negligable, but at the
very low range of S/N ratios the impact will become much higher.

Besides this, a large variation in background intensity also gobbles up
much of the dynamic range of the system, which diminishes the maximum
density ratio which can be quantified. Post-factum digital background
correction, may flatten the image, but at the cost of a reduced dynamic
range. So, measures to avoid the generation of an uneven background
should be the primary goal in my opinion.

Besides the lightsource there seem to be several components in the
lightpath which contribute to a variation in background intensity.
Non-plan corrected objectives, multiwell plates which act as polarisers
when placed in a lightpath which contains polarizing components.
Fluorescent probe leakage, etc. ... .

I am trying to find some literature on this topic, but up to now my
search did not succeed.

Regards,

Peter

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 04:12:48 2004

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I have seen the posting for a recipe book for use with The EMS Lynx
issue Processor. Please note that here at Electron Microscopy Sciences
we do have a complete recipe book that has been compiled by users all
over the world and for those woe quire it please do not esitate to
contact us and we shall send it to you
We look forwardto hearing from you

Stacie Kirsch
Electron Microscopy Sciences
Tel: 215-412-8400 Fax: 215-412-8450
www.emsdiasum.com

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:swatkins-at-pitt.edu]
Sent: Thursday, March 25, 2004 6:10 PM
To: Subject: [Microscopy] viaWWW: Lynx processor recipes

------------------------------------------------------------------------
------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (swatkins-at-pitt.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, March 25, 2004 at 10:21:33
------------------------------------------------------------------------
---

Email: swatkins-at-pitt.edu
Name: simon watkins

Organization: University of Pittsburgh

Title-Subject: [Microscopy] [Filtered] Lynx processor recipes

Question: FOlks, I am looking for a couple of things, 1: lynx
processor recipes. I know there are loads of machines out there, and
perhaps a little recipe sharing would be of common interest.
Also any critical comments on care and maintenance would also be welcome
Thanks

simon

-----------------------------------------------------------
Simon C. Watkins Ph.D. FRC Path.
Professor, Cell Biology and Physiology
Director Center for Biologic Imaging
BSTS 225
University of Pittsburgh
3500 Terrace St.
Pittsburgh PA 15261
Tel:412-648-3051
Fax:412-648-2797
URL: http://www.cbi.pitt.edu

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 07:08:09 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sylvain.maury-at-thalesgroup.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, March 26, 2004 at 03:48:24
---------------------------------------------------------------------------

Email: sylvain.maury-at-thalesgroup.com
Name: sylvain

Organization: intern at IXL laboratory, Talence, FRANCE(33)

Title-Subject: [Microscopy] [Filtered] high performance metallography (small grain size) for high performance SEM

Question: hello,
i'm doing a long internship on a high resolution SEM - about 1.5nm -
that permit magnification of about x800000. my problem is that Au-Pd metallization
grain size is too large and appears on the image, polluding it. same problem for polishing
micro-scratches on micro-cut samples. i'm currently searching
for new sample preparation methods for finer polishing or new kind of metallography.

please someone gives me some information on how to make a metal layer as fine as possible,
and innovations on this subject.
thanx for your answers and helping.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 08:09:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Sylvain, have you considered using electropolishing
methods on metallographic samples? This is the same
principle used in preparing many metal TEM samples,
and gives a superior finish using non-abrasive
methods.

If you decide to stick with abrasive methods, I find
the best final polish is obtained with a fine
colloidal suspension such as Buehler's Linde B or
Struer's AP aluminum oxide suspension and a vibratory
polisher.

Stu Smalinskas
Sr. Metallurgist
SKF
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Sylvain wrote:

Question: hello,
i'm doing a long internship on a high resolution SEM -
about 1.5nm -
that permit magnification of about x800000. my problem
is that Au-Pd metallization
grain size is too large and appears on the image,
polluding it. same problem for polishing
micro-scratches on micro-cut samples. i'm currently
searching
for new sample preparation methods for finer polishing
or new kind of metallography.

please someone gives me some information on how to
make a metal layer as fine as possible,
and innovations on this subject.
thanx for your answers and helping.

Email: sylvain.maury-at-thalesgroup.com
Name: sylvain

Organization: intern at IXL laboratory, Talence, FRANCE(33)

__________________________________
Do you Yahoo!?
Yahoo! Finance Tax Center - File online. File on time.
http://taxes.yahoo.com/filing.html

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 10:45:28 2004

Contents Retrieved from Microscopy Listserver Archives
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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Sylvain Maury wrote:
=========================================================
i'm doing a long internship on a high resolution SEM - about 1.5nm -
that permit magnification of about x800000. my problem is that Au-Pd
metallization
grain size is too large and appears on the image, polluding it. same problem
for polishing
micro-scratches on micro-cut samples. i'm currently searching
for new sample preparation methods for finer polishing or new kind of
metallography.

please someone gives me some information on how to make a metal layer as
fine as possible, and innovations on this subject.
thanx for your answers and helping.
---------------------------------------------------------------------------
My coments address only the need for a finer metal coating.

I can refer you to the OPC line of osmium plasma coaters as described on
URL
http://www.2spi.com/catalog/osmi-coat.html

This is not a sputtering process but is done by PVD (physical vapor
deposition). The deposition, instead of nucleating at "active sites" and
then growing as "islands" until they impinge (to be conductive), but also
growing vertically as well, with the OPC system, is on an atomic scale which
results in a zero grain size because the layer seems to be amorphous without
any structure whatsoever (or at least none that anyone has been able to
detect).

If you have an important sample and would like to have us do a
(complimentary) test coating, contact me off-line and we can set up a demo.

Disclaimer: SPI Supplies distributes the OPC line of osmium plasma coaters.

Chuck

============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 11:59:21 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Sylvain,
If you are looking at metals then why coat at all? You should be able to examine
the sample uncoated. Are you looking at grains? as polished? or slightly etched?
If you are looking at ceramics or other non-conductors, then a very thin
chromium coat or an ion-beam deposited coat of iridium or other coat
specifically made for high-resolution SEMs is recommended. The Au/Pd sputter
coat is not suitable for high resolution, although it provides a useful aid to
astigmatism correction. I have also had good success looking at ceramic grains
by TEM. You can just dimple the sample to perforation, since they don't suffer
damage or dislocation formation.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "by way of MicroscopyListserver" {sylvain.maury-at-thalesgroup.com}
To: {microscopy-at-ns.microscopy.com}
Sent: Friday, March 26, 2004 5:29 AM

Does anyone know of a Linux driver for Nikon DXM 1200?
Thanks!

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370
fax +54 11 4982-4494

From MicroscopyL-request-at-ns.microscopy.com Fri Mar 26 14:02:03 2004

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Dear Colleagues,
We have a JEOL JSM-6300V SEM available to donate, cost of shipping not
included. If interested, you may contact me off-list.
Audrey

Audrey Hubbell
Electron Microscopy Scientist
Anatomic Pathology Department
Wyeth Research
641 Ridge Road
Chazy, NY 12921
(518) 846-6233 tel
(518) 846-6345 fax
Hubbela-at-wyeth.com

From MicroscopyL-request-at-ns.microscopy.com Sat Mar 27 12:52:00 2004

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Hiroki, grab this one!

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "Audrey Hubbell" {HubbelA-at-wyeth.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Friday, March 26, 2004 3:23 PM

I seek advice on desktop evaporative coaters. Thed need is to
produce consistent evaporated gold coatings for use in an ion
microprobe. We have to use 99.999 purity gold wire as the source.

Any specific comment or experience (good and bad) with the emitech
K950X Turbo Evaporator would be appreciated.

Thanks

Brendan
--

Brendan J. Griffin
Director & Assoc. Professor in Electron Microscopy
Centre for Microscopy and Microanalysis (M010)
Director Western Australian Centre for Microscopy
Associate Director NANO-MNRF
President Australian Microbeam Analysis Society
The University of Western Australia
First floor, Physics Building,
35 Stirling Highway
CRAWLEY, WA, AUSTRALIA 6009
ph 61-8-6488-2739 fax 6488-1087
mobile 0409-104-096
bjg-at-cmm.uwa.edu.au
http://cmm.uwa.edu.au/

CRICOS Provider No. 00126G

From MicroscopyL-request-at-ns.microscopy.com Sun Mar 28 10:49:20 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (aa16678-at-isa.utl.pt) from http://216.239.39.104/translate_c?hl=pt&u=http://www.msa.microscopy.org/Ask-A-Microscopist.html&prev=/search%3Fq%3Dmicroscopy.com%26hl%3Dpt%26lr%3D%26ie%3DUTF-8%26oe%3DUTF-8 on Sunday, March 28, 2004 at 09:42:18
---------------------------------------------------------------------------

Email: aa16678-at-isa.utl.pt
Name: andreia

Organization: isa

Education: Undergraduate College

Location: City,

Question: what s the genome dimension of : s.cerevisae, a.thaliana, d.melanogaster, h.sapiens, e.elegans?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Mar 28 11:08:42 2004

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My apologies, listers! Wrong button...

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "Vitaly Feingold" {vitalylazar-at-worldnet.att.net}
To: "Audrey Hubbell" {HubbelA-at-wyeth.com} ; {Microscopy-at-msa.microscopy.com}
Sent: Saturday, March 27, 2004 2:13 PM

}
}
} Does anyone know how to accomplish a batch export of images from Autobeam in
} ISIS? I have 3000 odd images that need to be exported for processing on
} software that was written inhouse. Currently I have to open each image
} individually in Autobeam and then type/copy in a filename to export as tif.
}

We have used a shareware macro program called Macro Magic to export the
ISIS images. This program is basically a keystroke/mouse action
recorder. Currently, we use a visual basic routine that is more useful
in naming the files and performing other actions on the images that we
need for export to our software. In both cases, you will probably still
need to open each separate job that contains the images. We often
collect several hundred images on a single job, so the macro is
essential for getting the images out of ISIS for further analysis.

Good luck.

--
Larry D. Hanke, P.E.
Materials Evaluation and Engineering, Inc.
Practical Solutions Through Technology and Innovation
http://www.mee-inc.com (763) 449-8870

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 07:15:17 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (akoorts-at-medic.up.ac.za) from http://www.msa.microscopy.org/Ask-A-Microscopist.html#form on Monday, March 29, 2004 at 02:27:15
---------------------------------------------------------------------------

Email: akoorts-at-medic.up.ac.za
Name: Alida Koorts

Organization: University of Pretoria

Education: Graduate College

Location: Pretoria, Gauteng, South Africa

Question: I am at the moment doing immunolocalization and
in situ hybridization for TEM with gold markers.
I stain with uranyl acetate. Is it possible for
the uranyl acetate solution (pH 4.5) to remove
some of the antibodies/probes? If so what can be
done to prevent this?
Yours sincerely
Alida

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 07:49:57 2004

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Dear Alida,
A low pH may indeed have an interfering effect on antigen-antibody
interaction.
You can prevent this by including a glutaraldehyde postfixation step
(2% glutaraldehyde in PBS for 15 minutes) in your protocol prior to
water washes and contrasting with uranyl acetate.
Regards,
Peter

Monday, March 29, 2004, at 03:40 PM, by way of Ask-A-Microscopist
wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (akoorts-at-medic.up.ac.za) from
} http://www.msa.microscopy.org/Ask-A-Microscopist.html#form on Monday,
} March 29, 2004 at 02:27:15
} -----------------------------------------------------------------------
} ----
}
} Email: akoorts-at-medic.up.ac.za
} Name: Alida Koorts
}
} Organization: University of Pretoria
}
} Education: Graduate College
}
} Location: Pretoria, Gauteng, South Africa
}
} Question: I am at the moment doing immunolocalization and
} in situ hybridization for TEM with gold markers.
} I stain with uranyl acetate. Is it possible for
} the uranyl acetate solution (pH 4.5) to remove
} some of the antibodies/probes? If so what can be
} done to prevent this?
} Yours sincerely
} Alida
}
} -----------------------------------------------------------------------
} ----
}
}
}
-----------
Peter van de Plas
Aurion
Costerweg 5
6702 AA Wageningen
The Netherlands
Phone: +31 317 497676
Fax: +31 317 415955

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 08:11:52 2004

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I am seeking input from other university labs. Our lab is subsidized
through university general funds. However, due to the State of Michigan
budget crisis, our subsidy has been decreasing for the past three
years. Meanwhile our number of users has doubled and new equipment has
been added that requires support. It seems our users are doing better
than ever in writing grants that receive funding. However, there is no
formula or mechanism to direct any of the substantial overhead from these
grants to our lab or to the PIs on the grant. The only alternative is to
increase our user rates to well above average.

At some universities there is a mechanism to direct a portion of grant
overhead to the microscopy facility. Would any of you be willing to share
the formula or mechanism in use at your university? I think this topic may
be of great interest to many others.

Stanley L. Flegler, Director
Center for Advanced Microscopy
Michigan State University

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 08:41:44 2004

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Hi Alida,

In all my immuno-EM labeling (usually on cryo-sections
but also sometimes on plastic sections), I always fix the
sections in 1% glutaraldehyde (in PBS - 5 min) after the
final washes that follow the protein A-gold labeling step.
I then rinse the sections extensively with water (because
phosphate will make UA precipitate), usually 5 times 2-3
minutes each, then stain my sections with uranyl acetate
and air-dry them or embed them in methyl cellulose/UA.

To answer your question, I think antibody and gold complexes
can withstand a few quick washes in water and incubation in
UA, but I am sure some of it is falling off. With the fixation step
that I describe above, you maximize labeling efficiency and
avoid taking chances. It's always better being safe!

Best wishes

Marc

On Monday, March 29, 2004, at 08:40 AM, by way of Ask-A-Microscopist
wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (akoorts-at-medic.up.ac.za) from
} http://www.msa.microscopy.org/Ask-A-Microscopist.html#form on Monday,
} March 29, 2004 at 02:27:15
} -----------------------------------------------------------------------
} ----
}
} Email: akoorts-at-medic.up.ac.za
} Name: Alida Koorts
}
} Organization: University of Pretoria
}
} Education: Graduate College
}
} Location: Pretoria, Gauteng, South Africa
}
} Question: I am at the moment doing immunolocalization and
} in situ hybridization for TEM with gold markers.
} I stain with uranyl acetate. Is it possible for
} the uranyl acetate solution (pH 4.5) to remove
} some of the antibodies/probes? If so what can be
} done to prevent this?
} Yours sincerely
} Alida
}
} -----------------------------------------------------------------------
} ----
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 13:14:41 2004

Contents Retrieved from Microscopy Listserver Archives
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Could you tell me if there is such a thing as a Light microscopy system
that will project high quality images at high magnification that will
also transmit to the web? I welcome all comments.
Thank you,
Sue

--
Sue Tyler
Biologist
Cooperative Oxford Laboratory
Center for Coastal Environmental Health&
Biomolecular Research at Charleston ( CCHEBR)
USDOC/NOAA/NOS/NCCOS
904 S. Morris St.
Oxford, Maryland 21654-9724
410-226-5193 Fax: 410- 226-5925
Sue.Tyler-at-noaa.gov

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 15:06:02 2004

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Dear Alida,

A few years ago, the acidic uranyl acetate step as a possible source
for reduced immunodetection was subject of a vibrant and cheerful
discussion on this list. I still have fond memories of that one....
What about you, Paul? ;-)

To keep it brief: acidic conditions may uncouple the antibody/antigen
complex, and this is more likely to happen when the acidic environment
is chaotropic. Such conditions are put to good use in eluting bound
antibodies from affinity columns for antibody purification. If this
should happen on specimens it should be easily prevented using a
glutaraldehyde step after the wash steps following the secondary gold
reagent. In this way antibodies and gold reagents will become
covalently linked to the specimen.

for example:
.......
ImmunoGold Step
wash with incubation buffer
wash with PBS
fix with 2-2.5% of Glutaraldehyde in 0.1M Phosphate Buffer for 5-10
minutes
wash with PBS
distilled water
etc....

Hope this helps,

Jan Leunissen
--------------------
Aurion - President
Immunogold Reagents
Costerweg 5
6702 A Wageningen
The Netherlands
phone 31-317-497676
fax 31-317-415955
http://www.aurion.nl
Present Address:
EM-Unit
Otago School of Medicine
Dunedin, New Zealand
phone 64-3-4797109
http://ocem.otago.ac.nz/

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 21:48:11 2004

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Hi all,

I am researching sputter coaters for HR FESEM imaging. I would
appreciate hearing from users about their experiences with specific coater
makes and models. Ion beam is out of my price range so I am looking at
magnetron type coaters. Please no venders this round.

A couple of specific questions that I would like input on:
Value of cooled magnetron sputter head (specifically peltier cooling) vs.
non-cooled
Merits of getting a diaphragm pump rather than standard rotary pump to back
turbopump
Thickness monitor: how useful and how well do they work.
Reliability...

Also I have heard of the problems with Cr oxidizing and Ir is quite
expensive. What other metal do you like using that balances the desired
small grain with reasonable stability, performance, and cost.

Thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Mar 29 21:59:07 2004

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Email: pwebster-at-hei.org
Name: Paul Webster

Organization: House Ear Insitute

Title-Subject: [Microscopy] Re: AskAMicroscopist:immunolocalization and in situ hybridization for TEM

Question: Hi Jan,

How is New Zealand?

I have been watching this thread with interest and remember well our last disccusions. The technical problems with the listserver have kept me from replying. Getting lots of "away from the desk" messages when I contribute puts me off writing too.

I agree with everyone that low pH should in theory have the effect of stripping antibody or protein A from sections. So in theory, it would be wise to fix the labeled sections with a cross-linking agent, such as glutaraldehyde, before final contrasting in low pH uranyl acetate.

However, the situation remains the same as when we first discussed this issue. There are no published data to support the theory. We left the discussion last time with your comment that adding the final 10 min fixation step does no harm, so just do it. I agree with this.

This still leaves the issue unresolved. I can label cryosections or Lowicryl sections with antibodies and protein A gold but cannot differentiate (subjectively) from the levels of labeling on sections treated with glutaraldehyde with those that were not. This means that treating the sections with glutaraldehyde may not have such a drastic effect on labeling as theory suggests.

The field is open to anyone who wants to compare labeling efficiency on aldehyde-fixed, labeled sections with unfixed sections. It seems to be an easy experiment to do and is worthy of publication.

Paul Webster.

House Ear Institute
2100 W 3rd St
Los Angeles, CA 90057.

----------
} From: Jan Leunissen
Sent: Monday, March 29, 2004 1:30 PM
To: microscopy-at-msa.microscopy.com
Cc: akoorts-at-medic.up.ac.za

Dear Alida,

A few years ago, the acidic uranyl acetate step as a possible source
for reduced immunodetection was subject of a vibrant and cheerful
discussion on this list. I still have fond memories of that one....
What about you, Paul? ;-)

To keep it brief: acidic conditions may uncouple the antibody/antigen
complex, and this is more likely to happen when the acidic environment
is chaotropic. Such conditions are put to good use in eluting bound
antibodies from affinity columns for antibody purification. If this
should happen on specimens it should be easily prevented using a
glutaraldehyde step after the wash steps following the secondary gold
reagent. In this way antibodies and gold reagents will become
covalently linked to the specimen.

for example:
.....
ImmunoGold Step
wash with incubation buffer
wash with PBS
fix with 2-2.5% of Glutaraldehyde in 0.1M Phosphate Buffer for 5-10
minutes
wash with PBS
distilled water
etc....

Hope this helps,

Jan Leunissen
--------------------
Aurion - President
Immunogold Reagents
Costerweg 5
6702 A Wageningen
The Netherlands
phone 31-317-497676
fax 31-317-415955
http://www.aurion.nl
Present Address:
EM-Unit
Otago School of Medicine
Dunedin, New Zealand
phone 64-3-4797109
http://ocem.otago.ac.nz/

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 05:21:17 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Sue Tyler wrote:-

} Could you tell me if there is such a thing as a Light microscopy system
} that will project high quality images at high magnification that will
} also transmit to the web? I welcome all comments.
} Thank you,
} Sue

Sue

This is not going to be much use, but it may be better than nothing.

First, is this moving pictures you are after?

If you want to projection display a live slide in motion, and
simultaneously stream live MPEG video over the Net, the mind boggles.

It gets technically easier with a live slide if you view on a colour
TV monitor the same feed that is going to the Net. At the simplest,
buy a webcam, yank the lens out, and your microscope eyepiece,
assuming you can find an old 160mm tube length mono mic in the store
cupboard, and form the objective image direct on the webcam sensor,
and feed the webcam output out via Netmeeting or similar.

The next step up is a good quality C mount security type colour video
camera, with no lens, installed by someone who knows microscopes,
electronics and computers. I am down near Melbourne, Australia so that
lets me out.

If you have Government-style funding just throw money at a
consultant.

If you are basically after still images which can be then sent out as
JPG files on the Net there are a lot more options. I have spent the
last three years looking at producing nice images at up to 40X, which
may not fit your definition of high power. I have done the lot for
less than $500 plus a lot of home engineering. Success has been
embarrassing, in that results are so clear and sharp that the
shortcomings of my modest 160mm objectives are now painfully obvious,
and I have had to go shopping on Ebay.

All my stuff is written up on a browser-readable CD, and covers
removing lenses from fixed-lens digital cameras, which is a
prerequisite. It might be worth scanning through for 'background'. I
can't send it for nothing, because everyone will want one, but
covering postal charges is fine. It's all work for me, so don't take
one to be polite.

Please clarify your problem if I haven't helped at all

Breck

Breck Bowles Development, Pakenham, Australia
breck-at-jeack.com.au

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 07:18:24 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Breck Bowles writes ...

} Sue Tyler wrote:-
}
} } Could you tell me if there is such a thing as a LM system
} } that will project high quality images at high magnification
} } that will also transmit to the web? I welcome all comments.

} It gets technically easier with a live slide if you view on a colour
} TV monitor the same feed that is going to the Net. At the simplest,
} buy a webcam, yank the lens out, and your microscope eyepiece,
} assuming you can find an old ...

It seems to me you could employ a Nikon Coolpix setup. That is, the CP99x
series and I believe the CP5000 provide for NTSC (and PAL) TV output. This
video signal could then go into a video input as provided by many video
input cards. Forgive me if I don't have the time to research current
possibilities and manufacturers' model numbers, but the possibility has
existed for some time.

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 07:27:42 2004

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Debby,
We have a FEG-SEM and about three years ago we purchased a Cressington 208HR
sputter coater with the MTM-20 Thickness Monitor. The unit cost almost
$25,000 Cdn. We have used both Cr and Pt/Pd targets. The Cr target is 57 mm
diameter x 3.2 mm thick and should last a considerable length of time.
Oxidation of the Cr is one drawback as the sample chamber is not maintained
under vacuum once the coater is powered off. This becomes a problem at the
start of each coating cycle as it takes several minutes of operation before
Cr and not Cr oxide is being discharged from the target. Coating with Pt/Pd
is a much faster operation. Unfortunately the targets are also consummed
much faster. Typically our Pt/Pd targets last 2 to 4 months and we do not
consider our usage to be heavy. The targets are 57 mm diameter x 0.1 mm
thick. The unit's power is concentrated in a central ring of about 20 mm.
and when the targets fail a small crescent-shaped hole remains where the
Pt/Pd has been etched away. I have recently made some measurements of the
actual amount of Pt/Pd consummed when the target fails and it is a paltry 8
to 12%! When you spend $473.00 U.S. per Pt/Pd target and less than $60.00
worth is actually consummed before the target fails you can see that it is
neither an efficient use of Pt/Pd nor your money.

The thickness monitor works well and occasionally requires a replacement
quartz crystal.

Feel free to contact me if you have any further questions.

Regards,
Paul

Paul J. Gerroir
Microscopy
Materials Characterization
Xerox Research Centre of Canada
2660 Speakman Drive
Mississauga, Ontario L5K 2L1

Phone: 905-823-7091, ext.216
FAX: 905-822-7022
e-mail: paul.gerroir-at-crt.xerox.com

-----Original Message-----
} From: Debby Sherman [mailto:dsherman-at-purdue.edu]
Sent: Monday, March 29, 2004 11:13 PM
To: message to: MSA list

Actually, it doesn't sound that complicated to me.

Assuming that you have a microscope.
First, get a camera, C-mount and software that let's you stream images to
the net.
Second, get a PC and an LCD projector, connect to the camera and project the
images.
Done.

I am not sure what was meant by "will project high quality images at high
magnification". The first probably indicates a high-resolution camera, the
second a high quality microscope??

Anyway, we can offer you a solution to this problem. Please contact me
offline for more information.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Breck Bowles [mailto:breck-at-jeack.com.au]
Sent: Tuesday, March 30, 2004 14:54
To: Microscopy-at-MSA.Microscopy.com

Sue Tyler wrote:-

} Could you tell me if there is such a thing as a Light microscopy system
} that will project high quality images at high magnification that will
} also transmit to the web? I welcome all comments.
} Thank you,
} Sue

Sue

This is not going to be much use, but it may be better than nothing.

First, is this moving pictures you are after?

If you want to projection display a live slide in motion, and
simultaneously stream live MPEG video over the Net, the mind boggles.

It gets technically easier with a live slide if you view on a colour
TV monitor the same feed that is going to the Net. At the simplest,
buy a webcam, yank the lens out, and your microscope eyepiece,
assuming you can find an old 160mm tube length mono mic in the store
cupboard, and form the objective image direct on the webcam sensor,
and feed the webcam output out via Netmeeting or similar.

The next step up is a good quality C mount security type colour video
camera, with no lens, installed by someone who knows microscopes,
electronics and computers. I am down near Melbourne, Australia so that
lets me out.

If you have Government-style funding just throw money at a
consultant.

If you are basically after still images which can be then sent out as
JPG files on the Net there are a lot more options. I have spent the
last three years looking at producing nice images at up to 40X, which
may not fit your definition of high power. I have done the lot for
less than $500 plus a lot of home engineering. Success has been
embarrassing, in that results are so clear and sharp that the
shortcomings of my modest 160mm objectives are now painfully obvious,
and I have had to go shopping on Ebay.

All my stuff is written up on a browser-readable CD, and covers
removing lenses from fixed-lens digital cameras, which is a
prerequisite. It might be worth scanning through for 'background'. I
can't send it for nothing, because everyone will want one, but
covering postal charges is fine. It's all work for me, so don't take
one to be polite.

Please clarify your problem if I haven't helped at all

Breck

Breck Bowles Development, Pakenham, Australia
breck-at-jeack.com.au

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 08:14:52 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

if you use the TV output (video signal) you will lose the
high resolution possibility of the Nikon camera. The video signal
will be at standard video resolution which will not be more
than around 750x540. Why don't you use a higher resolution
C-mount camera which allows you to store the
images on your computer. You could then add jpg/bmp/tif to
the web as well as .avi (sequence) files.

Another possibility would be to connect a camcorder to the
C-Mount adapter of a microscope. This allows you to capture
sequences and films as well. If you want to know more about how
to connect a camcorder and how to capture these images, send
me an email to my email address below.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

ms} ------------------------------------------------------------------------------
ms} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
ms} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
ms} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
ms} -------------------------------------------------------------------------------

ms} Breck Bowles writes ...

} } Sue Tyler wrote:-
} }
} } } Could you tell me if there is such a thing as a LM system
} } } that will project high quality images at high magnification
} } } that will also transmit to the web? I welcome all comments.

} } It gets technically easier with a live slide if you view on a colour
} } TV monitor the same feed that is going to the Net. At the simplest,
} } buy a webcam, yank the lens out, and your microscope eyepiece,
} } assuming you can find an old ...

ms} It seems to me you could employ a Nikon Coolpix setup. That is, the CP99x
ms} series and I believe the CP5000 provide for NTSC (and PAL) TV output. This
ms} video signal could then go into a video input as provided by many video
ms} input cards. Forgive me if I don't have the time to research current
ms} possibilities and manufacturers' model numbers, but the possibility has
ms} existed for some time.

ms} hth & cheerios ... shAf :o)
ms} Avalon Peninsula, Newfoundland
ms} www.micro-investigations.com

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 08:50:01 2004

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Does STEM (scanning transmission electron microscopy) give
better resolution than the best FE SEMs?

Dave

On Tue, 30 Mar 2004 10:13:01 -0330 michael shaffer
{michael-at-shaffer.net} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Breck Bowles writes ...
}
} } Sue Tyler wrote:-
} }
} } } Could you tell me if there is such a thing as a LM system
} } } that will project high quality images at high magnification
} } } that will also transmit to the web? I welcome all comments.
}
} } It gets technically easier with a live slide if you view on a colour
} } TV monitor the same feed that is going to the Net. At the simplest,
} } buy a webcam, yank the lens out, and your microscope eyepiece,
} } assuming you can find an old ...
}
} It seems to me you could employ a Nikon Coolpix setup. That is, the CP99x
} series and I believe the CP5000 provide for NTSC (and PAL) TV output. This
} video signal could then go into a video input as provided by many video
} input cards. Forgive me if I don't have the time to research current
} possibilities and manufacturers' model numbers, but the possibility has
} existed for some time.
}
} hth & cheerios ... shAf :o)
} Avalon Peninsula, Newfoundland
} www.micro-investigations.com
}
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 09:57:29 2004

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David,

Yes.

With a thin TEM specimen the excitation volume is
negligible for a STEM image. The present 'Industry
Standard' for high resolution HAADF (high angle annular
dark field) STEM is Si dumbbells at 0.136nm.

With Cs correction probes of around 0.1nm can be
obtained in these instruments.

Of course HAADF imaging is not the same as secondary
imaging used on an SEM and the secondary signal from a thin
specimen would be low but in terms of resolution STEM
instruments are better.

There are (at least) two sites in UK (SuperStem at
Daresbury and Dept. Materials at Oxford) as well as others
around the world who can achieve this performance.

Ron

On Tue, 30 Mar 2004 16:15:33 +0100 (GMT Daylight Time)
"Patton, David" {David.Patton-at-uwe.ac.uk} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Does STEM (scanning transmission electron microscopy) give
} better resolution than the best FE SEMs?
}
} Dave
}
} On Tue, 30 Mar 2004 10:13:01 -0330 michael shaffer
} {michael-at-shaffer.net} wrote:
}
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } Breck Bowles writes ...
} }
} } } Sue Tyler wrote:-
} } }
} } } } Could you tell me if there is such a thing as a LM system
} } } } that will project high quality images at high magnification
} } } } that will also transmit to the web? I welcome all comments.
} }
} } } It gets technically easier with a live slide if you view on a colour
} } } TV monitor the same feed that is going to the Net. At the simplest,
} } } buy a webcam, yank the lens out, and your microscope eyepiece,
} } } assuming you can find an old ...
} }
} } It seems to me you could employ a Nikon Coolpix setup. That is, the CP99x
} } series and I believe the CP5000 provide for NTSC (and PAL) TV output. This
} } video signal could then go into a video input as provided by many video
} } input cards. Forgive me if I don't have the time to research current
} } possibilities and manufacturers' model numbers, but the possibility has
} } existed for some time.
} }
} } hth & cheerios ... shAf :o)
} } Avalon Peninsula, Newfoundland
} } www.micro-investigations.com
} }
} }
} }
} }
} }
} } This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
} }
}
} ----------------------------------------
} Patton, David
} Email: David.Patton-at-uwe.ac.uk
} "University of the West of England"
}
}
}
} This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}
}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 10:30:57 2004

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Can anyone suggest a source of #1.5 thickness coverslips with
manufactured accuracy and consistancy in thickness? I've been going
through boxes of coverslips from Corning, VWR and Clay-Adams to make
some test samples with 170 micron coverglass. A good box of Corning
has maybe 3 and 2/3 of the rest are 180 to } 200 microns. VWR has
proven to have the most consistency, but at least half are } 180.

thanks,
Glen

Glen MacDonald
Core for Communication Research
Virginia Merrill Bloedel Hearing Research Center
Box 357923
University of Washington
Seattle, WA 98195-7923 USA
(206) 616-4156
glenmac-at-u.washington.edu

************************************************************************
******
The box said "Requires Windows 95 or better", so I bought a Macintosh.
************************************************************************
******

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 10:32:43 2004

Contents Retrieved from Microscopy Listserver Archives
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We also have a Cressington 208HR and I agree with Pauls comments
below. One other thing to mention is the ability to tilt and rotate stage
and sample holders. This really helps for irregularly shaped samples. As
far as the targets are concerned is there anyone who will buy the remaining
material or take it as a trade. It really is a waste of both money and
material. Steve

Debby,
We have a FEG-SEM and about three years ago we purchased a Cressington 208HR
sputter coater with the MTM-20 Thickness Monitor. The unit cost almost
$25,000 Cdn. We have used both Cr and Pt/Pd targets. The Cr target is 57 mm
diameter x 3.2 mm thick and should last a considerable length of time.
Oxidation of the Cr is one drawback as the sample chamber is not maintained
under vacuum once the coater is powered off. This becomes a problem at the
start of each coating cycle as it takes several minutes of operation before
Cr and not Cr oxide is being discharged from the target. Coating with Pt/Pd
is a much faster operation. Unfortunately the targets are also consummed
much faster. Typically our Pt/Pd targets last 2 to 4 months and we do not
consider our usage to be heavy. The targets are 57 mm diameter x 0.1 mm
thick. The unit's power is concentrated in a central ring of about 20 mm.
and when the targets fail a small crescent-shaped hole remains where the
Pt/Pd has been etched away. I have recently made some measurements of the
actual amount of Pt/Pd consummed when the target fails and it is a paltry 8
to 12%! When you spend $473.00 U.S. per Pt/Pd target and less than $60.00
worth is actually consummed before the target fails you can see that it is
neither an efficient use of Pt/Pd nor your money.

The thickness monitor works well and occasionally requires a replacement
quartz crystal.

Stephen McCartney
Research Associate
Materials Research Institute
2108 Hahn Hall
Va Tech
Blacksburg, VA 24061
540-231-9765 - phone
540-231-8517 - FAX

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 10:57:54 2004

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Dear Paul,
I have had good results with Refining Systems Inc. of Las Vegas (phone:
702-368-0579, fax: 702-368-0933) for purchasing my precious metal supplies and
sputter coater targets. His prices are much closer to the actual precious metal
market cost. My last one cost about $200US. It depends on if you can use a
straight disc of the alloy and attach it to the coater yourself. Abe Dayani of
Refining Systems will also give you credit for your partially consumed targets,
so you can recycle them.
I have no interest, just a customer.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Gerroir, Paul J" {Paul.Gerroir-at-crt.xerox.com}
To: "Debby Sherman" {dsherman-at-purdue.edu} ; "message to: MSA list"
{microscopy-at-msa.microscopy.com}
Sent: Tuesday, March 30, 2004 5:46 AM

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 11:48:43 2004

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Indeed!

As Ron points out, high-end HAADF STEMs can achieve resolutions at, or even below, 0.1nm. Larry Allard and I had the honor (and task!) of organizing
the session on Advances in High Resolution Imaging at last year's Microscopy & Microanalysis meeting. We had several talks from STEM folks that
showed such resolutions -- check the High Resolution Imaging abstracts in last year's M&M proceedings, also the paper by Phil Batson in Nature:
Batson, P. E., Dellby, N. & Krivanek, O. L., Nature 418, 617-620 (2002).

This year's M&M meeting (in Savannah, Georgia) will also include a session on High Resolution Imaging (both STEM and TEM) organized by Larry Allard
and Jim Bentley. In addition, there will also be a pre-meeting congress on Cs-corrected electron microscopy ( for information, click on "Next TEAM
related discussions July31-August 1 2004 in Savannah" at http://ncem.lbl.gov/ ).

Mike O'Keefe

Ron Doole wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} David,
}
} Yes.
}
} With a thin TEM specimen the excitation volume is
} negligible for a STEM image. The present 'Industry
} Standard' for high resolution HAADF (high angle annular
} dark field) STEM is Si dumbbells at 0.136nm.
}
} With Cs correction probes of around 0.1nm can be
} obtained in these instruments.
}
} Of course HAADF imaging is not the same as secondary
} imaging used on an SEM and the secondary signal from a thin
} specimen would be low but in terms of resolution STEM
} instruments are better.
}
} There are (at least) two sites in UK (SuperStem at
} Daresbury and Dept. Materials at Oxford) as well as others
} around the world who can achieve this performance.
}
} Ron
}
} On Tue, 30 Mar 2004 16:15:33 +0100 (GMT Daylight Time)
} "Patton, David" {David.Patton-at-uwe.ac.uk} wrote:
}
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } Does STEM (scanning transmission electron microscopy) give
} } better resolution than the best FE SEMs?
} }
} } Dave
} }
} } On Tue, 30 Mar 2004 10:13:01 -0330 michael shaffer
} } {michael-at-shaffer.net} wrote:
} }
} } }
} } }
} } } ------------------------------------------------------------------------------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } -------------------------------------------------------------------------------
} } }
} } } Breck Bowles writes ...
} } }
} } } } Sue Tyler wrote:-
} } } }
} } } } } Could you tell me if there is such a thing as a LM system
} } } } } that will project high quality images at high magnification
} } } } } that will also transmit to the web? I welcome all comments.
} } }
} } } } It gets technically easier with a live slide if you view on a colour
} } } } TV monitor the same feed that is going to the Net. At the simplest,
} } } } buy a webcam, yank the lens out, and your microscope eyepiece,
} } } } assuming you can find an old ...
} } }
} } } It seems to me you could employ a Nikon Coolpix setup. That is, the CP99x
} } } series and I believe the CP5000 provide for NTSC (and PAL) TV output. This
} } } video signal could then go into a video input as provided by many video
} } } input cards. Forgive me if I don't have the time to research current
} } } possibilities and manufacturers' model numbers, but the possibility has
} } } existed for some time.
} } }
} } } hth & cheerios ... shAf :o)
} } } Avalon Peninsula, Newfoundland
} } } www.micro-investigations.com
} } }
} } }
} } }
} } }
} } }
} } } This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
} } }
} }
} } ----------------------------------------
} } Patton, David
} } Email: David.Patton-at-uwe.ac.uk
} } "University of the West of England"
} }
} }
} }
} } This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
} }
} }
} }
}
} ----------------------
} Mr. R.C. Doole
} Department of Materials,
} University of Oxford.
} Parks Road, Oxford. OX1 3PH. UK.
} Phone +44 (0) 1865 273701
} Fax +44 (0) 1865 283333
} ron.doole-at-materials.ox.ac.uk
} http://www-em.materials.ox.ac.uk/
} *********************************

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 13:15:22 2004

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Steve,
I have asked vendors about returning spent targets for trade/credit but
they won't do it. I have lots of AuPd around if anyone needs some. At
least if it is Au or Pd you could have some jewelry made for some special
person!

Most obvious use would be if the material was needed for thermal
evaporation in the HV coater. We have people on campus who do use some of
these metals in making thin films. Maybe I'll see if they can use it.

Debby

On 3/30/04 11:57 AM, "Stephen McCartney" {stmccart-at-vt.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} We also have a Cressington 208HR and I agree with Pauls comments
} below. One other thing to mention is the ability to tilt and rotate stage
} and sample holders. This really helps for irregularly shaped samples. As
} far as the targets are concerned is there anyone who will buy the remaining
} material or take it as a trade. It really is a waste of both money and
} material. Steve
}
}
} Debby,
} We have a FEG-SEM and about three years ago we purchased a Cressington 208HR
} sputter coater with the MTM-20 Thickness Monitor. The unit cost almost
} $25,000 Cdn. We have used both Cr and Pt/Pd targets. The Cr target is 57 mm
} diameter x 3.2 mm thick and should last a considerable length of time.
} Oxidation of the Cr is one drawback as the sample chamber is not maintained
} under vacuum once the coater is powered off. This becomes a problem at the
} start of each coating cycle as it takes several minutes of operation before
} Cr and not Cr oxide is being discharged from the target. Coating with Pt/Pd
} is a much faster operation. Unfortunately the targets are also consummed
} much faster. Typically our Pt/Pd targets last 2 to 4 months and we do not
} consider our usage to be heavy. The targets are 57 mm diameter x 0.1 mm
} thick. The unit's power is concentrated in a central ring of about 20 mm.
} and when the targets fail a small crescent-shaped hole remains where the
} Pt/Pd has been etched away. I have recently made some measurements of the
} actual amount of Pt/Pd consummed when the target fails and it is a paltry 8
} to 12%! When you spend $473.00 U.S. per Pt/Pd target and less than $60.00
} worth is actually consummed before the target fails you can see that it is
} neither an efficient use of Pt/Pd nor your money.
}
} The thickness monitor works well and occasionally requires a replacement
} quartz crystal.
}
}
} Stephen McCartney
} Research Associate
} Materials Research Institute
} 2108 Hahn Hall
} Va Tech
} Blacksburg, VA 24061
} 540-231-9765 - phone
} 540-231-8517 - FAX
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 14:50:27 2004

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A colleague of mine has a materials question for you experts out there.
Any recommendations would be helpful.
Pls respond to Mariel. TIA, ED

Hi, if you won't mind, I need your suggestions on this one. This is my
first time to encounter these kind of materials spot welded together. The
materials are gold plated nickel on stainless steel. Other co-workers of
mine already tried etching it with Kelling's reagant or 4% nital, but no
luck. They could not see any sign of fusion or heat affected zone. That's
why they decided to send the samples to me thinking that I can do it. And
since I know that you guys are all experts and I am just a novice, I am
asking your suggestions what kind of etching reagent I have to use for
etching these materials to see the heat affected zone and the fusion zone.

Thank you in advance for your help,
Best regard,
Mariel
Mariel_Lindemayer-at-gillette.com

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 17:18:09 2004

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A SEM-based STEM at 30kV can achieve subnanometer resolution (~0.8nm). This
is typically a solid state detector that integrates with an ultra-high
resolution SEM.

A dedicated STEM or TEM/STEM (200-300kV) can achieve ~0.8A resolution.

Regards,
Ed

*******************************************
Edward Principe, Ph.D.
LEO Electron Microscopy
Applications Development Scientist
principe-at-leo-usa.com
415-420-4299 (cell)
650-595-5516 (fax)
*******************************************

----- Original Message -----
} From: "Patton, David" {David.Patton-at-uwe.ac.uk}
To: "michael shaffer" {michael-at-shaffer.net}
Cc: {Microscopy-at-MSA.Microscopy.com}
Sent: Tuesday, March 30, 2004 7:15 AM

The stainless steel and the nickel may etch with Glyceregia or Aqua
Regia, depending on the the type of stainless steel and whether the
nickel is plain nickel or a nickel alloy. I am guessing that you have a
300 series stainless steel since you did not get any result with the
Kalling's Reagent. The weld should show up with glyceregia even if the
microstructure of the nickel is not well delineated. There probably will
not be much of a heat-affected zone for a spot weld in these materials.

Glyceregia is 10 ml nitric acid, 20 ml hydrochloric acid and 30 - 40 ml
glycerol. Etch by swabbing for a 20 - 30 seconds at a time until you
get a decent structure. A mixture of 1 part nitric and 1 part acetic
acid may also work well on the nickel, but may overetch the stainless
steel. Good Luck.

--
Larry D. Hanke, P.E.
Materials Evaluation and Engineering, Inc.
Practical Solutions Through Technology and Innovation
http://www.mee-inc.com (763) 449-8870

} Hi, if you won't mind, I need your suggestions on this one. This is my
} first time to encounter these kind of materials spot welded together. The
} materials are gold plated nickel on stainless steel. Other co-workers of
} mine already tried etching it with Kelling's reagant or 4% nital, but no
} luck. They could not see any sign of fusion or heat affected zone. That's
} why they decided to send the samples to me thinking that I can do it. And
} since I know that you guys are all experts and I am just a novice, I am
} asking your suggestions what kind of etching reagent I have to use for
} etching these materials to see the heat affected zone and the fusion zone.

From MicroscopyL-request-at-ns.microscopy.com Tue Mar 30 23:23:02 2004

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High quality cover slips are more difficult to
find these days. the bulk of covers are coming
from China and are garbage, IMO. They are almost
pre-cracked. Really bad quality. Several US suppliers
offer quartz covers at high prices, but for truly
important specimens, these are the way to go.

These cheap China covers under DIC or phase are
terrible. Check the source of each pack of covers
from each supplier. Try SPI, EMS, Pella, etc...the
usual "suspects." I suspect that they change sources
over time.

I got a call from Pella recently to evaluate a new
double sticky carbon tab. Nice. I'm looking forward
to doing this.

The suppliers really try to do a good job. Tell them
your concerns and needs and see if they can match up
a solution.

gary g.

t 08:53 AM 3/30/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 00:00:10 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Debby Sherman wrote:
============================================================================
=======
Steve,
I have asked vendors about returning spent targets for trade/credit but
they won't do it. I have lots of AuPd around if anyone needs some. At
least if it is Au or Pd you could have some jewelry made for some special
person!

Most obvious use would be if the material was needed for thermal
evaporation in the HV coater. We have people on campus who do use some of
these metals in making thin films. Maybe I'll see if they can use it.
============================================================================
========
I would refer anyone interested in the long established cathode recycling
program of SPI Supplies to review the details of our program on URL
http://www.2spi.com/catalog/spec_prep/metalcath-recyc.html

To summarize briefly, a 10% credit is given when the remains of the spent
cathode are returned with the new order for a replacement cathode. If you
are one who has more spent cathodes than you know what to do with, contact
me off line and I will tell you the options for taking this scrap material
off your hands and converting it into something of value to you. Precious
metals are non-renewable resources and as such, efforts should be made to
keep them in the stream of commerce to help ensure that there will be a good
supply for future generations of users.

Disclaimer: SPI Supplies is a supplier of replacement cathodes for the
leading sputter coaters, see URL
http://www.2spi.com/catalog/spec_prep/evapor_4.shtml

Chuck

============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 00:39:31 2004

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Hi Everyone

I am interested in hearing about how other labs run their departments.
What I would like to know is: the people running the EM labs, do they
rotate out to routine labs or do they stay in the EM lab.

I appreciate everyone's input.

Thanks
Helen Ilsley

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 07:26:58 2004

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Hello!

it's my second mail about this subject... you asked me to precise the
applications i'm studying : i'm working on microelectronics dies, in
failure analysis, like polished/microsectioned/metallized (Au/Pd)
components and cores ;
I often make observations of silicon or AsGa dies surface, Au/Pd
metallized or not. Actually, i work at low voltages (0.5kV-1.5KV) for
non-metallized microchips, and around 5-10kV for metallized microchips.

In this case, the problem is that the metallization grain size is too
large (8-10nm), "my" FE-SEM resolution is about 0.9-2nm, so it results
an image "pollution"at high magnifications (up to x150k-200k): grains
are now visible. i think i have to check the metallization conditions
(pressure, time, vaccum quality, etc...); it's one way. the other way is
to find new methods of metal depositon (not expensive, not too slow,
..).

Another problem : coating and polishing compents in order to study chip
microsections generates scratches now visible with the high resolution
FE-SEM. Once again, i think i have to check the polishing disks used,
and the methods used in general.

if you have any suggestion, advice or solution, i will thank u a lot
with all my respect.
and please forgive me and my poor english writing.

Sylvain MAURY, from FRANCE.

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 07:28:17 2004

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Glen:

May I inquire why No. 1-1/2? This thickness is recommended if, and only if,
there is little or no mounting medium between the specimen and the underside
of the cover glass (e.g., blood films spread on a cover glass, cells grown
in culture on a cover glass, freshly mounted slides that are "cooked" to
evaporate the solvent and reduce the mounting medium thickness). Otherwise,
No. 1 cover glasses are best -- despite what some have written. The
thickness engraved on microscope objective mounts is equivalent to No. 1-1/2
cover glasses, but fails to include real life mounting circumstances (i.e.,
substantially thick mounting medium). The No. 1-1/2 thickness is for the
benefit of lens designers, who must use specific thicknesses in their
optical calculations, and not for those who prepare specimens.

Gary Gill

-----Original Message-----
} From: Glen MacDonald [mailto:glenmac-at-u.washington.edu]
Sent: Tuesday, March 30, 2004 11:53 AM
To: MSA

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (echeung-at-eyetk.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, March 30, 2004 at 09:40:36
---------------------------------------------------------------------------

Email: echeung-at-eyetk.com
Name: Eunice Cheung

Organization: Eyetech

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have any suggestions in flattening tissue especially eye tissue?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 07:39:54 2004

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I have received a number of responses to my query below. A quick summation
is as follows:

No one has been able to indicate a benefit to a cooled magnetron head other
than that some designs get quite hot and need some sort of cooling. The
peltier cooling removes the need for water cooling. Other units do not
require this.

Most people indicate that a diaphragm pump is not as efficient as a standard
rotary pump. Since this is only to back the turbo pump in the HR coaters,
there seems to be little concern about getting oil back-streaming into the
sample chamber. However, the diaphragm pump would be preferable in
clean-room situations.

Ion beam systems are very desirable but also very expensive. Most have
opted for the magnetron type and seem satisfied with their choice.

Everyone suggested working with Pt rather than Cr routinely to avoid the
oxidizing problem. Ir works great if you can handle the additional expense.
I have not had specific comments on Pt/Pd vs. Pt vs. W. Anyone have a
preference?

There were a number of concerns about inefficient use of target material.
However, this is partially linked to evaporating current. As I understand
it, the higher the current the more focused the sputtering beam but this
results in a reduced diameter on the sputter head where metal is withdrawn.
Perhaps manufacturers need to provide better guidelines as to recommended
amperage to get most efficient use of the targets.

A number of people recommended getting targets from the source below (I have
no commercial interest in this company ...just glad to hear about them).
Apparently they will give credit for returned spent targets as will SPI.

Abe Dayani
Refining Systems Inc.
PO Box 72466
Las Vegas, NV 89170
Tel: 702-368-0579
Fax: 702-368-0933

Debby

=================================================

On 3/29/04 11:12 PM, "Debby Sherman" {dsherman-at-purdue.edu} wrote:

}
}
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} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Hi all,
}
} I am researching sputter coaters for HR FESEM imaging. I would
} appreciate hearing from users about their experiences with specific coater
} makes and models. Ion beam is out of my price range so I am looking at
} magnetron type coaters. Please no venders this round.
}
} A couple of specific questions that I would like input on:
} Value of cooled magnetron sputter head (specifically peltier cooling) vs.
} non-cooled
} Merits of getting a diaphragm pump rather than standard rotary pump to back
} turbopump
} Thickness monitor: how useful and how well do they work.
} Reliability...
}
} Also I have heard of the problems with Cr oxidizing and Ir is quite
} expensive. What other metal do you like using that balances the desired
} small grain with reasonable stability, performance, and cost.
}
} Thanks,
} Debby
}
}
} Debby Sherman, Manager Phone: 765-494-6666
} Life Science Microscopy Facility FAX: 765-494-5896
} Purdue University E-mail: dsherman-at-purdue.edu
} S-052 Whistler Building
} 170 S. University Street
} West Lafayette, IN 47907
} http://www3.agriculture.purdue.edu/microscopy
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 08:02:17 2004

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No. 1.5 thickness...maybe Glen has an inverted scope? 1.5 is optimal
for our inverted system.

J

Gary Gill wrote:

}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Glen:
}
} May I inquire why No. 1-1/2? This thickness is recommended if, and only if,
} there is little or no mounting medium between the specimen and the underside
} of the cover glass (e.g., blood films spread on a cover glass, cells grown
} in culture on a cover glass, freshly mounted slides that are "cooked" to
} evaporate the solvent and reduce the mounting medium thickness). Otherwise,
} No. 1 cover glasses are best -- despite what some have written. The
} thickness engraved on microscope objective mounts is equivalent to No. 1-1/2
} cover glasses, but fails to include real life mounting circumstances (i.e.,
} substantially thick mounting medium). The No. 1-1/2 thickness is for the
} benefit of lens designers, who must use specific thicknesses in their
} optical calculations, and not for those who prepare specimens.
}
} Gary Gill
}
} -----Original Message-----
}
} } From: Glen MacDonald [mailto:glenmac-at-u.washington.edu]
}
} Sent: Tuesday, March 30, 2004 11:53 AM
} To: MSA
} Subject: [Microscopy] Coverslip source
}
}
}
}
} ----------------------------------------------------------------------------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America To

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 08:23:17 2004

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Our microprobe lab is separate from most of the other electron microscopes
here at the University of Minnesota. Most of the others are under the
auspices of the "Characterization Facility" that has several staff members
with varying expertise -- I'm sure most of them are on this listserv, and
they could tell you a lot more about how the labs in their organization
operate.

My responsibilities lie solely in the Electron Microprobe Laboratory here
in the Department of Geology and Geophysics. I'm in charge of our JEOL
8900 and the associated equipment and facilities. I stay within our lab,
but I do help a variety of users: users from our department, users from
other departments (Materials Science, Chemistry, Physics, Dentistry, Civil
Engineering, etc.), users from other universities, commercial clients, and
government agencies. I also have a lab assistant helping me in our lab,
doing polishing, new standards testing, providing user assistance, etc.

More about how our lab is organized can be found at our website:
http://probelab.geo.umn.edu

If you have any more specific questions, feel free to contact me directly.

I also expect to be helping out the Anthropology Department when (actually
more like "if") they finally get a used SEM to use for their research.

Ellery

---------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
Department of Geology & Geophysics
University of Minnesota - Twin Cities
Lab Website: http://probelab.geo.umn.edu

On Mar 31, 2004, at 1:04 AM, hilsley wrote:
}
} I am interested in hearing about how other labs run their departments.
} What I would like to know is: the people running the EM labs, do they
} rotate out to routine labs or do they stay in the EM lab.
}
} I appreciate everyone's input.
}
} Thanks
} Helen Ilsley

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 08:23:56 2004

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Hi all!

I am interested to hear about experience with freeze drying instead of
CPD for SEM preparation. It is not for very high resolution imaging, we
have had problems with collapsing cells on delicate plant specimens
(mainly Arabidopsis) after CPD preparation and wonder if perhaps freeze
drying would do the trick. I have seen that EMITECH has a (relatively)
simple freeze drier at around -60°C and most likely there are other
brands as well.

cheers,
Stefan

+++++++++++++++++++++++++++++++++++++++++++++++++++++++
Dr Stefan Gunnarsson
Uppsala universitet Uppsala University
Evolutionsbiologiskt centrum Evolutionary Biology Centre
Enheten för biologisk strukturanalys Microscopy and Imaging Unit
Norbyvägen 18A
SE75236 Uppsala, Sweden Tel & Fax: +46 - 18 471 2638
+++++++++++++++++++++++++++++++++++++++++++++++++++++++

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 09:05:50 2004

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Stefan,
We do a lot of imaging of very young arabidopsis seedlings.
Freeze-drying will still cause sample shrinkage and cell collapse in these
very delicate tissues. The best way to deal with them is using cryo. This
is not an inexpensive option but can be easily justified not only for this
sample but for any hydrated sample such as hydrated gels. We have also
imaged pudding, ice cream, collagen gels, microvesicles, synthetic polymer
gels, etc. etc.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 3/31/04 9:52 AM, "Stefan Gunnarsson" {Stefan.Gunnarsson-at-ebc.uu.se} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Hi all!
}
} I am interested to hear about experience with freeze drying instead of
} CPD for SEM preparation. It is not for very high resolution imaging, we
} have had problems with collapsing cells on delicate plant specimens
} (mainly Arabidopsis) after CPD preparation and wonder if perhaps freeze
} drying would do the trick. I have seen that EMITECH has a (relatively)
} simple freeze drier at around -60°C and most likely there are other
} brands as well.
}
} cheers,
} Stefan
}
} +++++++++++++++++++++++++++++++++++++++++++++++++++++++
} Dr Stefan Gunnarsson
} Uppsala universitet Uppsala University
} Evolutionsbiologiskt centrum Evolutionary Biology Centre
} Enheten för biologisk strukturanalys Microscopy and Imaging Unit
} Norbyvägen 18A
} SE75236 Uppsala, Sweden Tel & Fax: +46 - 18 471 2638
} +++++++++++++++++++++++++++++++++++++++++++++++++++++++
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 09:20:01 2004

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Hello everyone,

We are about to take delivery of an FEI Quant 200 3D FIB/ESEM and I
have to move out my old E3 which was in very poor health when I turned
it off last night. It had had water in the electronics rack and
possibly needed up to $18K (FEI pricing) of repairs. I am going to
send it to our property disposition people, who will probably end up
junking it. So before it goes I am listing it here as available. It
is a E3 with a LaB6 filament and ion pumped gun. It has not Peltier
stage or hot stage (I am keeping those) and it has no ET or BSE
detector. It is basically a stock microscope with three Alcatel rotary
pumps. There is no chiller or compressor, just the scope. If you want
any of it then you are welcome. I will ship it, but the "winner" pays
the shipping and I don't want to hear any whining when it does not live
up to your expectations. the system served us well for nearly 14 years
and so you know what to expect. However, if you need a power supply or
board then this may be the thing for you.

--
John Mansfield PhD MInstP
North Campus Electron Microbeam Analysis Laboratory
417 SRB, University of Michigan
2455 Hayward, Ann Arbor MI 48109-2143 USA
Phone: (734) 936-3352
FAX (734) 763-2282
Cell. Phone: (734) 834-3913
(Leaving a phone message at 936-3352 is preferable to 834-3913)
Email: jfmjfm-at-engin.umich.edu
URL: http://emalwww.engin.umich.edu/people/jfmjfm/jfmjfm.html
Location: Lat. 42° 16' 48" Long. 83° 43' 48"
AIM: thejfmjfm

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 10:04:11 2004

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Dear Eunice,

In the early days of confocal, we had great success imaging eye tissue without any processing. As a matter of fact, I collected a great cross section with Dr. Barry Masters which revealed incredible surface and internal structure. (Last information was that he was at USUHS in Bethesda). There are also now companies which make confocals specifically for opthalmic research.

Good hunting!
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

~-at-~-at-~~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-

At 08:03 AM 3/31/04 -0600, echeung-at-eyetk.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 10:42:33 2004

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I recommend trying an electrolytic etch. I use a sheet of 300 series SS as
cathode, about 1.5 x 4 inches bent to fit around the inside of an etching
dish, of about 100 or 150ml capacity, sufficient anyway that the
metallographic mount is fully immersed in the etchant. The etchant can be
nitric acid at about 3:1 (water:conc nitric), but other etchants will work
as well or better and you can find solutions in one of many metallographic
sourcebooks. For an anode connection I use a stainless wire about 1mm
diameter held with a crocodile clip which I touch to a corner of the
polished specimen in the metallographic mount immersed in the etchant. I
use a voltage of around 1.5 up to about 3 volts DC, (you can use an ordinary
dry cell or two in series) the higher voltages act much more quickly. There
is no reaction of the specimen (if it is SS or nickel etc.) until you touch
the anode wire to the specimen. It's easy to over etch because it can be
difficult to see the progress of the etch. Most often I try to adjust
voltage until etching requires about 15 to 25 seconds. This is a simple
way to etch such alloys (and others) and avoids use of nasty solutions such
as glyceregia.

Vern Griffiths, Montana Tech

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 11:43:11 2004

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Hi, all

This thickness is actually an optical issue, designed as part of the engineering of the objective. If you read the engravings on the objective, you will see "0.17", indicating that that piece of glassware expects to see a coverslip of 0.17mm thickness on top of the sample. # 1-1/2 coverslips are designed to average that thickness.

Having said that, the sample always rules, so if you find that a thinner coverslip gives you better results, go for it. Caution: #2 coverslips are too thick and will cause spherical abberation (milky,hazy images).

Hope this is helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

~-at-~-at-~~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-

At 08:52 AM 3/31/04 -0500, Gary Gill wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 11:59:06 2004

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Mounting medium is an optical extension of the cover glass; it has
appreciable thickness, as well as refractive index and dispersion values
comparable to glass. Its thickness should be subtracted from the ideal
thickness of the No. 1-1/2 cover glass. Ergo, No. 1 in practice, not No.
1-1/2 in theory.

Imaging consequence of spherical aberration to which Barbara alluded can be
mimicked by glare and flare caused by dirty lenses and wide open substage
condenser aperture (i.e., non-Kohler illumination).

The negative imaging consequences of using No. 1-1/2 cover glasses will be
seen with objectives having a numerical aperture of 0.6 and greater, and not
the lower numerical aperture objectives such as those associated with 10x
achromat objectives. Apochromat objectives have higher NAs power-for-power
than do achromats and so are less forgiving.

Partially closing the aperture diaphragm reduces the working numerical
aperture of an objective, and is the user's safety net for capturing image
quality in specimens covered with overly thick mounting medium and cover
glass combinations.

Similar discussions have taken place several times on this listserve, once
resulting in a brief invited article by me in Microscopy Today.

Gary Gill

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 15:05:42 2004

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Thanks all for the suggestions.

I 'm contacting a specialty mfr. and switching our routine orders to
VWR. Gary raises good points. However, in using thinner coverslips,
one must assume that the refractive index on each side of the
coverslip is approximating the design specifications of the objective.
I've used #1 on exceptionally thick samples for brightfield, but the
specimens were cleared and mounted in a medium that closely matched
the RI of the coverslip. Oil immersion can compensate for thinner
glass as well, which is a good thing considering the variation across a
coverslip. but, in working with samples close to the coverslip or
mounted with RI mismatches (or inherently containing RI mismatch), then
coverslip thickness is important. Few labs have glycerol and water
immersion lenses for routine use, which means the spherical aberrations
become quite serious as one focuses into deeper samples.

My immediate need is to create fluorescent test specimens on
coverglass, and thick specimens. Known thicknesses eliminate
variability between samples mounted in various media.

Regards,
Glen

On Mar 31, 2004, at 5:52 AM, Gary Gill wrote:

} Glen:
}
} May I inquire why No. 1-1/2? This thickness is recommended if, and
} only if,
} there is little or no mounting medium between the specimen and the
} underside
} of the cover glass (e.g., blood films spread on a cover glass, cells
} grown
} in culture on a cover glass, freshly mounted slides that are "cooked"
} to
} evaporate the solvent and reduce the mounting medium thickness).
} Otherwise,
} No. 1 cover glasses are best -- despite what some have written. The
} thickness engraved on microscope objective mounts is equivalent to No.
} 1-1/2
} cover glasses, but fails to include real life mounting circumstances
} (i.e.,
} substantially thick mounting medium). The No. 1-1/2 thickness is for
} the
} benefit of lens designers, who must use specific thicknesses in their
} optical calculations, and not for those who prepare specimens.
}
} Gary Gill
}
} -----Original Message-----
} From: Glen MacDonald [mailto:glenmac-at-u.washington.edu]
} Sent: Tuesday, March 30, 2004 11:53 AM
} To: MSA
} Subject: [Microscopy] Coverslip source
}
}
} Can anyone suggest a source of #1.5 thickness coverslips with
} manufactured accuracy and consistancy in thickness? I've been going
} through boxes of coverslips from Corning, VWR and Clay-Adams to make
} some test samples with 170 micron coverglass. A good box of Corning
} has maybe 3 and 2/3 of the rest are 180 to } 200 microns. VWR has
} proven to have the most consistency, but at least half are } 180.
}
} thanks,
} Glen
Glen MacDonald
Core for Communication Research
Virginia Merrill Bloedel Hearing Research Center
Box 357923
University of Washington
Seattle, WA 98195-7923 USA
(206) 616-4156
glenmac-at-u.washington.edu

************************************************************************
******
The box said "Requires Windows 95 or better", so I bought a Macintosh.
************************************************************************
******

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 15:10:26 2004

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Hi Gary,

I think you don't quite have the whole story. It depends on whether
we are talking water or oil immersion.

Oil:

If you have an oil lens, oil between it and the coverslip AND the
specimen itself has an RI that is close to oil, then, to the extent
that all three optical layers have the same RI, it doesn't matter how
thick the coverslip is. A #1 (or, for that matter, a #00) will
allow you to look farther down into the specimen. (In reality, it
does matter a bit because the RIs don't match at all wavelengths).

The problem here is that most embedding media don't match the RI of
immersion oil, especially if they have biological material in them.

If you are looking at a water specimen with an oil lens and immersion
oil between it and the coverglass, then again the thickness of the
glass is not very optically important and things close to its surface
will look fine. Regardless of the thickness coverslip, the SA will
rapidly get worse as you penetrate into the aqueous medium.

Water:

If you have a water lens and water or something close to it, on both
sides of the coverslip, then the exact thickness of the coverglass
becomes VERY important (a 2 micrometer error is significant). This is
because, water (unlike immersion oil) has an RI VERY different from
that of the coverslip.

You can use a coverglass thinner than 170 micrometers but only if the
correction collar will allow you to adjust for its actual thickness.
(the calibration of such collars is often incorrect.)

Cheers,

Jim Pawley

}
}
} Glen:
}
} May I inquire why No. 1-1/2? This thickness is recommended if, and only if,
} there is little or no mounting medium between the specimen and the underside
} of the cover glass (e.g., blood films spread on a cover glass, cells grown
} in culture on a cover glass, freshly mounted slides that are "cooked" to
} evaporate the solvent and reduce the mounting medium thickness). Otherwise,
} No. 1 cover glasses are best -- despite what some have written. The
} thickness engraved on microscope objective mounts is equivalent to No. 1-1/2
} cover glasses, but fails to include real life mounting circumstances (i.e.,
} substantially thick mounting medium). The No. 1-1/2 thickness is for the
} benefit of lens designers, who must use specific thicknesses in their
} optical calculations, and not for those who prepare specimens.
}
} Gary Gill
}
} -----Original Message-----
} } From: Glen MacDonald [mailto:glenmac-at-u.washington.edu]
} Sent: Tuesday, March 30, 2004 11:53 AM
} To: MSA
} Subject: [Microscopy] Coverslip source
}

--
**********************************************
Prof. James B. Pawley, Ph. 608-263-3147
Room 223, Zoology Research Building,
FAX 608-265-5315
1117 Johnson Ave., Madison, WI, 53706
JBPAWLEY-at-WISC.EDU
3D Microscopy of Living Cells Course, June 12-24, 2004, UBC, Vancouver Canada
Info: http://www.3dcourse.ubc.ca/ Applications due by March 15, 2004

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 15:28:37 2004

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Thanks, Jim. My experience is with oil, not water. I'm familiar with the
information you provided, but some of my scholarly reprints take exception
with some of your remarks. Specifically, thickness does matter -- even when
all three RI's match, differences in dispersion notwithstanding (i.e., the
Abbe number [?]).

As I recall, the formula that optical engineers use when computing cover
glass thickness and so forth shows that thickness matters. This is the
formula that Setterington published (Setterington R. VI. - The
specification of a standard microscope cover-glass. J Roy Micr Soc.
1953;73:69-76).

Whether the correction collar is correctly calibrated is moot, IMHO, as long
as the user can adjust it to get maximum resolution and contrast.

In my world of cytopathology (e.g., Pap smears), dry objectives are used
virtually exclusively. Conventional Pap smears are often so thick that
substantial volumes of mounting medium are needed to permit coverslipping.
Even the so called thin-layer Pap smears benefit from the use of No. 1 cover
glasses.

A side benefit of using No. 1 cover glasses is cost savings. Since cover
glasses are priced by the ounce, we get more No. 1's per oz than we would if
we used No. 1-1/2.

As I've moved on to become a compliance officer, it's been quite some time
since I thought about these issues, so please excuse my apparent fuzziness.

Gary

-----Original Message-----
} From: James Pawley [mailto:jbpawley-at-facstaff.wisc.edu]
Sent: Wednesday, March 31, 2004 4:32 PM
To: Microscopy-at-sparc5.microscopy.com

Hello everybody:

I am looking for a copy of "Desktop Microscopist" (either Mac or PC
version). Can anybody please tell me where I can buy it? It seems Lacuna
Labs / Virtual Labs are no longer selling this product (They haven't
mentioned about it on their websites).

Thanks and Best Regards
Nina,
State Univ. of New York at Stony Brook

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 16:13:30 2004

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I'm looking for feedback on charges for using the confocal microscope. We have
been charging people in the institution $40/hour to use the scope. (That
includes the training sessions; once they are trained, they use it themselves).
Outside the institution, we charge $65.00/hour. We think these charges are too
low and would like to raise them.

What do other facilities charge? You can respond directly to me or to the
listserver.

Thanks!
Peggy
Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 16:33:31 2004

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Hi:

I need some advice so I can help a student in the lab.

She is looking at sea shells to check for grinding marks. The shells were
used for beads and 'money' by ancient people. She wants to see if the
shells have tool marks, or were collected from the beach with holes made by
natural processes.

She has some 'modern' shells she had prepared. These are expendable and
will be easy to cut and coat for SEM.

She has some museum specimens that she cannot do much to, making it
difficult to do the SEM.

I do not have access to an ESEM. I do have a Robinson BSED. I don't think
she can coat these samples.

She might be able to make a replica of the museum samples using dental
impression material. Anybody tried this? What are the details?

Any other ideas?

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 16:43:01 2004

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For shells, wouldn't a stereo zoom microscope
do the job? Most research models will go up
to about 100X. Need more? Then probably an
ESEM or VPSEM application.

gary g.

At 02:54 PM 3/31/2004, you wrote:

} Hi:
}
} I need some advice so I can help a student in the lab.
}
} She is looking at sea shells to check for grinding marks. The shells were
} used for beads and 'money' by ancient people. She wants to see if the
} shells have tool marks, or were collected from the beach with holes made by
} natural processes.
}
} She has some 'modern' shells she had prepared. These are expendable and
} will be easy to cut and coat for SEM.
}
} She has some museum specimens that she cannot do much to, making it
} difficult to do the SEM.
}
} I do not have access to an ESEM. I do have a Robinson BSED. I don't think
} she can coat these samples.
}
} She might be able to make a replica of the museum samples using dental
} impression material. Anybody tried this? What are the details?
}
} Any other ideas?
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 16:49:57 2004

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Hi,

I have an investigator that wants to see the distribution of Bromated FR
and clay particles in nylon. Do you have any suggestions on embedding and
staining of this type of material?

Thanks in advance,

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 17:19:05 2004

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John,

Infiltrate the bead bore with Dow Corning Silastic "E" from its wide end.
After curing, the silicon rubber should be easy to remove and will
faithfully represent the topography of the inside of the bore.

Scratch marks perpendicular to the long axis of the bore would suggest
rotary abrasive drilling .

Bart Cannon
Cannon Microprobe
Seattle

----- Original Message -----
} From: "Jon Krupp" {jmkrupp-at-cats.ucsc.edu}
To: {Microscopy-at-sparc5.microscopy.com}
Sent: Wednesday, March 31, 2004 2:54 PM

try spraying them with StaticGard -

At 05:54 PM 3/31/2004, Jon Krupp wrote:

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From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 19:44:11 2004

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Hi Debby
There is last cent to your report. It's about diaphragm pumps. Mechanical
pumps produces oil vapors, which will contaminate your sample (it's not
back streaming, it's just oil when you backing the system). So, when you
evaporate metal on the surface, one should be aware that the surface is
quite oily if mechanical pump was used, so it compromise the fine details
on your sample. How much and how it's critical to your application - I
don't know. Diaphragm pumps may help to resolve this problem. They are
noisy, less effective than mechanical pumps and you need to change
diaphragms every few months (quite expensive). Not every turbomolecular
pump could work in tandem with diaphragm (you need to check with
manufacturer). Better solution is "scroll pump" - it's oil-free and pretty
like a mechanical pump by its technical characteristics. It's noisy and
it's big. I remember EDWARDS introduced another kind of dry (oil-free)
pump a few years ago, which is less noisy and smaller. The bottom line
here is: if you need high quality metal coating especially for frozen
samples (oil will condense) you better use dry (oil-free) backing
pump. Personally, I am using tandem of ESDP12 scroll pump and
magnetically levitated STP450 turbo-pump on my home-made system. It
produces 5x10-7 torr vacuum in 20 min from air in 12x14" Bell Jar with
collar and a LOT of O-rings (viton). It seems to me the prime reason for
such efficiency is dry vacuum, because on another system with similar
characteristics equipped with mechanical pump and 800 l/sec DP (Santovac-5)
I could barely have 2x10-6 torr in 1 hour (no LN2). My theory is that oil
in the system (from the "backing" cycle) "traps" air and then it takes time
for air to be released, so it slows down the pumping speed. I have to
admit, I had hard time with Cressington. For some reason they were quite
nasty to me when I was asking questions about performance of their vacuum
evaporators. Finally, I force somebody (poor guy, he has to ask
permission) at Ted Pella's stand to show me how Cressington's desk-top
vacuum evaporator (I don't remember what the model was, it was surely TP
with mechanical) works. So, we vent the chamber in order to see how
quickly it will maintain the vacuum. It was able to make 5x10-5 torr in 2
hours and next day it was still 10-5 range (they did not shut it down and
actually had directions from Cressington DO NOT vent the chamber
anymore). It was at the time I was hunting for new vacuum
evaporator. Honestly, I did not find anything good on the market and
decided to build my own system and I am quite happy with my design. In
general, I do find (no financial or other interest, just happy user) that
EDWARDS produces very good solid vacuum equipment. As a matter of fact, my
vacuum system built on 80% from EDWARDS components. If Cressington guys is
here, there is message to them: I don't want to compromise their equipment,
but express my personal experience.
Sergey.

At 11:39 AM 3/30/2004, you wrote:

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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 21:58:24 2004

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Colleagues:

This is the second announcement for a 2-day mini-workshop in
Cryoultramicrotomy for The Materials Sciences which will be held at RJ Lee Group in
Pittsburgh, PA next week. If you plan to attend but have not yet responded, please see
below for the contact persons to whom you may send your RSVP. As always, we
need an accurate head count for meals and refreshments.

The details are as follows:

List members in the Pittsburgh, PA area who have an interest in materials
science are cordially invited to a free two-day "mini-workshop" on
Cryoultramicrotomy for The Materials Sciences.

This topic is of special interest for those who work with polymers or other
materials which could benefit from ultrathin sectioning or surface "polishing"
at low temperatures (no embedding required).

The workshop will be hosted by RJ Lee Group, Inc. in Monroeville, PA. This
invitation is open to everyone in the Pittsburgh, PA / Youngstown, OH / Akron,
OH area.

Below are the details:

**What**:
Mini-Workshop on Cryoultramicrotomy for Materials Science

**When**:
Tuesday, April 6th, 2004, 9:00 am through Wednesday, April 7th, 2004, 4:00 pm.

A tour of the facilities at RJ Lee Group will be given at the beginning of
the workshop.

**Where**:
RJ Lee Group,Inc., 350 Hochberg Rd., Monroeville, PA.

**Format**:
A presentation on cryoultramicrotomy and its applications in the materials
sciences will be given on the first day, as well as demonstrations on the
preparation of cryotools (hair probes, large and small wire loops, etc.) and glass
knife making and evaluation. The care and cleaning of diamond knives will also
be discussed.

The demonstrations will be followed by open lab sessions for the attendees to
prepare their own cryotools and glass knives.

Also on the first day an introduction to the cryoultramicrotome will be
given, and attendees will have an opportunity for hands-on use of the Instrument.

The second day will be reserved for attendees to sign up in small groups for
additional time and training on the instrumentation, depending on the
attendees' individual needs.

**Limited Space Available**:
The lectures and demonstrations on the first day are open to everyone, but
space is limited to *10 persons* for the in-depth training and extended use of
the instrumentation on the second day.

**Contacts**:
To RSVP and to reserve a seat for the second day's sessions, please contact
any of the following people. We also need to know if you are bringing
specimens with you.

Ms. Kim Megaw, RMC Products / Boeckeler Instruments, Inc.,
800.552.2262
{kim-at-boeckeler.com}

Mr. Hank Beebe, RJ Lee Group
724-325-1776
{hbeebe-at-rjlg.com}

Dr. Robert Chiovetti, RMC Products / Boeckeler Instruments, Inc.,
800.552.2262
{bob-at-boeckeler.com}

We hope to see you soon in Monroeville!

Robert (Bob) Chiovetti, Ph.D.
RMC Products
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed Mar 31 22:20:32 2004

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First off, high resolution needs to be defined.
What mag range are you working in? If you are
less than say 75KX, then extreme measures are
not needed, IMO.

The magnet/magnetron sputter coaters are cool coaters--no heat.
Specimens are not affected. I have used Anatech Hummer
VII, Denton Desk II and Cressington 208HR. All but the
208HR use mechanical pumps. The 208HR uses a mech pump
and small turbo. The Denton uses a diaphragm pump.
The Anatech uses a dual stage mech pump (Edwards, et. al.).

Target life with the 208HR is very short. I suspect
that this is due to thin targets (they fall out). The Hummer uses a
proprietary annular target but it lasts a long time
(longer it seems than the coater system lasts). The Denton target
is also very long lived. I have used Au, Au/Pd and Pt.
For high resolution fine grain, Pt is very good. Use
low current, high vacuum, long time. You can get a very
fine grain. With Au and even Au/Pd at wrong conditions,
it is not hard to see the coating structure at 100KX.

I do not use thickness measuring accessories. My method
is to coat cover slips and use an elipsometer to calibrate
them according to thickness and then put them in a transmitted
LM. The elipsometer (Nanospec) is very accurate. Using
the LM is more routine (digicam exposure time). I do this
every quarter to make sure that my coatings are within my specs.

The Denton Desk II that I use has variables of vacuum,
current and time. I keep time constant, current constant
and vacuum constant for specific coating thicknesses.
Then, I only vary time to get different thicknesses.
It uses a Japanese diaphragm pump. It works quite well.
Quiet, fast and repeatable. Not costly either.

The Nevada target source is a great asset. Very good.
If you are sold thin targets at high prices from OEMs,
get replacements from NV at a fraction of the cost for
a much more long lived target. But...it must be a simple
geometry target--a disc. I don't think that they supply
annular targets.

Os is probably an ultimate coater. But the cost is also
stratospheric. With the advent of VPSEM, coating may
be history. I'm looking forward to this with a new
VPSEM. If not eliminating coating, reducing the need
for it will be nice.

Other questions, please e-mail...less clutter.

gary g.

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Most of the cost of supplying one sputter target to a specific size direct from
the manufacturer is the setup and handling cost to cut a specific shape or
diameter. If you order direct from a specialist manufacturer of sputter
targets such as Testbourne Ltd http://www.testbourne.com (I suspect this is
the source Gatan uses for targets for the Alto, for example) you will find
that their quotation for 10 off is only about 10% more than the quotation for 1
off, making the cost of targets suddenly remarkably affordable. The unit cost
will fall further as the number ordered increases. Also, doubling the foil
thickness requested from, say, 0.05mm to 0.10 mm, does not have a commensurate
impact on the price, and thicker targets last longer. Try it - I think you'll
like it.

Best wishes
Chris Jeffree

University of Edinburgh

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Hello everyone,

Can anybody kindly provide me with the following info
about "Carbon films on Metal grids" for HRTEM sample
preparation. Thank you in advance.

1. How high temperature the carbon films can withstand
in the reactors (e.g. oven) without damage? What
negative effect can result from the high temperature
on the C films?

2. We need to collect TEM samples directly from the
high-temperature (around 1200 C) reactor onto
Carbon-support films (or any other alternative) on
some metal grids. Do you have any good suggestions?

Thank you very much in advance.

- juha

Electron Microscope Unit,
Helsinki Univ. Tech.

__________________________________
Do you Yahoo!?
Yahoo! Small Business $15K Web Design Giveaway
http://promotions.yahoo.com/design_giveaway/

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 09:15:15 2004

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Jon,

We have an archeologist here who routinely makes replicas of beads
and other objects that can't be sputter coated. He uses 3m Express,
vinyl polysiloxane impression material, light body, medium set,
product number 7302HB and gets fine-scale impressions. Fine enough to
determine the technology used the drill the hole, including if the
drilling was done recently using an ancient method (commonly done to
make "ancient beads" to sell to tourists). This material should do
for your student's work.
There have also been several articles on replicating surfaces run in
Microscopy Today which might help.

Phil

} Hi:
}
} I need some advice so I can help a student in the lab.
}
} She is looking at sea shells to check for grinding marks. The shells were
} used for beads and 'money' by ancient people. She wants to see if the
} shells have tool marks, or were collected from the beach with holes made by
} natural processes.
}
} She has some 'modern' shells she had prepared. These are expendable and
} will be easy to cut and coat for SEM.
}
} She has some museum specimens that she cannot do much to, making it
} difficult to do the SEM.
}
} I do not have access to an ESEM. I do have a Robinson BSED. I don't think
} she can coat these samples.
}
} She might be able to make a replica of the museum samples using dental
} impression material. Anybody tried this? What are the details?
}
} Any other ideas?
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 10:06:03 2004

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} I was supposed to receive TEM pictures of my silica powder (SiO2), but
} that never happened. So, I am looking for a way to analyze the surface
} and structure of my silica - the sooner, the better.

} Does Wellesley own a TEM machine or any other device that would give me
} more insight into the surface structure of my powder?

We need to view silica powder (SiO2) surface structure with an electron
microscope. We are in a biological facility and have no experience with
this type of sample. What sort of instrument is best suited for viewing
this sample? What are the sample preparation techniques? Are there labs
that we can bring our sample to for, let's say, an hour of observation and
a few pictures? We are in the Boston, Massachusetts area. Thank you in
advance.

Vachik Hacopian

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 10:49:43 2004

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I've actually done some backscatter SEM on uncoated shells, which worked
pretty well. The resolution isn't as good as a coated specimen, of course,
but would probably work for what your student needs to see. So if you have
a backscatter detector on your SEM, I would try that. I can forward you
some images that I have taken if you like. Let me know.
Regards,
Aaron Bell

} From: Gary Gaugler {gary-at-gaugler.com}
} To: jmkrupp-at-cats.ucsc.edu (Jon Krupp)
} CC: MSA listserver {Microscopy-at-MSA.Microscopy.Com}
} Subject: [Microscopy] Re: SEM of shells
} Date: Wed, 31 Mar 2004 15:07:41 -0800
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_________________________________________________________________
Get tax tips, tools and access to IRS forms – all in one place at MSN Money!
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From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 12:47:18 2004

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I would think that a Robinson BSE should give
excellent image results in BSE mode. If you
have the mixer option or can mix SE+BSE, that
may allow optimization of the image. The problem,
I would think, is that you are looking for morphology
info whereas the BSE produces Z contrast info.
Low KV (2-4KV) should produce excellent surface detail.
At this low KV, you may avoid charging. If you mix
the Robinson with SE, it may do what you need. I've
done this with coral and got good results.

gary g.

At 09:01 AM 4/1/2004, you wrote:

} I've actually done some backscatter SEM on uncoated shells, which worked
} pretty well. The resolution isn't as good as a coated specimen, of
} course, but would probably work for what your student needs to see. So if
} you have a backscatter detector on your SEM, I would try that. I can
} forward you some images that I have taken if you like. Let me know.
} Regards,
} Aaron Bell
}
}
} }
} } At 02:54 PM 3/31/2004, you wrote:
} }
} }
} } } Hi:
} } }
} } } I need some advice so I can help a student in the lab.
} } }
} } } She is looking at sea shells to check for grinding marks. The shells were
} } } used for beads and 'money' by ancient people. She wants to see if the
} } } shells have tool marks, or were collected from the beach with holes made by
} } } natural processes.
} } }
} } } She has some 'modern' shells she had prepared. These are expendable and
} } } will be easy to cut and coat for SEM.
} } }
} } } She has some museum specimens that she cannot do much to, making it
} } } difficult to do the SEM.
} } }
} } } I do not have access to an ESEM. I do have a Robinson BSED. I don't think
} } } she can coat these samples.
} } }
} } } She might be able to make a replica of the museum samples using dental
} } } impression material. Anybody tried this? What are the details?
} } }
} } } Any other ideas?
} } }
} } } Thanks
} } }
} } } Jonathan Krupp
} } } Microscopy & Imaging Lab
} } } University of California
} } } Santa Cruz, CA 95064
} } } (831) 459-2477
} } } jmkrupp-at-cats.ucsc.edu
} }
}
} _________________________________________________________________
} Get tax tips, tools and access to IRS forms all in one place at MSN
} Money! http://moneycentral.msn.com/tax/home.asp
}

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 14:23:28 2004

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On Apr 1, 2004, at 7:19 AM, Juha Dapper wrote:

} Can anybody kindly provide me with the following info
} about "Carbon films on Metal grids" for HRTEM sample
} preparation. Thank you in advance.
}
} 1. How high temperature the carbon films can withstand
} in the reactors (e.g. oven) without damage? What
} negative effect can result from the high temperature
} on the C films?
}
} 2. We need to collect TEM samples directly from the
} high-temperature (around 1200 C) reactor onto
} Carbon-support films (or any other alternative) on
} some metal grids. Do you have any good suggestions?

Dear Juha,
For depositing samples at high temperature, you want the support film
to have the same coefficient of expansion as the grid material, and the
easiest way to do that is to make the film from the same material as
the grid. You also want a low-z material that is strong, so that a
thin film will not interfere with microscopy of the sample. If the
pieces of the sample are larger than 2 um, you can use a holey film and
examine the areas of the specimen that lie over the holes. Cu grids
themselves will not work, since Cu melts at 1083 C. Ti grids will be
useable at 1200 C, and either Ti or Ti-Si (88%Ti + 12% Si) should make
a suitable film. A lower-z alternative is Be, but it is very toxic.
Mo grids have a similar coefficient of expansion to C at LN2 temp, so
these grids have been used with cryo specimens to eliminate crinkling,
but I don't know what will happen to this combination at high temps.
Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

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Dear Juha,
I think that the carbon film on your TEM grids would burn away if you put it in
a furnace at 1200 degrees C, unless you could exclude all oxygen or oxidizing
sources. If it is a carbon-coated formvar or collodion (plastic) film it will be
even more heat-sensitive. You may find a SiO film is more oxidation-resistant.
It evaporates much like carbon in an evaporator, but I have not tried to heat
it. When we did heat-treat studies of an Al alloy by sandwiching the TEM foil in
a Cu folding grid and putting it back and forth from the TEM to the furnace, we
found the Cu grid oxidized too much, and so we switched to Ni folding grids, and
they worked fine. Can you sample the outlet of the reactor, where the gas has
cooled a bit?
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Juha Dapper" {juha_dapper-at-yahoo.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, April 01, 2004 7:19 AM

A not unknown fenomena: in our lab there are too some people who have
problems with it, although not that strong, when moving away from the
microscope for a short time (a minute or so), they feel already better. And
I must admit, I also suffer a very little bit from it, and (but this is feed
for psychologists I think), more when working on a Leica then on a Zeiss...
No offence Leica! ;-) And more on high then on low magnification...
A solution:, easy in a way, but possibly not immediate applicable: project
the image on a screen. You also have those small screens attached on an
ocular which project the image of the ocular onto this 'personal', small
screen, so a camera is not needed.
Also, move away often and let the eyes relax.
Good luck,

Sven Terclavers

-----Original Message-----
} From: Tom Phillips [mailto:phillipst-at-missouri.edu]
Sent: Friday, March 05, 2004 16:17 PM
To: Microscopy-at-MSA.Microscopy.com

My undergrad histology class has given me a new and novel problem. One of
the students is experiencing severe motion sickness while she views
specimens on a standard binocular compound microscope. I have had students
bothered when viewing specimens on the 6-headed scope and someone else is
moving the specimen field but this is a first. Any one have an easy
suggestion?

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 18:35:03 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (pwebster-at-hei.org) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, April 1, 2004 at 11:12:05
---------------------------------------------------------------------------

Email: pwebster-at-hei.org
Name: Paul Webster

Organization: House Ear Institute

Title-Subject: [Microscopy] [Filtered] MListserver: HR Sputter Coater

Question: I have been watching this disccusions with some interest. However, the replies have confused me. It seems that high resolution sputter coating requires a clean, high vacuum - yet most sputter coaters use an intert gas to create an inonizable environment and operate at a pre-set, low vacuum. What is the need for high vacuum?

There also seems to be a need for magnetron cooling, but other messages suggest that magnetrons do not warm up when being used. Which is correct?

} From the literature on metal coating of freeze-fractured specimens, it is clear that the best (fine grain) coats are obtained when the specimen (not the source) is cooled. From what I understand of this literature it seems that warm metal grains can actually move around on the specimen before settling in place. It is during this migration that they aggregate to form the grains we see. If specimen cooling is important, why don't any of the commercial sputter coaters cool the specimens?

No-one has mentioned the possibility of using non-coating methods that employ multiple exposures to osmium tetroxide so that metal is placed in the specimen and not over it. Are there so many disadvantages to this approach for it to be disregarded so easily?

} From my experience in coating very complex specimens it is clear that the metal coat really has no chance of covering large parts of the specimen, yet even small coverings of platinum over only small areas seem to improve the ability of the SEM to image the specimen. Given this proactical observation, do we really need to make sure the specimen is properly grounded before examining it?

Regards,

Paul Webster.

Hosue Ear Institute
2100 W 3rd St.
Los Angeles, CA 90057.

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From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 18:36:07 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (basgen-at-umn.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, April 1, 2004 at 11:44:59
---------------------------------------------------------------------------

Email: basgen-at-umn.edu
Name: John Basgen

Organization: University of Minnesota

Title-Subject: [Microscopy] [Filtered] MListserver:Stereology Course

Question: The 8th American Stereology Course sponsored by the International Society for Stereology will be held September 26-October 1, 2004 in Minneapolis, Minnesota, USA.

The course is an intense 6-day learning experience, which includes lectures and hands on exercises each day. In the evenings, participants have the opportunity to discuss their individual projects with the instructors. Topics covered include: 1) The measurement of volumes, surfaces (area), lengths, number, and connectivity in 3-dimensional space using 2-dimensional images; 2) The measurement of these structural parameters, in homogeneous and non-homogeneous tissues; 3) The design of efficient, unbiased sampling strategies; 4) How to determine the optimal number of animals per experimental group and the optimal number of measurements per animal.

Instructors:
Hans JŻrgen G. Gundersen, Stereological Research Laboratory, University of Aarhus, Aarhus, Denmark
Jens R. Nyengaard, Stereological and Electron Microscopy Laboratory, University of Aarhus, Aarhus, Denmark,
Bente Pakkenberg, Research Laboratory for Stereology and Neuroscience, Bispebjerg University Hospital, Copenhagen, Denmark,
Karl-Anton Dorph-Petersen, Department of Neuroscience, University of Pittsburgh School of Medicine, Pittsburgh, PA

The course is intended for persons interested in obtaining morphometric data from biological specimens using unbiased and efficient sampling designs. No prior stereological experience is necessary. The course will be limited to 25 participants.

Registration fee: $675
(includes course materials, lunches, coffee breaks)

To register or for more information contact: John Basgen, University of Minnesota basgen-at-umn.edu 612-625-7979

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From MicroscopyL-request-at-ns.microscopy.com Thu Apr 1 22:33:49 2004

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Osmium tetroxide has been discussed and is available
for coating specimens. It is just too costly to
be viable...IMO. SPI offers this unit. Check it out.

What is interesting is to actually define what "high
resolution" really means. Let's assume that it is fine
grain...whatever that means. Au is definitely out in
this regard. I have had better fine grain results
with Au/Pd and Pt. The key is to keep a high vacuum
( {=100mT) and low current ( {=20mA). Keep these constant
and use time as the final determinator of end point
thickness.

Modern (and most older) coaters use magnetron heads
and do not require water cooling. They work very well.
The differences are in how they allow different variables
to be introduced (time, pressure, current) and the thickness
of the original target material.

At {= 75KX, Au is OK. At or above that, Au/Pd is better.
Ultimately, Pt is best for non-complex sputter coating.
It is fine grain and is not seen below 200KX. Au is
definitely seen as a honeycomb web. Au/Pd is more
difficult to image.

As far as grains moving, they probably do. However,
the issue is "how much?" I do not see them move at
all at normal temperatures. At elevated temperatures,
they do. but this is a separate and more complex
issue.

If the coating is done right, the whole specimen will
be conductive and will not charge. But one must keep
in mind the 3-D nature of specimens. i.e., if a high
dimension specimen is coated without rotating and/or
tilting, it may not have a conductive path to the specimen
stub. Depending on what you are trying to see, some coloidal
silver dag will help form a conductive path from the
specimen to the stub and to ground. This is the way
it is for large and irregular specimens.

gary g.

At 04:47 PM 4/1/2004, you wrote:

} Email: pwebster-at-hei.org
} Name: Paul Webster
}
} Organization: House Ear Institute
}
} Title-Subject: [Microscopy] [Filtered] MListserver: HR Sputter Coater
}
} Question: I have been watching this disccusions with some interest.
} However, the replies have confused me. It seems that high resolution
} sputter coating requires a clean, high vacuum - yet most sputter coaters
} use an intert gas to create an inonizable environment and operate at a
} pre-set, low vacuum. What is the need for high vacuum?
}
} There also seems to be a need for magnetron cooling, but other messages
} suggest that magnetrons do not warm up when being used. Which is correct?
}
} } From the literature on metal coating of freeze-fractured specimens, it
} is clear that the best (fine grain) coats are obtained when the specimen
} (not the source) is cooled. From what I understand of this literature it
} seems that warm metal grains can actually move around on the specimen
} before settling in place. It is during this migration that they aggregate
} to form the grains we see. If specimen cooling is important, why don't
} any of the commercial sputter coaters cool the specimens?
}
} No-one has mentioned the possibility of using non-coating methods that
} employ multiple exposures to osmium tetroxide so that metal is placed in
} the specimen and not over it. Are there so many disadvantages to this
} approach for it to be disregarded so easily?
}
} } From my experience in coating very complex specimens it is clear that
} the metal coat really has no chance of covering large parts of the
} specimen, yet even small coverings of platinum over only small areas seem
} to improve the ability of the SEM to image the specimen. Given this
} proactical observation, do we really need to make sure the specimen is
} properly grounded before examining it?
}
} Regards,
}
} Paul Webster.
}
} Hosue Ear Institute
} 2100 W 3rd St.
} Los Angeles, CA 90057.
}
}
}
}
}
} ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 01:19:40 2004

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Hi all

Why high vaccum before sputtering ? To remove most of the water vapor from
the vaccum, before introducing the (dry) inert gas. One reason for grain
formation, typicaly with gold, is the formation of gold clusters arround
water molecules from the residual vaccum. For the same reason one will
prefere high (dry) gas flow, to diluate and evacuate the water desorbing
from the walls of the chamber. It-s the same goal when one purge the
chamber with argon, before sputtering, on coater which have only a
roughing pump. The effet is only not suffisent to avoid grain formation.

Cooling the head or not ? Depends on the sputter time and current. For 30"
at 20 mA, no matter in cooling. For 5' at 80 mA, depending how the head is
built, but I would cool it... On production magnetrons, the head is always
cooled.

A last word about the grain formation . We are always comparing coating
materials, without any consideration of the substrate. In a good clean
vaccum, saying UHV (!), the grain or film formation depends on the pair
substrate/adsorbate. Of coarse, on a clean substrate, without water and
organics on it, what's not the case with SEM samples ! An for example, on
glass or in general on oxydes, gold will give in most cases grains. Ir
not. But gold on mica or MoS2 gives a layer. So there are general rules
and particuar cases ! In a good sputter coater, Ir, Pt or Cr (apart the
oxydation pb) seems to give acpetable results for HR SEM, what not the
case with Au. The goal is not to build a conducting film, but to have an
minimum, homogeneous and stable charging of the sample. Carbon and low
voltage work too.

Hope it helps;

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 08:11:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (staylor-at-fit.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Thursday, April 1, 2004 at 11:02:08
---------------------------------------------------------------------------

Email: staylor-at-fit.edu
Name: Scott Taylor

Organization: Florida Institute of Technology

Education: Graduate College

Location: Melbourne, FL 32901

Question: We are considering purchasing a used Sorvall MT-5000 ultramicrotome, and would like some information about this particular model. It appears that the older MT-2 models are more widely used, and we would like to know if the MT-5000 is an instrument of as high as, or better quality than the MT-1 and 2 models. Can you also suggest one or more companies that can service either of these pieces of equipment in the state of Florida? Thank you very much for your assistance.

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From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 11:59:00 2004

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Has anybody tried direct scanning of glass microscope slides using
one
of the Nikon Coolscan series scanners? I would appreciate any comments or
experiences. Feel free to contact me directly.

Thank you!

George

George Laing
National Graphic Supply
ph 800.223.7130 x3109
f 800.832.2205
email scisales-at-ngscorp.com

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 12:57:45 2004

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Dear Vachik,

I worked in the area of precipitated silica powders and other
submicron particles and aggregates for many years. My TEM lab was closed
down in an ongoing restructuring and I am currently available for free
consulting while I find a new job in electron microscopy somewhere in the USA.

I probably ran 4,000+ samples of silica in the past. I assume you are
not talking about quartz particles but a higher tech material like a
manufactured silica.
First of all, what is the primary particle size of the silica that you
are trying to view or disperse? Is it a precipitated silica, a colloidal
silica, a clustered nanoparticle powder, a CMP silica, or what? Is it
agglomerated or aggregated? If it's aggregated or agglomerated, it has
pores and intergrowth can come into play with the surface area and
structural interpretation from supporting techniques outside microscopy.
Is the sample hydrophobic or hydrophilic?
The sample prep can depend on the degree of dispersion you want and if the
sample is hydrophilic or not.

Start with alcohol and water but you might have to switch to pure
alcohol for some level of dispersion. Some people use acidic water but
that can change the aggregate size. Stick to pure water, if you feel you
must use water with hydrophilic silicas. I suggest 100KV for submicron
primary particle sized silicas.

You didn't state the level of structure you are interested in. For
example, there are three basic types of silanols on the surfaces of things
like precipitated silica. These molecular structures and the near
molecular pores detected by nitrogen BET are not observable in a TEM.
Above those levels, the structures of silicas are directly observable in a
TEM. BET is made up of at least four different factors that are summed
together when used to characterize molecular pores and molecular roughness
in materials like ppt'd silica powders. BET can tell you about surface
area but determining the structural differences from that parameter
requires other techniques like TEM, for example. Argon, nitrogen and CTAB
surface areas could give totally different answers for surface area on the
same sample. TEM relates well to the mean surface volume diameter that you
can calculate from a CTAB surface area value or the MSVD that can be
determined in a TEM by image analysis and post analysis.

As for getting the samples run fast, have you tired to search the
membership list to see who might be located close to you? Most
professional microscopists would be willing to help you out at least once.
I would think JEOL in Boston could give you a complimentary real world
sample 'demo'. Call their salesman. Maybe you will buy a microscope
within the next few years and that kind of PR help should give JEOL the
inside track on a future purchase. Somebody in Boston will help you run
the sample(s). They/you can call me free for any help you might need with
the sample prep.

Sincerely,

Paul Beauregard
Senior Research Associate
Microscopy, Microtomy and Image Analysis
(724) 834-2247 (home)

}
} We need to view silica powder (SiO2) surface structure with an electron
} microscope. We are in a biological facility and have no experience with
} this type of sample. What sort of instrument is best suited for viewing
} this sample? What are the sample preparation techniques? Are there labs
} that we can bring our sample to for, let's say, an hour of observation and
} a few pictures? We are in the Boston, Massachusetts area. Thank you in
} advance.
}
} Vachik Hacopian
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 13:01:27 2004

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After much discussion last year (6/03) on this list
about problems with sticky tabs, I found
another source to replace Pella's tabs.
The earlier ones worked great but when I
re-ordered, the new Pella tabs were unacceptable.
They were stiff, not sticky and not conductive.
I wound up using EMS/Nissin.

I received a nice telecon from Ted Pella last
week asking if I would try their new tabs.
Of course I would like to. He sent them and
here are the results:

A B C
Original Pella 25K not meas. thin sticky
Re-order Pella open open stiff not very sticky
Newest Pella 10K 55K-200K thin sticky
EMS/Nissin 45K 112K-1.5M thin sticky
Fullam 20K 27K-500K thin sticky

A=initial resistance (Ohms)
B=overnight resistance; compressed (first value)-uncompressed
C=consistency of material

Tests were conducted using a pair of Pella 16242
pin stub mounts with a sample sticky tab sandwiched
in between. Resistance measurements were taken using
a Simpson #467 DVM. The initial resistance was taken
after pressing the stubs together. The overnight
resistance was taken the next day and was recorded
under two-hand compression and then after release
of compression. Resistance decreases under compression.

Another test comparison was done in the sputter
coater. I had noticed that different tabs were
differently affected by the coating experience.
The original Pella tabs would show small linear
cracks in the surface. The re-ordered tabs did
not show any evidence of surface effects but
were unusable due to non-conductance. The EMS/Nissin
tabs show circular and concentric circular deformations
at numerous locations on the tab. The Fullam tab
shows similar deformations. The new Pella tabs
appear to be affected in the same manner. I don't
think that any of these effects are killers. It is
just interesting and useful to note for comparison.

Pella's new 16084-1 replacement tab is definitely
a viable replacement. Thanks Ted.

Looking at the data I've taken, I conclude that
I'd rate Pella #1, Fullam #2, EMS/Nissin #3.
All are thin and sticky but the differentiation is
initial and final resistance (lower the better).
That said, it likely makes little difference in
operation since the specimen currents are so low.
At a high specimen current of say 10nA, using the
EMS/Nissin tab, the specimen could be about 15 mV
above ground. Not a big deal, IMO.

Therefore, the new Pella, EMS/Nissin and Fullan
tabs are all good tabs. The only remaining
discriminator is cost. The new Pella tabs are
$14.50/100.

Note that all three flavors of the Pella tabs have the
same 16084-1 part number. If you have any of the old
Pella tabs around (esp the hard ones), be sure your
techs check new tabs to be sure they are thin. If
you order new Pella tabs, there could be some confusion
as to which is which until all the old ones are used
or trashed.

gary g.

cc: Ted Pella, Tom Pella

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 15:28:52 2004

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Recently I tried examining some thin sections of fossil bone
(hydroxylapatite, R.I. around 1.6) and siderite (extreme birefringence, R.I.
from around 1.9 to about 1.6) using immersion oils that matched the R.I. of
the target mineral in the thin sections. This brought out lots of detail
missing with normal mounting media (nominally about R.I. 1.5). Out of
curiosity, does anyone know of some permanent mounting media that has an
index in the 1.6 - 1.8 range? I know high R.I. melts were used at one time,
but I seem to remember they were formulated with things like arsenic and
antimony (?).

Henry Barwood
Associate Professor of Science, Earth Science
Department of Math and Physics
MSCX 312G
Troy State University
Troy, Alabama 36082
hbarwood-at-troyst.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 2 18:48:13 2004

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There are number of old mounting media - I have a few -

Styrax
Hyrax
Styrene dissolved in methyl iodide
and the highest I know of - arsenic tribromide from Cargill - R.I. 2.31

Cargill makes (or made) Carmount in a range of R.I.s - I have three
different viscosities of some 1.65

Bill Miller

At 04:45 PM 4/2/2004, Henry Barwood wrote:

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From MicroscopyL-request-at-ns.microscopy.com Sat Apr 3 01:05:17 2004

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Hello Dr. Stefan

You can find such book in Earth Sciences Library, Geocentrum, next block
of your department or even at Sverige Geological Survey, SGU.
For a mutimedia of SEM&EDS , Oxford instrument has a CDROM set.

Hopefully you'll find it.

Paiboon

_______________________________________________
Paiboon Nuannin
Department of Physics
Facylty of Science
Prince of Songkla University
Hatyai
Thailand.
now on leave to
Deapartment of Earth Sciences
Geocentrum
Uppsala University
Villavagen 16
Uppsala, Sweden
_________________________________________________________

Quoting "Patton, David" {David.Patton-at-uwe.ac.uk} :

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} The book below is one of the first to have a section on low
} vacuum/ESEM.
}
} Dave
}
} 3rd Edition (2003)
} Scanning electron microscopy and X-ray microanalysis a text for
} biologists, materials scientists, and geologists Joseph I.
} Goldstein
} ... [et al]
}
}
}
} On Tue, 9 Mar 2004 11:28:33 +0100 Stefan Gunnarsson
} {Stefan.Gunnarsson-at-ebc.uu.se} wrote:
}
} }
} }
} }
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} -------------------------------------------------------------------------------
} }
} } Hi all!
} }
} } What textbooks and multimedia teaching aids for EM in general, SEM and
} } EDS in particular, would you recommend? I am especially looking for
} } those with (at least some) emphasis on low voltage FEG-SEM and low
} } vacuum techinques and theory.
} }
} } tia,
} } Stefan
} }
} } +++++++++++++++++++++++++++++++++++++++++++++++++++++++
} } Dr Stefan Gunnarsson
} } Evolutionsbiologiskt Centrum Evolutionary Biology Centre
} } Enheten för biologisk strukturanalys Microscopy and Imaging
Unit
} } Norbyvägen 18A
} } SE75236 Uppsala, Sweden Tel & Fax: +46 - 18 471
2638
} } +++++++++++++++++++++++++++++++++++++++++++++++++++++++
} }
}

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From MicroscopyL-request-at-ns.microscopy.com Sat Apr 3 09:39:10 2004

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Will the individual who posted a used TEM for sale recently please call
972-488-1414, ask for Leslie.

Thanks.

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 4 10:10:39 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kuwahara-at-ag.arizona.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, April 2, 2004 at 12:06:47
---------------------------------------------------------------------------

Email: kuwahara-at-ag.arizona.edu
Name: Sara Kuwahara

Organization: University of Arizona

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Greetings!

I'm looking for information about protocals and methods that would allow me to affix antibodies to a glass or silicon surface, but would leave the antibody freee to bind to its associated antigen. If you could direct me to any articles, procedues or texts it would be greatly appreciated.

*****note*****
I am not a memeber of this Listsever, so please respond to me directly.

Thank you

Sara Kuwahara

Dept of Ag and Biosystems Engineering
University of Arizona

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From MicroscopyL-request-at-ns.microscopy.com Sun Apr 4 10:11:26 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mingram-at-rohmhaas.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, April 2, 2004 at 14:16:11
---------------------------------------------------------------------------

Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Organization: Rohm and Haas

Title-Subject: [Microscopy] [Filtered] Wafer Cross Section Equipment

Question: I am looking for recommendations for 8-inch wafer cross section equipment. Please suggest.

Thanks

Mike Ingram
Rohm and Haas
Newark, DE

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 4 13:16:02 2004

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Hi, Mike

Check out SELA. They have been doing this sort of thing for a long time.

Caveat: MME has no financial interest in this product.

Best regards,
Barbara Foster
Microscopy/Microscopy Education, Inc. (MME, Inc.)
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Optimizing Light Microscopy is still available through MME. For information on ordering single or small quantities, visit our website. For discounts on classroom-sized, call us today.
^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&

At 10:27 AM 4/4/04 -0500, mingram-at-rohmhaas.com wrote:

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From MicroscopyL-request-at-ns.microscopy.com Sun Apr 4 15:11:47 2004

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Can you elaborate a bit about what you are trying
to do? I'm having trouble figuring out why
anyone would want to cross section a whole wafer
of any size. Typically, the individual die are
sliced out of the wafer and then cross sectioned
as a die. If the wafer is 8", then this strongly
suggests that the feature size is { 0.35u and would
be a likely candidate for FIB rather than mechanical
or fracture cross sectioning.

What are you trying to do?

gary g.

At 07:28 AM 4/4/2004, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Apr 5 06:07:34 2004

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hi all!

someone (ican't remember who) told me to use iridium...

Does anyone have informations about iridium (Ir) metallization coating
for FE-SEM observations of VLSI/ULSI microsectionned Si or AsGa dies,
instead of Au/Pd?

If so, can you detail the main differences in terms of performance :
granulometry, deposition process, conditions of the process (time
vaccum, which gas used...), cost... ?

d'avance merci!

Sylvain MAURY, de FRANCE

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 5 10:39:32 2004

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Dear Mike:

At South Bay Technology we can provide equipment and process information
to handle cleaving 8" wafers to preparing SEM and TEM cross-sections.
If you can supply me with more details on your application, I would be
pleased to send you information on the most appropriate solution.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

by way of MicroscopyListserver wrote:

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--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 5 13:55:09 2004

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Hi Sylvain,

Last year another research lab and I looked into an iridium high
resolution coater. I suggested Ir and someone else did the 'leg work'
evaluating the contender companies. Some manufacturers said they had Ir
but the only one that DELIVERED one to that lab last November was Emitech.

My retired old boss and I had a VCR Group micro sputter system that
was one of the original systems sold by Vince Carlino. Later, this
technology was sold and merged into South Bay and Vince worked for them.
(My take on the situation.) He retired and you should send him an email
because he contacted me about the Ir unit we were considering. He is very
very very knowledgeable and helpful.
Vince Carlino - Sales Manager
415-566-5774
Evactron.Com

Cressington says they have an Ir unit but I didn't see one on their
web page. Contact them too. A lady in Europe wrote me an email and said
she was getting one from Cressington shortly.

So you have the following four choices:
South Bay
EmiTech
Talking to Vince Carlino at Evactron.Com
and Cressington.

Vince can tell you where the original Ir idea came from in the US and
how the various metal high resoution coatings perform; Cr, Pt, and Ir.
He's a great guy to get in touch with about these coatings and knows the
strength and weakness of each of them.

Hope this helps,

Paul Beauregard
Senior Research Associate
Microscopy and Image Analysis

Disclaimer: I have no interest in any of these companies mentioned.

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 5 17:59:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (muchphoto-at-earthlink.net) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Monday, April 5, 2004 at 10:23:03
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Email: muchphoto-at-earthlink.net
Name: Michael Reese Much

Organization: Michael Reese Much Photographic Illustration

Education: Undergraduate College

Location: Bethlehem, PA

Question: I have recently purchased a microscope and have adapted it for digital photography. Could you recommend a good textbook about the preparation of specimen slides (staining, preparing protozoa for mounting and staining, etc.). I am also intereted in an atlas of protozoans.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 5 18:45:28 2004

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Hi-

This may be of NO use to you whatsoever, but when I heard that Ir gave a
smaller grain size, I bought some wire and wadded it up and put it in a
drilled-out carbon rod and deposited it with our (mostly unused) Balzers
400T freeze-fracture device (electron gun deposition). Worked great! More
complicated than a sputter coater, but we needed the resolution. I believe
Kent MacDonald's EM lab at Berkeley has a Balzers 300 that they have used
to coat for high-res SEM, using Pt. Again, kind of a pain, but if one of
these machines, used and about to be discarded, crosses your path... They
generally have a thickness monitor as well.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 5 23:51:49 2004

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muchphoto-at-earthlink.net (by way of Ask-A-Microscopist) wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (muchphoto-at-earthlink.net) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Monday, April 5, 2004 at 10:23:03
} ---------------------------------------------------------------------------
}
} Email: muchphoto-at-earthlink.net
} Name: Michael Reese Much
}
} Organization: Michael Reese Much Photographic Illustration
}
} Education: Undergraduate College
}
} Location: Bethlehem, PA
}
} Question: I have recently purchased a microscope and have adapted it for digital photography. Could you recommend a good textbook about the preparation of specimen slides (staining, preparing protozoa for mounting and staining, etc.). I am also intereted in an atlas of protozoans.
}
}
Hello Michael -
I am not familiar with a textbook about specimen slide preparation, especially at it concerns protozoa. However, I did extensive work with ciliates while I was pursuing my M.A. degree. I used basic microscopy techniques--that is, take a sample containing protozoa, put it on a slide, line the edges of the coverslip with vaseline (to act as a humid chamber), and then put it in a light microscope. About an atlas..the Society of Protozoologists (http://www.protozoa.uga.edu) (pretty sure) sells a book on protozoa called the Illustrated Guide To The Protozoa. I am unsure how the public can buy it, but perhaps if you visited that web site, you may be able to find some helpful information.
Good luck,
Nelson Conti

--
164 Ferne Court
Palo Alto, CA 94306
Home: (650) 494-0472
Cell: (650) 906-1159
Email: [ncontiSFSU-at-netscape.net]

__________________________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 01:15:26 2004

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Dear Mike:

We at South Bay Technology can help you with any of your
cross-sectioning requirements from cleaving an 8" wafer to making SEM
and TEM cross-sections. If you can narrow down your requirements a
little further, I'll be happy to direct you to our most appropriate
solution.

Best regards-

David

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 01:31:17 2004

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Dear Sylvain:

Paul Beauregard was correct in that Vince Carlino did some of the early
work on ion beam sputtered Ir films . In fact, I have a copy of a
paper by Cardinale, Carlino and Howitt titled "Comparison of Ion Beam
Sputtered Chromium and Iridium Films for Electron Microscopy
Applications" which I would be pleased to share with you.

Basically, the paper indicates that Ir produces very thin, extremely
fine grain, conductive coatings without the negative effects caused by
oxidation of chromium films. It is also of sufficiently high atomic
number to enhance electron scattering. Ir is routinely sputtered with
our IBS/e system and, in fact, is one of the standard targets supplied
with the system.

If you send me your maling address, I'll be pleased to send you a copy
of the paper. Paul Beauregard was correct in that the original
sputtering system (IBS/TM200) used in this analysis was acquired by
South Bay Technology back in 1999 when they purchased VCR Group. South
Bay Technology does continue to support The IBS/TM200 although a newer
generation Ion Beam Sputter Deposition and Etching System (IBS/e) has
been developed as well.

I have a fairly substantial library of technical papers covering ion
beam deposition as well as ion beam sources that I would be pleased to
share with anyone interested. Send me an email with your mailing
address and I'll send out the relevent papers.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

sylvain maury wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 07:49:36 2004

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Director of Microscopy and Imaging
University of Richmond

The Department of Biology at this highly selective, private, primarily
undergraduate university invites applications for a Director of
Microscopy and Imaging. Duties including supervising operation of a new
biological imaging facility, including operation and routine
maintenance of a TEM, SEM, and laser scanning confocal microscope and
associated equipment. Teaching responsibilities include training and
supervising faculty and student users in research and classroom
activities and courses based on interests and department needs;
assisting faculty and students in experimental design, specimen
preparation, digital photography, and analysis of results.

Qualifications: MS or PhD degree and experience with light and electron
microscopy and digital imaging, strong interpersonal skills and desire
and ability to work well in a team environment. This is a continuing
appointment that is not eligible for tenure but may include faculty
status.

Applications including a letter of interest, CV, evidence of expertise
in microscopy, and three letters of recommendation should be sent to
Dr. Gary Radice, Department of Biology, University of Richmond,
Richmond VA 23173 (gradice-at-richmond.edu). Review of applications will
begin on April 23, 2004. The appointment is expected to begin June 1,
2004.

The University of Richmond is committed to increasing the diversity of
our faculty and strongly encourages applications from women and
minorities. For more information on the department, resources, and
teaching assignment, see (http://biology.richmond.edu/)

Gary P. Radice gradice-at-richmond.edu
Department of Biology 804-289-8107 (voice)
University of Richmond 804-289-8233 (FAX)
Richmond VA 23173 http://www.richmond.edu/~gradice

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 08:51:01 2004

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A rather strange story read in the BBC online this morning.
A new chemical to become regulated in EM labs in the
US (after uranyl acetate)? Let's hope not!
{ http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 10:02:08 2004

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Available a Philips EM300 with goniometer and STEM, mecury free pump.

Instrument is Totaly Disambled in storage.

Entertaining Offers.

Thank You

Joseph Passero

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 10:33:30 2004

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I did a search on Amazon for "Illustrated Guide To The Protozoa" and
came up with a book by John Lee, which is out of print but they say
they have limited availability. Found several others from that search
as well including:
Marine Interstitial Ciliates: An Illustrated Key (Chapman & Hall
Identification Guide, No 2)
by Philip G. Carey (Hardcover - July 1992) (though it's a bit pricey)

Bettye

On Apr 5, 2004, at 10:06 PM, Nelson Conti wrote:

} Hello Michael -
} I am not familiar with a textbook about specimen slide preparation,
} especially at it concerns protozoa. However, I did extensive work with
} ciliates while I was pursuing my M.A. degree. I used basic microscopy
} techniques--that is, take a sample containing protozoa, put it on a
} slide, line the edges of the coverslip with vaseline (to act as a
} humid chamber), and then put it in a light microscope. About an
} atlas..the Society of Protozoologists (http://www.protozoa.uga.edu)
} (pretty sure) sells a book on protozoa called the Illustrated Guide To
} The Protozoa. I am unsure how the public can buy it, but perhaps if
} you visited that web site, you may be able to find some helpful
} information.
} Good luck,
} Nelson Conti
}
}
} --
} 164 Ferne Court
} Palo Alto, CA 94306
} Home: (650) 494-0472
} Cell: (650) 906-1159
} Email: [ncontiSFSU-at-netscape.net]
}
---------------
Bettye L. (Smith) Maddux
Dept. Biochemistry & Biophysics
ALS 2011
Oregon State University
Corvallis, OR 97330
Lab: 541.737.1870
Off: 541.737.8018
madduxb-at-onid.orst.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 12:07:30 2004

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The University of Chicago has a FEI (formerly Philips) CM120 for sale
for $15,000. The instrument is in excellent working condition and
includes a Haskris closed circuit water cooling system. For further
information contact

Robert Josephs
773 702 1077

186,000 miles a second -- it's not just a good idea -- it's the law

Bob Josephs

http://gingi.uchicago.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 13:06:31 2004

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Dear Researchers;
Our immunogold workshop in Madison, Wisconsin is being rapidly filled
up. If you are interested in attending, contact us asap. The
following is the original announcement, Thank you very much.

=======================

Immunogold Workshop Announcement

Dear Researcher:

      The Electron Microscopy Facility-Medical School at the University
of Wisconsin is hosting a three-day workshop on immunogold techniques
from May 24-26, 2004. Dr. Jan Leunissen from Aurion Immunogold Reagents
& Accessories, an internationally known expert in the field, will be
the instructor for the workshop. The workshop will include lectures,
hands-on training, round table discussions, and presentations on
applications. Also, participants of the workshop will be able to work
on their own samples during the workshop. The workshop main curriculum
is detailed below. If you are interested in attending or need more
information about the workshop, please contact the workshop technical
coordinator Hong Yi by phone (404-727-8692) or email (hyi-at-emory.edu).

MAIN CURRICULUM

The properties of gold particles and their protein conjugates.
Theories underlying immunogold labeling protocols.
Silver enhancement of gold particles
Immunogold labeling on a variety of sample preparations for LM.
Immunogold labeling for EM
a. Pre-embedding immunogold labeling using ultrasmall gold conjugates
and silver enhancement.
b. Post-embedding immunogold labeling using conventional colloidal gold
conjugates and   ultrasmalll gold conjugates.
Pre- and post-embedding double immunogold labeling.
Background minimization in immunogold labeling
Signal amplification in immunogold labeling.

Thanks and we hope to see you in Madison.

Randall Massey
Operations Manager
UW-Electron Microscope Facility
1300 University Ave.
Madison, WI 53706
voice (608)262-2993
Fax  (608)262-7306

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 15:38:24 2004

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This story was on ABC Evening News last night (Monday April 5) too.

Marc Pypaert wrote:

} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} A rather strange story read in the BBC online this morning.
} A new chemical to become regulated in EM labs in the
} US (after uranyl acetate)? Let's hope not!
} { http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }
}
} --
} Marc Pypaert
} Department of Cell Biology
} Center for Cell and Molecular Imaging
} Ludwig Institute for Cancer Research
} Yale University School of Medicine
} 333 Cedar Street, PO Box 208002
} New Haven, CT 06520-8002
} TEL 203-785 3681
} FAX 203-785 7446
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 18:19:15 2004

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They also could count sodium borhydride and other nasty staff from
laboratory shelves. Sergey

At 07:06 AM 4/6/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 18:34:13 2004

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Today, per request of NRL security, our chemical hygiene officer came by
my TEM lab to check that my small amount of osmium tetroxide was present
and secure.

} This story was on ABC Evening News last night (Monday April 5) too.

} Marc Pypaert wrote:

}
------------------------------------------------------------------------------

}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------

}
}
} A rather strange story read in the BBC online this morning.
} A new chemical to become regulated in EM labs in the
} US (after uranyl acetate)? Let's hope not!
} { http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }
}
} --
} Marc Pypaert
} Department of Cell Biology
} Center for Cell and Molecular Imaging
} Ludwig Institute for Cancer Research
} Yale University School of Medicine
} 333 Cedar Street, PO Box 208002
} New Haven, CT 06520-8002
} TEL 203-785 3681
} FAX 203-785 7446
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

--
_____________________________________________________
Tyrone L. Daulton
Director: Marine Geosciences - Electron Microscopy Facility
Physicist and Senior Electron Microscopist

Naval Research Laboratory
Marine Geosciences Division (Code 7400)
Stennis Space Center, MS 39529-5004

Voice (228)-688-4877
Fax (228)-688-4093
email tdaulton-at-nrlssc.navy.mil
tld-at-howdy.wustl.edu

http://www7430.nrlssc.navy.mil/facilities/emf/index.htm

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 19:01:17 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Mark Pypaert wrote:
=======================================================
A rather strange story read in the BBC online this morning.
} A new chemical to become regulated in EM labs in the
} US (after uranyl acetate)? Let's hope not!
} { http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }
=======================================================
Based on the sudden media interest in osmium tetroxide, I agree with Mark
that burdensome regulations could be placed on another important tool used
in electron microscopy.

As an industry, we should be developing standards for security for where
osmium tetroxide is being stored in a laboratory setting and suppliers
should be establishing standards not only for the storage of OsO4 in their
inventory, but procedures for the reporting of suspicious appearing
customers. SPI Supplies has had a long standing policy of selling only to
institutions (and not to individuals) but this approach "works" only so long
as our institutional customers keep materials such as osmium tetroxide in
secure locations and in ways that all of the material is accounted for (a
"cradle to grave" kind of accounting system). Shortages would have to be
explained just as is the case now for laboratories with a US federal tax-
free alcohol permit.

I fear that if we don't do this voluntarily and quickly, then regulations
will be forced upon us, and without the benefit of input from our industry
and this means that the costs of doing research will be increased, perhaps
substantially for the shipment and storing of osmium tetroxide.

It would seem to me that developing such standards would be a legitimate
role for MSA and other of the world's microscopy societies. But someone has
to take some leadership responsibility to start the ball rolling in that
direction so that as an industry, we can police ourselves and not have
governments dictate to us how it should be done.

Disclaimer: SPI Supplies has been a long time worldwide supplier of osmium
tetroxide to electron microscope laboratories.

Chuck

============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 19:46:23 2004

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Hi Sergey,

I note with interest that you keep your nasty staff on laboratory shelves, I would like to introduce a similar policy here in Australia. Cheers,

Mark Blackford
Materials and Engineering Science, ANSTO
PMB 1,
Menai, N.S.W., 2234
Australia

Phone 61 2 9717 3027
Fax 61 2 9543 7179

Disclaimer:
The views expressed in this E-mail message do not necessarily represent the official views of ANSTO from which this message was conveyed.

-----Original Message-----
} From: Sergey Ryazantsev [mailto:sryazant-at-ucla.edu]
Sent: Wednesday, 7 April 2004 9:35 AM
To: Microscopy-at-sparc5.microscopy.com

They also could count sodium borhydride and other nasty staff from
laboratory shelves. Sergey

At 07:06 AM 4/6/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 21:00:24 2004

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The sudden concern regarding osmium tetroxide probably relates to the
following

Poison gas attack foiled in Britain

07.04.2004
By KIM SENGUPTA
A planned poison gas attack, with the London underground system as a
likely target, has been foiled by the security agencies, it was claimed
today.

The plot, by British based supporters of al Qaeda, allegedly involved
detonating a combined chemical and explosive "dirty bomb", producing
fumes which can choke victims in a confined place.

The conspiracy was uncovered after British and United States
intelligence intercepted telephone calls within this country, as well as
calls to alleged senior members of the group in Pakistan.

As well as tube trains, passenger terminals at London's Gatwick and
Heathrow airports are believed to have been in the list of targets.
However, it is believed the plot was exposed before the alleged terror
cells had reached the position to carry out an attack.

Security sources said yesterday that the attack involved the use of a
chemical called osmium tetroxide to set off a blast.

The substance turns from solid to gas in confined space and is highly
corrosive to eyes, skin tissue and lungs, producing a symptom called
"dry land drowning." It is believed that a fertiliser-based explosive
would have been part of the package.

............

} -------------------------------------------------------------------------------
}
} A rather strange story read in the BBC online this morning.
} A new chemical to become regulated in EM labs in the
} US (after uranyl acetate)? Let's hope not!
} { http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }
}
} --
} Marc Pypaert
} Department of Cell Biology
} Center for Cell and Molecular Imaging
} Ludwig Institute for Cancer Research
} Yale University School of Medicine
} 333 Cedar Street, PO Box 208002
} New Haven, CT 06520-8002
} TEL 203-785 3681
} FAX 203-785 7446
}

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

Ian Hallett
HortResearch
Mt Albert Research Centre, Private Bag 92 169
Auckland, New Zealand
Fax +64 9 815 4201
Telephone +64 9 815 4200
EMail ihallett-at-hortresearch.co.nz

______________________________________________________
The contents of this e-mail are privileged and/or confidential to the
named recipient and are not to be used by any other person and/or
organisation. If you have received this e-mail in error, please notify
the sender and delete all material pertaining to this e-mail.
______________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 22:12:37 2004

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Having seen several listings of open positions on this list, I thought I
would post my CV and let people know that I am looking for positions in
microscopy. If anyone is interested, please let me know!

Here is my CV:

D. Scott Snyder
8100 Cambridge #103
Houston, TX 77054
(713)799-9165
dscottsnyder-at-earthlink.net

Education:
B. S., Chemistry, University of Idaho (1987)
Graduated with a 3.8 GPA

M. S., Biochemistry, Medical College of Wisconsin (1990)
Thesis: Interaction of Elongation Factor 3 from the Yeast S. cerevesiae
with Azido ATP:
Photoaffinity labeled ATP binding sit of EF-3; Proved specificity by
competitive enzyme inhibition, completeness of inactivation, stoichiometry,
and kinetics of inactivation
Coursework: Molecular Genetics, Protein Chemistry, Enzyme Mechanics,
Medical Biochemistry, Physical Methods of Biochemistry
Rotations: Purification of ubiquitin, enzyme isolation and analysis,
affinity labeling of enzyme active sites, western screening for elongation
factor 3 clones

Ph. D., Cell Biology with certification in Biological Chemistry, Duke
University, 2000
Mentor: Thomas J. McIntosh
Dissertation: Structure and Antibiotic Permeability of Bacterial
Lipopolysaccharide Bilayers – Determined microbial membrane bilayer
structure with XRD, DSC and other analytical techniques then correlated
structure with permeability as determined by stopped flow fluorimetry and
spectroscopic methods
Coursework: Advanced Molecular Biology, Analytical Spectroscopy,
Stereochemistry, Cell Biology, Cell Signaling, Bioorganic Chemistry,
Genetics
Rotations: Lipid A biosynthesis, Lab of Christian Raetz
LPS Vaccine formulation, Lab of Thomas McIntosh and MDT, Inc.

Experience
Lab Manager, Integrated Microscopy Core, Baylor College of Medicine,
Houston, TX
Responsible for developing new techniques in microscopy such as FRET, FLIP
and spectral imaging applications, training users, maintaining equipment,
grant writing to obtain new equipment and general managerial duties in
regional microscopy facility. Also involved in research project involving
estrogen receptor based signal transduction.

Researcher and Confocal Systems Manager, National Institutes of Health,
Rocky Mountain Laboratories, Hamilton MT
Responsible for independent research examining the inflammatory response
of cultured mammalian cells in response to the TLR2 lipoprotein ligand OspA
and the internalization of OspA in such cells. Techniques involved NF
kappa B localization assays, as well as TNF and IL-1 ELISAs and extensive
live cell confocal microscopy. Also responsible for managing confocal
facility.
Post Doctoral Fellow, National Institutes of Health, Rocky Mountain
Laboratories, Hamilton MT (2000-2001)
Project involved determining the mechanism of action of mycolactone, a
toxin derived from Mycobacterium ulcerans which is capable of eliminating
the inflammatory response as well as inducing cytoskeletal rearrangement
and apoptosis in a variety of cell types and is required for virulence in
vivo. Techniques involved isolation, derivatization and analysis of
mycolactone, mass spectroscopy, cell culture, inhibition of various cell
signaling pathways, confocal microscopy, examination of calcium release
from the endoplasmic reticulum and apoptosis assays.

M.S. Level Research Associate for Ribi Immunochem Inc., Hamilton, MT
(1990-1995)
Developed GLP methods for the isolation, fractionation, derivatization and
analysis of lipid based inflammatory mediators using HPLC, LC, GC, TLC,
NMR, UV/VIS and wet chemical methods
Fluorescently labeled and analyzed the cell localization patterns of
inflammatory mediators
Refined lab bench procedures for industrial setting (scale-up)
Developed novel analytical methods for GMP adjuvants and vaccines
Assayed effects of inflammatory mediators and derivatives on cell cultures
and in animal models using both the ELISA and NO assays
Interviewed and trained research technicians
Conducted facility tours for investors, lawmakers and the public
Received 3 raises and 1 promotion in this position

Other Advanced Training:
HPLC Method Development: Lloyd Snyder and John Dolan (LC Resources)
HPLC Troubleshooting and Repair: Waters Corporation
Interpretation of Mass Spectra: American Chemical Society
Advanced Topics in Live Cell Imaging: University of Connecticut Health
Sciences Center

Publications
SR Hagen, JD Thompson, DS Snyder and KR Myers, Analysis of a Monophosphoryl
Lipid A Immunostimulant Preparation from Salmonella R595 by HPLC, Journal
of Chromatography, 767 (1997) pages 53-61

DS. Snyder, D Kim and TJ. McIntosh, LPS Bilayer Structure: Effect of
Chemotype, Core Mutations, Divalent Cations and Temperature, Biochemistry,
v38, number 33 (1999) pages 10758-10767

K Kulkarni, DS Snyder, and TJ McIntosh, Adhesion Between Cerebroside
Bilayers, Biochemistry, v38, number 46, (1999) pages 15264-15271

DS Snyder and TJ. McIntosh, The LPS Permeability Barrier: Correlation of
Antibiotic Permeabilities with Antibiotic Susceptibilities and Fluorescent
Probe Binding Kinetics Biochemistry, v39, number 38 (2000) pages 11777-87

EB Guererro, TJ McIntosh, GR Barclay, DS Snyder, RJ Gibbs, MG Mythen and IR
Poxton, Preparation and Preclinical Evaluation of a Novel Liposomal
Complete Core Lipopolysaccharide Vaccine, Infection and Immunity, v68
number 11 (2000) pages 6202-8

DS Snyder and PLC Small, Staining of Cellular Mitochondria with LDS-751,
JIM, v257 (2001) pages 35-40

DS Snyder and PLC Small, Uptake and cellular actions of mycolactone, a
virulence determinant for Mycobacterium ulcerans. Microb Pathog. 2003
Feb;34(2):91-101.

DS Snyder and CF Garon Decreased uptake of bodipy-labelled compounds in the
presence of the nuclear stain, DRAQ5.J Microsc. 2003 Sep;211(Pt 3):208-11.

D Welty, DS Snyder. Internalization of OspA in rsCD14 complex and
aggregated forms.
Mol Microbiol. 2003 Nov;50(3):835-43.

KA Jackson, DS Snyder, MA Goodell, Stem Cell Engraftment: Distinguishing
GFP from Autofluorescence. Stem Cells. 2004;22(2):180-7

Patents
Vaccine Against Lipopolysaccharide Core, Application # WO 98/51217 by
Elliott Bennett Guererro, George Robin Barclay, Ian Raymond Poxton, Thomas
James McIntosh and David Scott Snyder (pending)

Method for the Production of 3 O Deacylated 4’ Monophosphoryl Lipid A Kent
Myers and Scott Snyder (pending)

Invited Presentations

A Tale of Two Ligands University of North Texas Health Sciences Center at
Fort Worth, April 2002

Abstracts
DS Snyder, KL Whitaker and KR Myers, Structural and Biological
Characterization of Unmodified Re Lipopolysaccharide by Normal Phase
Chromatography 1995 FASEB meeting

DS Snyder and TJ McIntosh, Bacterial Antibiotic Susceptibility and
Lipopolysaccharide Structure/Permeability, 1999 International Endotoxin
Society Meeting

Scholarships, Honors and Awards
Richard Asofsky Award for Special Achievement in Equal Employment
Opportunity, Hoggsey-Cossey Award, WMA Scholarship, Whitman E Scholarship,
5th Marine Division Scholarship, others available upon request

References
Thomas J. McIntosh, Mentor, Phone (919) 684-8950, e-mail
mcint001-at-mc.duke.edu
Kent Myers, Supervisor at Ribi, Phone (406) 363-6214, e-mail
kmyers-at-corixa.com
Elliott Bennett Guererro, Director Cardiothoracic Anesthesia, Columbia
University and President of MDT, Inc (212) 996-8234, e-mail
elliott_guererro-at-smtplink.mssm.edu
Pam Small, Supervisor at NIH, Phone (865) 974-4042, e-mail psmall-at-utk.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 6 23:29:33 2004

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Reminder to Everyone

Posting of Resumes/ CVs to the listserver is strictly against our rules and has been so for
more than a decade!

Please review the rules and/or the FAQ pages, a copy of which everyone automatically
receives with their subscription confirmation.

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 08:07:40 2004

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The videos of the Tutorials presented at the 2003 MSA meeting in
San Antonio are now available. See the current catalog at this URL:
http://www.biotech.ufl.edu/sems/newtape00.htm
All new titles are available on DVD only. Some VHS tapes of old
titles remain. We are no longer producing any new tapes.
This is a continuing service of the Education Committee of the Microscopy
Society of America.
Contact me to order.

Greg Erdos

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 08:32:10 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (dmwilliams-at-dow.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 7, 2004 at 08:15:27
---------------------------------------------------------------------------

Email: dmwilliams-at-dow.com
Name: David M. Williams

Organization: The Dow Chemical Company

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have a good fixative formula for whole body perfusions of rats? I am primarily interested in getting optimal fixation of the periferal nerves for optical and possibly TEM examination. Thank you.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 09:11:35 2004

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Well yes! It opens up a whole new sphere for bureaucratic interference. But
surely, OsO4 is so expensive that each lab knows exactly where every
microgram is.

Lesley Weston.

on 06/04/2004 4:34 PM, Sergey Ryazantsev at sryazant-at-ucla.edu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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--} -
}
} They also could count sodium borhydride and other nasty staff from
} laboratory shelves. Sergey
}
} At 07:06 AM 4/6/2004, you wrote:
}
}
} }
----------------------------------------------------------------------------
-} } -
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
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} } -----------------------------------------------------------------------------
} } --
} }
} } A rather strange story read in the BBC online this morning.
} } A new chemical to become regulated in EM labs in the
} } US (after uranyl acetate)? Let's hope not!
} } { http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }
} }
} } --
} } Marc Pypaert
} } Department of Cell Biology
} } Center for Cell and Molecular Imaging
} } Ludwig Institute for Cancer Research
} } Yale University School of Medicine
} } 333 Cedar Street, PO Box 208002
} } New Haven, CT 06520-8002
} } TEL 203-785 3681
} } FAX 203-785 7446
} }
}
} _____________________________________
}
} Sergey Ryazantsev Ph. D.
} Electron Microscopy
} UCLA School of Medicine
} Department of Biological Chemistry
} 10833 Le Conte Ave, Room 33-089
} Los Angeles, CA 90095
}
} Phone: (310) 825-1144 (office)
} (310) 206-1029 (Lab)
} FAX (departmental): (310) 206-5272
} mailto:sryazant-at-ucla.edu
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 09:33:21 2004

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I was hoping someone could point me in the right direction for finding out
about average salaries Electron Microscopist. The average salary for
Electron Microscopists just starting out of college with a B.S. and one
with several years of experience.

Thank you very much

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 10:09:30 2004

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hello everyone!

Maybe it's not correct to ask this, but does anyone know the email
adress of Linda DAILEY of EMITECH Products Inc. ?

I have to ask her some questions about SEM Sputter coating...

d'avance merci...

Sylvain MAURY, de France ! cocorico! ;-)

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 10:59:00 2004

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Hi all
I agree with these sentiments about developing our own standards,
especially as we have the most to gain from this. Maybe we can
discuss this at the meeting in Savannah in August for the MSA and in
Wolfville, Nova Scotia, Canada in May for the MSC meeting. I would
like to be part of this policy making.
Elaine

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 11:30:51 2004

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Colleagues:
Our Bio-Imaging facility has merged with our E-M facility and I now have
a Hitachi TEM under my care. Can any one recommend a basic introductory
course in electron microscopy. It would be preferable if it was near New
York City, or at least in the North East.
Thanks

Lloyd Williams

Manager Bio-Imaging Facility
Hunter College
695 Park Ave
New York, NY 10021

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 11:53:39 2004

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Hello,

We have Leica inverted (DMIRE2) and upright
(DMRXA2) microscopes in our Confocal facility that we would
like to add live cell imaging capabilities to. At the
moment, a heating stage would be adequate. If you are
using such a stage (even on a different brand
microscope) and are really happy with it, would you please
share the manufacturer with me?

Thank you in advance,

Doug

----------------------
Douglas R. Keene
Associate Investigator
Micro-Imaging Center
Shriners Hospital for Children
3101 S.W. Sam Jackson Park Road
Portland, Oregon 97239-3009
phone: 503-221-3434
FAX: 503-412-6894

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 12:10:57 2004

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Hello,

I am wanting to localize GFP within cultured fibroblasts at
the ultrastructural level (TEM). We are using anti-GFP
antibodies provided by Rockland and another provided by
Assay Design. We have tried a variety of protocols using
prefixation in 0.1% glut and/or rendering the cells
permeable with 0.01% saponin. We've also prefixed the
cells with 100% methanol (this results in reasonable
labeling density but terrible ultrastructure). Our typical
protocol utilizes colloidal gold conjugated secondary
antibodies.

In any of these protocols I have tried, I am either not
satisfied with the preservation of the cells or I am not
satisfied with labeling density. Certainly not an unusual
quandary for immuno-EM, but surely there is a more
satisfactory protocol than the ones I have tried!

My question: Does anyone use a TEM protocol for
intracellular labeling that they are happy with?

Many thanks,

Doug

----------------------
Douglas R. Keene
Associate Investigator
Micro-Imaging Center
Shriners Hospital for Children
3101 S.W. Sam Jackson Park Road
Portland, Oregon 97239-3009
phone: 503-221-3434
FAX: 503-412-6894

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 12:35:47 2004

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I agree with the concerns about 0s04. We also must limit our sales to U.S.
agencies, institutions, some industries and other vendors who understand the
procedures required when chemicals are involved.

Internally we limit access to all our stains, fixatives, epoxies, etc., even
those that are not hazardous. We have close to 50 years experience in
handling a wide range of chemicals so if anyone needs any assistance that we
might be able to provide please contact us.

Disclaimer: Ladd is a manufacturer and worldwide distributor of
EM/Laboratory supplies and chemicals such as Osmium tetroxide.

John Arnott

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 12:39:58 2004

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It is specific to electron microprobe labs and their managers/technicians,
but the following report is available on-line:

Survey of User Fees, Laboratory Support, and Operator Salaries in Electron
Microprobe Laboratories

http://research.ou.edu/microprobe/feesurv.pdf

Hope it helps,

Ellery

---------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
Department of Geology & Geophysics
University of Minnesota - Twin Cities
Lab Website: http://probelab.geo.umn.edu

On 7 Apr 2004, kathy lowe wrote:
} I was hoping someone could point me in the right direction for finding
out
} about average salaries Electron Microscopist. The average salary for
} Electron Microscopists just starting out of college with a B.S. and one
} with several years of experience.
}
} Thank you very much

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 13:24:16 2004

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List members,

By way of background, some of you may recall that there was a meeting of
Facility Managers at M&M 2003. The intent to form a formal group to discuss
problems such as this one concerning osmium tetroxide as well as many other
issues of major interest to facility managers and also of interest to all EM
users. The request to form a Focused Interest Group was denied by the MSA
Council for reasons that have not yet been fully explained but hopefully
will be soon. However, we still hope to meet as a group at M&M2004. I was
elected to serve as chair of the group at M&M 2003.

Perhaps this is where the facility manager's group can be of assistance.
This would be a reasonable topic for discussion if we meet at M&M2004
providing the MSA council does not want to act prior to that time. I could
envision our putting together a draft proposal that would then go to the MSA
Council for their discussion/ revision followed by a formal policy statement
at the winter council meeting. Does this seem reasonable? Would the
Facility Managers like to be involved with this issue?

Please get back to me and I will try to act accordingly.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 4/7/04 11:14 AM, "Elaine Humphrey" {ech-at-interchange.ubc.ca} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Hi all
} I agree with these sentiments about developing our own standards,
} especially as we have the most to gain from this. Maybe we can
} discuss this at the meeting in Savannah in August for the MSA and in
} Wolfville, Nova Scotia, Canada in May for the MSC meeting. I would
} like to be part of this policy making.
} Elaine
}
}
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} }
} } Mark Pypaert wrote:
} } =======================================================
} } A rather strange story read in the BBC online this morning.
} } } A new chemical to become regulated in EM labs in the
} } } US (after uranyl acetate)? Let's hope not!
} } } { http://news.bbc.co.uk/go/em/fr/-/1/hi/uk/3603961.stm }
} } =======================================================
} } Based on the sudden media interest in osmium tetroxide, I agree with Mark
} } that burdensome regulations could be placed on another important tool used
} } in electron microscopy.
} }
} } As an industry, we should be developing standards for security for where
} } osmium tetroxide is being stored in a laboratory setting and suppliers
} } should be establishing standards not only for the storage of OsO4 in their
} } inventory, but procedures for the reporting of suspicious appearing
} } customers. SPI Supplies has had a long standing policy of selling only to
} } institutions (and not to individuals) but this approach "works" only so long
} } as our institutional customers keep materials such as osmium tetroxide in
} } secure locations and in ways that all of the material is accounted for (a
} } "cradle to grave" kind of accounting system). Shortages would have to be
} } explained just as is the case now for laboratories with a US federal tax-
} } free alcohol permit.
} }
} } I fear that if we don't do this voluntarily and quickly, then regulations
} } will be forced upon us, and without the benefit of input from our industry
} } and this means that the costs of doing research will be increased, perhaps
} } substantially for the shipment and storing of osmium tetroxide.
} }
} } It would seem to me that developing such standards would be a legitimate
} } role for MSA and other of the world's microscopy societies. But someone has
} } to take some leadership responsibility to start the ball rolling in that
} } direction so that as an industry, we can police ourselves and not have
} } governments dictate to us how it should be done.
} }
} } Disclaimer: SPI Supplies has been a long time worldwide supplier of osmium
} } tetroxide to electron microscope laboratories.
} }
} } Chuck
} }
} } ============================================
} } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } President 1-800-2424-SPI
} } SPI SUPPLIES FAX: 1-610-436-5755
} } PO BOX 656 e-mail:cgarber-at-2spi.com
} } West Chester, PA 19381-0656 USA
} } Cust.Service: spi2spi-at-2spi.com
} }
} } Look for us!
} } ########################
} } WWW: http://www.2spi.com
} } ########################
} } ============================================

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 13:27:28 2004

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test

186,000 miles a second -- it's not just a good idea -- it's the law

Bob Josephs

http://gingi.uchicago.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 13:30:20 2004

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The New England Society for Microscopy and the Connecticut Microscopy
Society announce the annual Spring Symposium, preceded by a workshop on
Image Analysis using LISPIX, presented by Dr. David Bright (NIST). The
workshop and symposium will be held April 29th. - May 1st. 2004, at the
Marine Biological Laboratory, Woods Hole, Massachusetts.

Full details of both events, including registration information, are
available on the NESM Web site, accessible at
{http://www.msa.microscopy.com/MSALAS/NESM/NESMHome.htm} http://www.msa.microscopy.com/MSALAS/NESM/NESMHome.htm

***********************************************
Anthony J. Garratt-Reed, M.A., D.Phil.
MIT Room 13-1027
77 Massachusetts Avenue
Cambridge, MA 02139-4307
USA

Tel: 617-253-4622
Fax: 617-258-6478
************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 14:41:22 2004

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Lloyd wrote...

Colleagues:
Our Bio-Imaging facility has merged with our E-M facility and I now have
a Hitachi TEM under my care. Can any one recommend a basic introductory
course in electron microscopy. It would be preferable if it was near New
York City, or at least in the North East.
Thanks

Lloyd Williams

Dear Lloyd:

Dr. Hayat used to teach a course at Kean College of New Jersey ( I think it is Kean University, now). It is located in Union, New Jersey; and not too far from NYC.

Also, Montclair State University (in Montclair, New Jersey) used to have an EM course years ago. I don't know if they still offer it.

Finally, Lehigh University in Pennsylvania offers EM mini-courses/workshops (usually held in the summer).

I hope this helps.

Good Luck,

Jackie

------------------------------
Jacqueline Garfield,
Electron Microscopist
Research & Development
Lifecell Corporation
One Millennium Way
Branchburg, NJ 08876
(908) 947-1182

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Hi everyone:
I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of a
series of holes within micron (or ideally submicron) accuracy on a strip
of metal that has been laser holes drilled into.

I hope to achive this by using the change in z from the top and the
bottom of hole using a calibrated stage. Does anyone out there have a
device that they had made or purchased at a reasonable price. Are you
willing to share your drawings/expertise?
Thanks,
Michael Coviello
UT Arlington

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} } They also could count sodium borhydride and other nasty staff from
} } laboratory shelves.

Dear List,
I wonder just how toxic a "dirty bomb" using OsO4 would actually be.
The conditions of an explosion often are hypoxic, so OsO4 could be
reduced to a non-toxic state. On the other hand, the presence of OsO4
could enhance combustion in the explosion making it more powerful.
Maybe those attempting to test such a bomb would then be killed in
their own, surprisingly large explosion. If we're very lucky, they
might try to make a really dirty bomb using both OsO4 and NaBH4.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 15:24:03 2004

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Doug,

I have had good luck locating various GFP constructs in COS-7 cells
using this general technique;

Fix in 4% paraformaldehyde
Quench with .1% NaBH4
Permeablize with .1% Triton x-100
Block
Molecular Probes' polyclonal anti GFP
Aurion GAR ultra small immuno gold
Silver enhancement
Convention fixation and embedment

Let me know if you want a detailed protocol.

Cheers,

Tom

-----Original Message-----
} From: drk-at-SHCC.org [mailto:drk-at-SHCC.org]
Sent: Wednesday, April 07, 2004 12:26 PM
To: Microscopy-at-sparc5.microscopy.com

Hello,

I am wanting to localize GFP within cultured fibroblasts at
the ultrastructural level (TEM). We are using anti-GFP
antibodies provided by Rockland and another provided by
Assay Design. We have tried a variety of protocols using
prefixation in 0.1% glut and/or rendering the cells
permeable with 0.01% saponin. We've also prefixed the
cells with 100% methanol (this results in reasonable
labeling density but terrible ultrastructure). Our typical
protocol utilizes colloidal gold conjugated secondary
antibodies.

In any of these protocols I have tried, I am either not
satisfied with the preservation of the cells or I am not
satisfied with labeling density. Certainly not an unusual
quandary for immuno-EM, but surely there is a more
satisfactory protocol than the ones I have tried!

My question: Does anyone use a TEM protocol for
intracellular labeling that they are happy with?

Many thanks,

Doug

----------------------
Douglas R. Keene
Associate Investigator
Micro-Imaging Center
Shriners Hospital for Children
3101 S.W. Sam Jackson Park Road
Portland, Oregon 97239-3009
phone: 503-221-3434
FAX: 503-412-6894

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 16:11:12 2004

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Lloyd,

Lehigh University in Bethlehem, PA is your closest bet for a formal course
in TEM. I took that course and another one years ago in Boston. It's very
good, near you and has very good instructors.

Try www.lehigh.edu/microscopy for information and course times.
(610) 758-5133

Sincerely,

Paul Beauregard
Senior Research Associate
Microscopy and Image Analysis

At 12:48 PM 04/07/04 -0400, Lloyd Williams wrote:
}
}
} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 16:29:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kcarson-at-odu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 7, 2004 at 13:47:34
---------------------------------------------------------------------------

Email: kcarson-at-odu.edu
Name: Keith Carson

Organization: Old Dominion University

Title-Subject: [Microscopy] [Filtered] digitizing TEM negatives

Question: I am looking for suggestions on equipment and settings to digitize TEM negatives and produce high quality hard copies from the digital image files.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 16:36:46 2004

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Dear Debby
There is no need to discuss (and provoke therefore) the issue, which does
not exist as a scientific matter (are we scientists or
politicians?). There are plenty of strict regulations which are already
enforced. It's ridiculous, we spent time for such matters. I think, we
should keep this place out of political issues. Unsuccessful OsO4 attack in
England IS a political matter, not scientific. Sergey

At 11:39 AM 4/7/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 17:08:22 2004

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Have you tried frozen ultrathin sections (the Tokuyasu method)?
This is the ultimate method for this kind of work.
Alternatively, you could use lowicryl or similar type of
hydrophilic resins. Maybe combined with high-pressure
freezing and freeze-substitution for better preservation
of morphology.

For the labeling, I have never tried anti-GFP antibodies
from Rockland, but I have great results with antibodies
from Molecular Probes. Also, we have stopped using
gold-conjugated secondary antibodies as these do not
always give great labeling efficiency. We prefer to use
protein A-gold instead. You might want to try.
Best

Marc

On Wednesday, April 7, 2004, at 01:26 PM, Doug Keene wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Hello,
}
} I am wanting to localize GFP within cultured fibroblasts at
} the ultrastructural level (TEM). We are using anti-GFP
} antibodies provided by Rockland and another provided by
} Assay Design. We have tried a variety of protocols using
} prefixation in 0.1% glut and/or rendering the cells
} permeable with 0.01% saponin. We've also prefixed the
} cells with 100% methanol (this results in reasonable
} labeling density but terrible ultrastructure). Our typical
} protocol utilizes colloidal gold conjugated secondary
} antibodies.
}
} In any of these protocols I have tried, I am either not
} satisfied with the preservation of the cells or I am not
} satisfied with labeling density. Certainly not an unusual
} quandary for immuno-EM, but surely there is a more
} satisfactory protocol than the ones I have tried!
}
} My question: Does anyone use a TEM protocol for
} intracellular labeling that they are happy with?
}
} Many thanks,
}
} Doug
}
} ----------------------
} Douglas R. Keene
} Associate Investigator
} Micro-Imaging Center
} Shriners Hospital for Children
} 3101 S.W. Sam Jackson Park Road
} Portland, Oregon 97239-3009
} phone: 503-221-3434
} FAX: 503-412-6894
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 17:11:53 2004

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I recommend the Lehigh short course at Lehigh University this June. Check out
http:// www.lehigh.edu/microscopy for more information.

Lloyd Williams wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Colleagues:
} Our Bio-Imaging facility has merged with our E-M facility and I now have
} a Hitachi TEM under my care. Can any one recommend a basic introductory
} course in electron microscopy. It would be preferable if it was near New
} York City, or at least in the North East.
} Thanks
}
} Lloyd Williams
}
} Manager Bio-Imaging Facility
} Hunter College
} 695 Park Ave
} New York, NY 10021

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 7 19:28:39 2004

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Sergey;
I wish you were right, but I think you can be sure that some
knee-jerk bureaucratic bungler will make life miserable for everyone
that uses osmium tetroxide in their research. Just remember the weapons
of mass deception.....

John Mardinly

-----Original Message-----
} From: Sergey Ryazantsev [mailto:sryazant-at-ucla.edu]
Sent: Wednesday, April 07, 2004 2:53 PM
To: Microscopy-at-sparc5.microscopy.com

Dear Debby
There is no need to discuss (and provoke therefore) the issue, which
does
not exist as a scientific matter (are we scientists or
politicians?). There are plenty of strict regulations which are already

enforced. It's ridiculous, we spent time for such matters. I think, we

should keep this place out of political issues. Unsuccessful OsO4 attack
in
England IS a political matter, not scientific. Sergey

At 11:39 AM 4/7/2004, you wrote:

} -----------------------------------------------------------------------
-------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 01:31:01 2004

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Hi,
it might be better to use a piezo driven objective
positioner. This guarantees a higher precision and
repeatability than a motorized Z-stage.

mfg / regards

Anneliese Schmaus

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

c} ------------------------------------------------------------------------------
c} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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c} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
c} -------------------------------------------------------------------------------

c} Hi everyone:
c} I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of a
c} series of holes within micron (or ideally submicron) accuracy on a strip
c} of metal that has been laser holes drilled into.

c} I hope to achive this by using the change in z from the top and the
c} bottom of hole using a calibrated stage. Does anyone out there have a
c} device that they had made or purchased at a reasonable price. Are you
c} willing to share your drawings/expertise?
c} Thanks,
c} Michael Coviello
c} UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 02:27:13 2004

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hi everyone!

does anyone have some informations, or some theory about the charging
phenomenon of SEM ?

I know it's because of the secondary electrons yield, producing a dark
rectangle on image, when setting a too low voltage (low electron energy)
, and a bright one, appearing like a false relief, at a too high voltage
(high electron energy). But, is that all?

Where can i find a good bibliography?

thanx.

Sylvain

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 05:53:47 2004

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I'm very, very worried about this topic. If this topic is treated as a
political matter, it will make the life of researches that work in
developmental countries, like me, extremely difficult. We depend on
importation to do our research and it is already hard enough to obtain some
drugs without the absurd regulations that emerge from time to time due to
the politics ignorance and paranoid in what concerns to the scientific
matters. It is not rules that will stop terrorists to acquire material that
may be used in attacks because these people do not obey rules. They obtain
their material in the black market.

As an example, I had to stop working with the effect of aflatoxin in
tropical fishes, a serious problem in Brazil, because it became almost
impossible to buy the product after some menace of its use by terrorist.
Before the application of absurd regulations by the US government, it could
take six months to receive the product, now it takes almost two years, after
several formularies are filled. Now, I have colleagues that had to agree to
received US inspectors in their laboratories asking if they have contact
with terrorist groups because they want to buy 10 mg of aflatoxin.

Prof. Dr. Francisco Javier Hernandez Blazquez
University of Săo Paulo
Fac. Veterinary Medicine and Animal Sciences
Departament of Surgery - Sector of Anatomy
Av. Prof. Dr. Orlando Marques de Paiva, 87
05508-000 - Săo Paulo (SP) - Brasil
Tel..55 (11) 3091 1374 Fax 55 (11) 3091 7805
email: fjhblazq-at-usp.br

----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
To: {Microscopy-at-sparc5.microscopy.com}
Sent: Wednesday, April 07, 2004 6:52 PM

Hi, all,

I am looking for an EM and Imaging Lab manager for my lab immediately, at Agriculture and Agri-Food Canada in Kentville, Nova Scotia Canada. Please visit the following website:

http://www.jobs.gc.ca/jobs/p032847e.htm

for more information and instructions for applying.

Kind regards,

Paula.

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 07:14:02 2004

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Hi Folks,
I tend to agree with Bill Tivol about the use of osmium tetroxide in a
'dirty bomb'. If you consider how reactive the compound is, I would think
that the chances of OsO4 actually surviving the delivery explosion in that
toxic form would be minimal (a common problem with chemical weapons). It
reacts quickly with a variety of things, so the combustion products from an
explosion would be likely to change the situation to more of a heavy metal
issue than a toxic gas problem. If you look at the way the concept has been
presented in the media (especially in the US) there is more emphasis on the
fear factor than on the science.

Cheery thoughts for the morning,
Robert Simmons

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 07:20:06 2004

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Michael;

Sounds like an AFM [Atomic Force Microscope] may do what you need. The reasonable price part is another matter but you need to define "reasonable."

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: coviello [mailto:coviello-at-mae.uta.edu]
Sent: Wednesday, April 07, 2004 6:10 PM
To: Microscopy-at-MSA.Microscopy.Com

Hi everyone:
I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of a
series of holes within micron (or ideally submicron) accuracy on a strip
of metal that has been laser holes drilled into.

I hope to achive this by using the change in z from the top and the
bottom of hole using a calibrated stage. Does anyone out there have a
device that they had made or purchased at a reasonable price. Are you
willing to share your drawings/expertise?
Thanks,
Michael Coviello
UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 08:05:13 2004

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Hi There,
I am of need for repair/service on our two PIPS and two DUO-mills from Gatan. Are there any independent service persons that are experts in dealing with these tools? If so, could you please contact me off list to discuss the details. I would like to explore independent route before I ship them to Gatan-Warrendale for repairs.

Thanks,

Jerzy

******************************************************
Jerzy Gazda, Ph.D. Advanced Micro Devices
Supervising Engineer 5204 E. Ben White Blvd. - MS 512
PCAL - AIM Section Austin, TX 78741
TEL: 1-800-538-8450, Ext. 51453
jerzy.gazda-at-amd.com
******************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 08:15:00 2004

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Hi Folks,
I tend to agree with Bill Tivol about the use of osmium tetroxide in a
'dirty bomb'. If you consider how reactive the compound is, I would think
that the chances of OsO4 actually surviving the delivery explosion in that
toxic form would be minimal (a common problem with chemical weapons). It
reacts quickly with a variety of things, so the combustion products from an
explosion would be likely to change the situation to more of a heavy metal
issue than a toxic gas problem. If you look at the way the concept has been
presented in the media (especially in the US) there is more emphasis on the
fear factor than on the science.

Cheery thoughts for the morning,
Robert Simmons

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 08:43:44 2004

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Michael, if you can't find a light microscope to suit
your needs, most metallographs that I've used have a
focus knob with scales graduated down to 1 micron.
Coupled with the extremely low depth of field, it can
make rather accurate depth measurements by focusing on
each plane and measuring the difference. I haven't
used it enough to judge the practical accuracy of this
technique. It serves us well to measure depth of
corrosion pits in metal. Nearly every metallurgical
lab has one of these microscopes. You should be able
to find one locally.

If this technique doesn't work for you, there's a
relatively new instrument developed by my former
employer, ERIM International, in Ann Arbor, called a
Holomapper. Essentially, it's an expensive instrument
that performs two-dimensional surface metrology on
parts up to 7" x 7". It does this nearly
instantaneously using laser technology with an
advertised 0.5 micron uncertainty. This technique
would be well-suited to a sample such as yours where
you mention all the subject holes are on one sample.
One shot collects the information. Analysis would be
just a series of mouse clicks using the computer
software.

If interested, I can provide contact information.
Though ERIM is most interested in selling the
equipment, they'd be very willing to direct you to a
user to promote wider use of this instrument.

Disclaimer: I have no financial interest in ERIM or
its products, I'm just a former employee of the
company.

Stu Smalinskas, P.E.
Sr. Metallurgist
SKF
Plymouth, Michigan
(734) 414-6862
stu.smalinskas-at-skf.com

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Michael wrote:

Hi everyone:
I am looking to retrofit a Nikon Eclipse ME600 to
measure the depth of a series of holes within micron
(or ideally submicron) accuracy on a strip of metal
that has been laser holes drilled into.

I hope to achive this by using the change in z from
the top and the bottom of hole using a calibrated
stage. Does anyone out there have a device that they
had made or purchased at a reasonable price. Are you
willing to share your drawings/expertise?
Thanks,
Michael Coviello
UT Arlington

__________________________________
Do you Yahoo!?
Yahoo! Small Business $15K Web Design Giveaway
http://promotions.yahoo.com/design_giveaway/

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 10:21:04 2004

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Hi Doug,

Boy, is this the question that raises its ugly head.
I have on a couple of occassions used zambonies fixative (containing 4% para and picric acid) to
fix and immunolabel cells for light and EM. Depending on the antibody you can get very good
immunolabeling but the ultrasctructure isn't near as good as if glut was in the mix. I am having
trouble remembering if I used saponin or if the picric acid poked sufficient holes to get the
labelling done. Can you then fix it hard in EM fix? If I was going into LRWhite to do post
embedded labelling the key for improving the ultrastructure for me was to minimize the time spent
dehydrating. Due to the light fixation the dehydration extracted a lot of tissue components. I
ended up just one minute each, 35%, 50%, 70%, 95% then into 100% for a couple changes and
into the infiltration.

However, the next thing I am going to try is light fixation, pelleting, cryoprotection, freezing and
ultrathin cryosectioning so the membranes show up. We just got the equipment to do this. If you
want to go this direction you are welcome to come up and give it a shot...But not before I get a
shot on the new toy. Come to think of it don't you have toys. Have you tried the high pressure
freeze and into Lowicryl on these fibroblasts?

Bob Underwood
U of Washington
Dermatology

On Wed, 7 Apr 2004, Doug Keene wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hello,
}
} I am wanting to localize GFP within cultured fibroblasts at
} the ultrastructural level (TEM). We are using anti-GFP
} antibodies provided by Rockland and another provided by
} Assay Design. We have tried a variety of protocols using
} prefixation in 0.1% glut and/or rendering the cells
} permeable with 0.01% saponin. We've also prefixed the
} cells with 100% methanol (this results in reasonable
} labeling density but terrible ultrastructure). Our typical
} protocol utilizes colloidal gold conjugated secondary
} antibodies.
}
} In any of these protocols I have tried, I am either not
} satisfied with the preservation of the cells or I am not
} satisfied with labeling density. Certainly not an unusual
} quandary for immuno-EM, but surely there is a more
} satisfactory protocol than the ones I have tried!
}
} My question: Does anyone use a TEM protocol for
} intracellular labeling that they are happy with?
}
} Many thanks,
}
} Doug
}
} ----------------------
} Douglas R. Keene
} Associate Investigator
} Micro-Imaging Center
} Shriners Hospital for Children
} 3101 S.W. Sam Jackson Park Road
} Portland, Oregon 97239-3009
} phone: 503-221-3434
} FAX: 503-412-6894
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 10:37:24 2004

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You might be able to use an AFM (probably a Dimension scope, depending
on the size of your strip) in another department at UT-Arlington to
measure the holes in your strip. Try engineering, materials science, or
the new Institute for Nanoscale Science and Engineering Research and
Teaching (INSERT) at UTA to see if there is an AFM on campus.

Bettye
Oregon State University

On Apr 8, 2004, at 5:34 AM, Tomic, Peter (Peter) wrote:

} Michael;
}
} Sounds like an AFM [Atomic Force Microscope] may do what you need. The
} reasonable price part is another matter but you need to define
} "reasonable."
}
} Peter Tomic
} Agere Systems
} Allentown, PA
}
} -----Original Message-----
} } From: coviello [mailto:coviello-at-mae.uta.edu]
} Sent: Wednesday, April 07, 2004 6:10 PM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] LM-measuring depths of holes
}
}
}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Hi everyone:
} I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of
} a
} series of holes within micron (or ideally submicron) accuracy on a
} strip
} of metal that has been laser holes drilled into.
}
} I hope to achive this by using the change in z from the top and the
} bottom of hole using a calibrated stage. Does anyone out there have a
} device that they had made or purchased at a reasonable price. Are you
} willing to share your drawings/expertise?
} Thanks,
} Michael Coviello
} UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 11:07:23 2004

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Gee, I would have thought you could have found that much in a can
of peanuts off the grocery store shelf!

On 8 Apr 2004 at 8:08, Francisco J. Hernandez Blazquez wrote:

} Now, I have colleagues that
} had to agree to received US inspectors in their laboratories asking if
} they have contact with terrorist groups because they want to buy 10 mg of
} aflatoxin.

All the best,

Andy Buechele, Washington, D.C., U.S.A.

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 12:29:57 2004

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Dear Doug,
I have done a lot of pre-embedding immuno EM localization of GFP in
cultured hippocampal neurons using the microwave and a 5 hour protocol.
GFP stands up to glutaradehyde fixation (I use 4% pf and 1% glut in PBS),
methanol is too harsh for EM studies.You have to quench the aldehydes with
either sodium borohydride or glycine to be able to see your specific
fluorescence. I have used anti-GFP from Roche successfully. I
permeabilize with 0.025 % to 0.05% saponin -the microwave increases the
efficiency of permeabilization.
For my secondary, I use Texas Red conjugated fluoronanogold so you can see
both the red (anti-GFP) and green fluorescence (GFP) and can check your
labeling at the light level before proceeding to EM processing. I silver
enhance the nanogold and embed my coverslips in Embed 812 resin.
What organelle is the GFP associated with?
I will be happy to send you a detailed protocol if you like. Good luck,
JoAnn Buchanan

Department of Molecular and Cellular Physiology
Stanford University School of Medicine
Stanford, CA 94305
650-723-5856

Hello,
I am wanting to localize GFP within cultured fibroblasts at
the ultrastructural level (TEM). We are using anti-GFP
antibodies provided by Rockland and another provided by
Assay Design. We have tried a variety of protocols using
prefixation in 0.1% glut and/or rendering the cells
permeable with 0.01% saponin. We've also prefixed the
cells with 100% methanol (this results in reasonable
labeling density but terrible ultrastructure). Our typical
protocol utilizes colloidal gold conjugated secondary
antibodies.
In any of these protocols I have tried, I am either not
satisfied with the preservation of the cells or I am not
satisfied with labeling density. Certainly not an unusual
quandary for immuno-EM, but surely there is a more
satisfactory protocol than the ones I have tried!
My question: Does anyone use a TEM protocol for
intracellular labeling that they are happy with?
Many thanks,
Doug

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 12:32:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Michael,

You may want to consider doing this through software. We have a product
called EFI, other manufacturers have similar products by different names.
Essentially, the software acquires images at different focus settings and
extracts the focused part. Since the software usually controls the z-motor,
each focused piece has a definite height value, and the entire 3-dimensional
structure can be extracted. You can then display and measure your object in
3D. The technique does not work for everything, but your application might
work. The resolution you can expect is related to the depth of focus of your
lens and the number of images you take.
With a motorized z-stage, you can do the whole analysis automatically.

If you are interested in getting more information, contact me directly. I'd
be more than happy to find out if this works for you, if you can send me a
sample.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: coviello [mailto:coviello-at-mae.uta.edu]
Sent: Wednesday, April 07, 2004 16:10
To: Microscopy-at-MSA.Microscopy.Com

Hi everyone:
I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of a
series of holes within micron (or ideally submicron) accuracy on a strip
of metal that has been laser holes drilled into.

I hope to achive this by using the change in z from the top and the
bottom of hole using a calibrated stage. Does anyone out there have a
device that they had made or purchased at a reasonable price. Are you
willing to share your drawings/expertise?
Thanks,
Michael Coviello
UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 12:44:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Apr 8, 2004, at 9:19 AM, Andrew Buechele wrote:

} Gee, I would have thought you could have found that much in a can
} of peanuts off the grocery store shelf!
}
} On 8 Apr 2004 at 8:08, Francisco J. Hernandez Blazquez wrote:
}
} } Now, I have colleagues that
} } had to agree to received US inspectors in their laboratories asking if
} } they have contact with terrorist groups because they want to buy 10
} } mg of
} } aflatoxin.
} }
Dear Andrew,
10 mg is a lot of aflatoxin; I'd switch markets.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 14:02:14 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Sylvain: I recommend you get yourself the following two books:

Scanning Electron Microscopy: A Student's Handbook by Postek, Howard, Johnson,
McMichael
Ladd Research (I got my copy from Ladd, but I think other vendors carry it.)

Scanning Electron Microscopy and X-Ray Microanalysis, 3rd edition, by Goldstein,
Newbury, Joy, Lyman, et. al.
Kluwer academic Press (You can get this one from Kulwer or MSA)

Both of these will answer many questions for you.

sylvain maury wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} hi everyone!
}
} does anyone have some informations, or some theory about the charging
} phenomenon of SEM ?
}
} I know it's because of the secondary electrons yield, producing a dark
} rectangle on image, when setting a too low voltage (low electron energy)
} , and a bright one, appearing like a false relief, at a too high voltage
} (high electron energy). But, is that all?
}
} Where can i find a good bibliography?
}
} thanx.
}
} Sylvain

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 14:16:08 2004

Contents Retrieved from Microscopy Listserver Archives
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Mike;

Does this method work on "soft" surfaces. For example, what does the system do if there are no nice crisp edges to focus on or if there is poor contrast? If at the bottom of Michael's hole or indentation the surface is like a hemisphere, would the system have a tough time hunting for a surface? I've had a similar imaging/measurement problem but AFM resolved the issue within angstroms and without any optical issues like depth of field or sample tilt relative to the objective lens.

Peter
Agere Systems

-----Original Message-----
} From: Mike Bode [mailto:mb-at-soft-imaging.com]
Sent: Thursday, April 08, 2004 1:47 PM
To: Microscopy-at-MSA.Microscopy.Com

Michael,

You may want to consider doing this through software. We have a product
called EFI, other manufacturers have similar products by different names.
Essentially, the software acquires images at different focus settings and
extracts the focused part. Since the software usually controls the z-motor,
each focused piece has a definite height value, and the entire 3-dimensional
structure can be extracted. You can then display and measure your object in
3D. The technique does not work for everything, but your application might
work. The resolution you can expect is related to the depth of focus of your
lens and the number of images you take.
With a motorized z-stage, you can do the whole analysis automatically.

If you are interested in getting more information, contact me directly. I'd
be more than happy to find out if this works for you, if you can send me a
sample.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: coviello [mailto:coviello-at-mae.uta.edu]
Sent: Wednesday, April 07, 2004 16:10
To: Microscopy-at-MSA.Microscopy.Com

Hi everyone:
I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of a
series of holes within micron (or ideally submicron) accuracy on a strip
of metal that has been laser holes drilled into.

I hope to achive this by using the change in z from the top and the
bottom of hole using a calibrated stage. Does anyone out there have a
device that they had made or purchased at a reasonable price. Are you
willing to share your drawings/expertise?
Thanks,
Michael Coviello
UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 18:37:12 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello Peter,

as I had mentioned in my posting, the method does not work for everything.
Transparent samples are of course an issue, and you also have to be able to
"look into" the structure, which rules out holes deeper than the working
distance of your lens. A hemispherical indentation should not really be a
problem, unless it is very smooth and featureless.

I think, soft materials are one example where the optical method has some
advantages, as they work without touching the sample, while with an AFM type
instrument you "drag" a tip across the surface, and you might have problems
with soft materials. The optical technique does not really rely on crisp
edges, but rather on some contrast from the material. I don't want to go
into a description of the technique here, but if you are interested, you can
go to our web site www.soft-imaging.com, then go to Products-"Add-ins"-efi
and you'll find an explanation.

An AFM type of instrument can definitely give you results with a much higher
resolution (nm), but I understood from Michael's post, that a) he wants to
use a microscope, and b) he's looking at micron resolution, not nm. I am
also not sure what happens if the holes are tens or hundreds of microns
deep, and if you can use an AFM for those aspect ratios.

Otherwise I agree with you, of course. An AFM type instrument is certainly
an option that can give you the same or in many cases better results.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Sent: Thursday, April 08, 2004 13:31
To: Mike Bode; Microscopy-at-MSA.Microscopy.Com

Mike;

Does this method work on "soft" surfaces. For example, what does the system
do if there are no nice crisp edges to focus on or if there is poor
contrast? If at the bottom of Michael's hole or indentation the surface is
like a hemisphere, would the system have a tough time hunting for a surface?
I've had a similar imaging/measurement problem but AFM resolved the issue
within angstroms and without any optical issues like depth of field or
sample tilt relative to the objective lens.

Peter
Agere Systems

-----Original Message-----
} From: Mike Bode [mailto:mb-at-soft-imaging.com]
Sent: Thursday, April 08, 2004 1:47 PM
To: Microscopy-at-MSA.Microscopy.Com

Michael,

You may want to consider doing this through software. We have a product
called EFI, other manufacturers have similar products by different names.
Essentially, the software acquires images at different focus settings and
extracts the focused part. Since the software usually controls the z-motor,
each focused piece has a definite height value, and the entire 3-dimensional
structure can be extracted. You can then display and measure your object in
3D. The technique does not work for everything, but your application might
work. The resolution you can expect is related to the depth of focus of your
lens and the number of images you take.
With a motorized z-stage, you can do the whole analysis automatically.

If you are interested in getting more information, contact me directly. I'd
be more than happy to find out if this works for you, if you can send me a
sample.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: coviello [mailto:coviello-at-mae.uta.edu]
Sent: Wednesday, April 07, 2004 16:10
To: Microscopy-at-MSA.Microscopy.Com

Hi everyone:
I am looking to retrofit a Nikon Eclipse ME600 to measure the depth of a
series of holes within micron (or ideally submicron) accuracy on a strip
of metal that has been laser holes drilled into.

I hope to achive this by using the change in z from the top and the
bottom of hole using a calibrated stage. Does anyone out there have a
device that they had made or purchased at a reasonable price. Are you
willing to share your drawings/expertise?
Thanks,
Michael Coviello
UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 8 19:40:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

-------- Original Message --------

We've been discussing how it costs us $5,000 U.S. to dispose of a liter of
fluid with a gram or two of uranium in it while over in Iraq the U.S. is
dumping tons of the stuff.

There's compliance here and compliance there...

-Michael

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 9 00:00:21 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Dr. Williams:

I am a private consultant which specializes in training in all phase of
electron microscopy. If you would like to have me come to your facility and
train you on your equipment, please contact me to discuss details.

Bill McManus
President
Mt Ogden Scientific Services LLC
moss-at-cut.net
435-946-8739

} From: "Lloyd Williams" {Williams-at-genectr.hunter.cuny.edu}
} To: {Microscopy-at-sparc5.microscopy.com}
} Subject: [Microscopy] Course To Learn Basics of TEM
} Date: Wed, 7 Apr 2004 12:48:35 -0400
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_________________________________________________________________
Tax headache? MSN Money provides relief with tax tips, tools, IRS forms and
more! http://moneycentral.msn.com/tax/workshop/welcome.asp

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 9 10:08:10 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I am trying to locate a manual for a Forma Bio-Freezer. Model 8407. It is
a chest type -85 freezer. If any one has such could I get a copy?

Greg

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Sat Apr 10 04:47:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi

I have just spotted your question and hope I am able to provide a simple
explanation?

1. It is not correct to say that an accelerating voltage is too low when
viewing an image at a single kV. The only time that this comment may be
justified is when, having increased the accelerating voltage, you see the
subsurface detail that you desired . In another case when considering EDS
the accelerating voltage may be too low to stimulate the specific peak that
you may desire. I do not believe there is such a situation that a kV is
too low, but of course it may be too low to display the information that you
require. In general most operators of non FEG instruments run at too high a
kV to truly resolve the specimen surface (i.e. } 5kV)! There are other
interesting reasons for contrast changes within images at very low voltages,
these relate to secondary electron emission coefficients and are well
presented by N.R.Whetton in Methods of Experimental Physics, Vol IV (1962)

2. The dark patch on the image at low accelerating voltages is due to
contamination that has deposited on the specimen surface. The contamination
is invariably a lower emitter of electrons, thus it shows up as a dark patch
or line. You do not see this at a higher kV because the additional voltage
causes the beam
to penetrate further into the specimen, the sub surface information
generated dominating the image hiding the "surface" contamination from your
view. Thus
to see contamination is an indication that you are seeing the "true
surface" of the specimen.

3. Charge on the specimen surface is due to an insufficient earth leakage
path in relation to the incident beam current and you are correct in the
belief that this may give rise to a bright square on the image.

4. Another visualisation of charge is the bright particle with a black
halo around it. Here the charge field that has built up around the particle
is preventing the
low energy SE escaping, whilst if you look closely the high energy BSE do
escape and provide information within the charge (black) cloud.

5. In a charge-discharge situation, often seen on slow scans, the image
will dim (through a reduction in SE emitted) as the specimen charges,
flashing bright when the system discharges due to the sudden freeing of the
SE held under the charge. Thus a progressively darkening area in an image
indicates charge, the bright flash across one or more lines indicates
discharge!

Good luck with your microscopy.

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob 07711 606967
www.emcourses.com

----- Original Message -----
} From: "sylvain maury" {sylvain.maury-at-thalesgroup.com}
To: "Microscopy community" {microscopy-at-msa.microscopy.com}
Sent: Thursday, April 08, 2004 8:42 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mahtab977-at-yahoo.com) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Friday,
April 9, 2004 at 11:59:09
---------------------------------------------------------------------------

Email: mahtab977-at-yahoo.com
Name: Mahtab Shahkarami

Organization: San Jose State University

Education: Graduate College

Location: San Jose, CA USA

Question: I'm working on SEMs of bacterial cells attached to various
surfaces (eg glass and chitin) and I've been successfully dehydrating
my specimens using the basic CPD/CO2 procedure. However I am limited
to the number of CPD runs I have time and $$ for. A labmate suggested
I try actetone dehydration....is acetone a worthy alternative?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Apr 10 12:23:59 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Andrews,

I think one should be grateful rather then sarcastic to anybody that takes
seriously any potential threat of terrorism, small and remote as it may be.
At least I am, whenever the guard in front of Pizza-Hut, or the movies, or a
bus looks into my pockets.

And as Bill Tivol says, 10mg is sometimes a lot of material.

Dr. Uri Admon
Israel

----- Original Message -----
} From: "Andrew Buechele" {andrewb-at-vsl.cua.edu}
To: {Microscopy-at-sparc5.microscopy.com} ; "Sergey Ryazantsev"
{sryazant-at-ucla.edu}
Sent: Thursday, April 08, 2004 5:19 PM

Mahtab,

Acetone can work, and so can ethanol, or freeze-drying, or even air,
sometimes. The other way is to use hexamethylsilizane (HMDS). This
works very well for most bacteria. Procedures and more information
can be found in Microscopy Today ( http://www.microscopy-today.com
for a table of contents of back issues) and on the Univ. Florida
"Tips and Tricks" web site
http://www.biotech.ufl.edu/EM/tips/index.html .
But briefly:
after the final absolute ethanol step, transfer the samples through
an EtOH:HMDS series to 100% HMDS. 2:1, 1:2 EtOH:HMDS, 3 X 100% HMDS
usually works. Then dry either at room temperature or at 60 deg C.
All this IN A FUME HOOD. You do NOT want to breathe HMDS.
The rest of the details depend on things like: are the bacteria in
suspension or on filters and so forth.
Contact me if you have further questions.

Phil

} Email: mahtab977-at-yahoo.com
} Name: Mahtab Shahkarami
}
} Organization: San Jose State University
}
} Education: Graduate College
}
} Location: San Jose, CA USA
}
} Question: I'm working on SEMs of bacterial cells attached to various
} surfaces (eg glass and chitin) and I've been successfully
} dehydrating my specimens using the basic CPD/CO2 procedure. However
} I am limited to the number of CPD runs I have time and $$ for. A
} labmate suggested I try actetone dehydration....is acetone a worthy
} alternative?
}
} ---------------------------------------------------------------------------

--
Philip Oshel
Supervisor, AMFSC and BBPIC microscopy facilities
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 11 21:25:44 2004

Contents Retrieved from Microscopy Listserver Archives
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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Francisco J. Hernandez Blazquez wrote:
=====================================================
} I'm very, very worried about this topic. If this topic is treated as a
} political matter, it will make the life of researches that work in
} developmental countries, like me, extremely difficult. We depend on
importation
} to do our research and it is already hard enough to obtain some drugs
without
} the absurd regulations that emerge from time to time due to the politics
} ignorance and paranoid in what concerns to the scientific matters. It is
not
} rules that will stop terrorists to acquire material that may be used in
attacks
} because these people do not obey rules. They obtain their material in the
black
} market.
}
} As an example, I had to stop working with the effect of aflatoxin in
tropical
} fishes, a serious problem in Brazil, because it became almost impossible
to buy
} the product after some menace of its use by terrorist. Before the
application
} of absurd regulations by the US government, it could take six months to
receive
} the product, now it takes almost two years, after several formularies are
} filled. Now, I have colleagues that had to agree to received US inspectors
in
} their laboratories asking if they have contact with terrorist groups
because
} they want to buy 10 mg of aflatoxin.
}
===============================================================
I would respectfully like to point out that the matter of export controls
over certain potentially dangerous materials is not the result of "absurd
regulations" by the US government but the result of consensus agreements
through the UN, the IAEA, IATA and other world bodies to which Brazil is
also a signor. These regulations may indeed be absurd, but your complaint
is with these world bodies, not specifically the US government!

The people who have restricted your access to aflatoxin are the same type of
people who have mandated that a $30 bottle of silver paint, something no
more "dangerous" than a woman's fingernail polish remover, has to be shipped
(to certain countries, including Brazil) by air freight (for several
hundred dollars) as "dangerous goods" instead of via FedEx or UPS for a
fraction of the amount (as it could be shipped for example, to Japan or to
most of the EC countries).

Beryllium TEM grids are restricted for shipment to certain countries because
some bureaucrat thought that some rogue nation might purchase a large enough
number of beryllium grids to melt down the metal and turn it into some
critical part for a nuclear reactor. But these are regulations not of the
US government but of one or more of these world bodies. The list of
examples is endless.

We as an industry have let this happen because too many of us want to "stay
out of politics" but when we think that way, the bureaucrats who have
nothing better to do with their time, saddle us with these kinds of onerous
situations. I would suggestion we do just the opposite: We have to become
politically involved and lobby our legislators to bring some semblance of
sanity back to the shipping (and export) regulations. In our own small way
, we invite to our company every few years either one of our representatives
in Harrisburg or in Washington, DC and explain how government regulations
are holding us back from growing and innovating even more. It does have an
impact. But this is only a drop in the bucket in terms of what really has
to be done in terms of lobbying. Everyone has to be doing it! Worldwide.

In the mean time, so long as researchers using these materials are not going
to be willing to keep such materials under some system of strict
accountability, with the reporting and explaining of any unaccountable
losses, the future would seem to be one where there will indeed be more and
more regulation of these materials which will add to everyone's cost of
doing research.

I apologize to anyone who might think this an inappropriate topic for
discussion on the listserver.

Chuck
============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 11 22:34:03 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (John_Wahlert-at-baruch.cuny.edu) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Sunday, April 11, 2004 at 19:48:44
---------------------------------------------------------------------------

Email: John_Wahlert-at-baruch.cuny.edu
Name: John H. Wahlert

Organization: Baruch College, CUNY

Education: Graduate College

Location: New York, New York, USA

Question: I would like to repair some old slides of lamprey cross sections. The glue has turned white all around the specimens. Where can I find information about renewing old slides that cannot be replaced?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 06:34:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (akoorts-at-medic.up.ac.za) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Monday, April 12, 2004 at 02:20:53
---------------------------------------------------------------------------

Email: akoorts-at-medic.up.ac.za
Name: Alida Koorts

Organization: University of Pretoria

Education: Graduate College

Location: Pretoria, South Africa

Question: I am performing immunolocalization and in situ
hybridization on ultrathin sections (LR White)
of core bone marrow biopsies. I am interested
in ferritin subunit expression in the macrophage.
It seems as though either the vacuolar contents
are extracted or the sections are torn in the
vacuolar areas when ultrathin sections are cut.
(Fixed: 4% paraformaldehyde, 0.05% glutaraldehyde)
Is there perhaps someone that have encountered
these problems and are able to make some comments.
Any advice would be much appreciated.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 06:49:14 2004

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University of Connecticut
Institute of Materials Science

Staff Position in Transmission Electron Microscopy

The Institute of Materials Science (IMS) at UConn is an interdisciplinary
center with the threefold mission of fostering education, research and
outreach in all areas of the materials sciences. The Microscopy Laboratory
is a user facility which houses the main research microscopes (optical, SEM
and TEM) for the IMS. These include a recently commissioned JEOL 2010 UHR
FasTEM equipped with EDAX UTW EDS and Gatan EELS/image filter. There is an
opening in the Laboratory for a Transmission Electron Microscopy specialist.
The appointee will be involved in a range of academic and industrial
projects, and will assist in the operation of the Laboratory including
performing routine maintenance and training/assisting users of the TEMs.

Candidates should hold a higher degree (MS or PhD) in Materials Science,
Physics or a related discipline and must have extensive hands-on experience
in a broad range of TEM techniques. Experience in instrument development
and/or computer image processing/simulation would be beneficial. This is a
fixed-term appointment and is available from July 1st. Screening of the
applications will begin immediately and will continue until the post is
filled. Applications from under-represented groups, including minorities,
women and persons with disabilities are encouraged.

Interested candidates should send a curriculum vitae, including publication
list, and the names of at least three referees with postal addresses,
telephone numbers and Email addresses to: Prof. M. Aindow, Institute of
Materials Science, University of Connecticut, 97 North Eagleville Road,
U-3136, Storrs, CT 06269-3136 USA. Email: m.aindow-at-uconn.edu

--
*********************************************************

Mark Aindow, Associate Professor,
Department of Metallurgy and Materials Engineering
Institute of Materials Science,
97 North Eagleville Road, Unit 3136
University of Connecticut, Storrs,
CT 06269-3136, USA

Tel: +1 (860) 486-2644
FAX: +1 (860) 486-4745
Email: m.aindow-at-uconn.edu

**********************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 07:22:50 2004

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Electron Diffraction Post Doc

I expect to have a vacancy, starting immediately (more or less) for a
post doc (up to three years) to work on EBSD in the SEM. The ideal
candidate will have prior experience of three kinds: experimental
electron microscopy, dynamical diffraction theory and programming.
Although the project is in SEM, experimental experience in TEM would be
equally suitable. The aim of the work is to advance the technique of
EBSD. Prior work has advanced the ability of EBSD to measure strain.
Recent work has shed light on the formation of EBSD patterns through
energy filtering. The next steps are a) to further the use of EBSD to
measure strain and to apply it to electromigration, b) to develop better
spatial resolution in EBSD through energy filtering and c) to write
software to simulate EBSD patterns.

Candidates interested in this post please contact me. If you have sent
me email enquiring about a job and have got a reply saying I have no
vacancies (which was true at the time), please feel free to send your
details again - I have deleted the information you sent previously.

Alwyn Eades
--
..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 08:01:58 2004

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} I am limited to the number of CPD runs I have time and $$ for. A
} labmate suggested I try actetone dehydration....is acetone a worthy
} alternative?
}
} ---------------------------------------------------------------------------
NO. You may have good success using Hexamethyldisilazane (HMDS).
Lee

--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 08:11:56 2004

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The woman who shares my lab space is the caretaker of the histology
slide collection for the medical students here. She has about 250
sets of slides in her care. At the end of each course, when the
boxes are turned in, she goes through them all and selects out those
whose mounting medium has dried out, clouding the specimen as you
described. She has been very successful in refurbishing these slides
simply by soaking them (sometimes for days) in a staining jar filled
with xylene. At some point, the old coverglass drops off. If the
staining has faded, she restains them, then remounts them with fresh
media and a new coverglass. Most of these slides were originally
mounted with either Canada Balsam or Permount, and she stills prefers
Permount to remount them.
Try it with one or two slides.
Good luck,
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 12:54:36 2004

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Hi,

I have a client that is having difficulty keeping their fly heads in
their thin sections. The chiton tends to seperate from the surrounding
plastic. The head is taken off the fly, probosis removed and then
processed more or less using a typical proceedure into epoxy.

any ideas.

Robert J. Kayton, Ph.D.
C.R.O.E.T., L606
Oregon Health & Science Univ.
kayton-at-ohsu.edu
503-494-2504-Office
503-703-3938-Cell
www.ohsu.edu/croet/facilities/emicroscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 13:31:05 2004

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Chuck;
Excellent note, but there is an even more insidious thing coming
in the way of export controls: I had to have an investigation to
determine if hiring a summer intern (in the US) who happened to be from
China (a Ph.D. student at Berkeley) required an export license. Being
student from China is a category that covers a lot of people, and when
the legality of hiring somebody can be covered by export control law,
these bureaucratic tentacles have extended too far.

John Mardinly
Intel

-----Original Message-----
} From: Garber, Charles A. [mailto:cgarber-at-2spi.com]
Sent: Sunday, April 11, 2004 8:44 PM
To: MICROSCOPY BB

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Francisco J. Hernandez Blazquez wrote:
=====================================================
} I'm very, very worried about this topic. If this topic is treated as a
} political matter, it will make the life of researches that work in
} developmental countries, like me, extremely difficult. We depend on
importation
} to do our research and it is already hard enough to obtain some drugs
without
} the absurd regulations that emerge from time to time due to the
politics
} ignorance and paranoid in what concerns to the scientific matters. It
is
not
} rules that will stop terrorists to acquire material that may be used
in
attacks
} because these people do not obey rules. They obtain their material in
the
black
} market.
}
} As an example, I had to stop working with the effect of aflatoxin in
tropical
} fishes, a serious problem in Brazil, because it became almost
impossible
to buy
} the product after some menace of its use by terrorist. Before the
application
} of absurd regulations by the US government, it could take six months
to
receive
} the product, now it takes almost two years, after several formularies
are
} filled. Now, I have colleagues that had to agree to received US
inspectors
in
} their laboratories asking if they have contact with terrorist groups
because
} they want to buy 10 mg of aflatoxin.
}
===============================================================
I would respectfully like to point out that the matter of export
controls
over certain potentially dangerous materials is not the result of
"absurd
regulations" by the US government but the result of consensus agreements
through the UN, the IAEA, IATA and other world bodies to which Brazil is
also a signor. These regulations may indeed be absurd, but your
complaint
is with these world bodies, not specifically the US government!

The people who have restricted your access to aflatoxin are the same
type of
people who have mandated that a $30 bottle of silver paint, something no
more "dangerous" than a woman's fingernail polish remover, has to be
shipped
(to certain countries, including Brazil) by air freight (for several
hundred dollars) as "dangerous goods" instead of via FedEx or UPS for a
fraction of the amount (as it could be shipped for example, to Japan or
to
most of the EC countries).

Beryllium TEM grids are restricted for shipment to certain countries
because
some bureaucrat thought that some rogue nation might purchase a large
enough
number of beryllium grids to melt down the metal and turn it into some
critical part for a nuclear reactor. But these are regulations not of
the
US government but of one or more of these world bodies. The list of
examples is endless.

We as an industry have let this happen because too many of us want to
"stay
out of politics" but when we think that way, the bureaucrats who have
nothing better to do with their time, saddle us with these kinds of
onerous
situations. I would suggestion we do just the opposite: We have to
become
politically involved and lobby our legislators to bring some semblance
of
sanity back to the shipping (and export) regulations. In our own small
way
, we invite to our company every few years either one of our
representatives
in Harrisburg or in Washington, DC and explain how government
regulations
are holding us back from growing and innovating even more. It does have
an
impact. But this is only a drop in the bucket in terms of what really
has
to be done in terms of lobbying. Everyone has to be doing it!
Worldwide.

In the mean time, so long as researchers using these materials are not
going
to be willing to keep such materials under some system of strict
accountability, with the reporting and explaining of any unaccountable
losses, the future would seem to be one where there will indeed be more
and
more regulation of these materials which will add to everyone's cost of
doing research.

I apologize to anyone who might think this an inappropriate topic for
discussion on the listserver.

Chuck
============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 19:06:58 2004

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Hi,

We use Cytovision(v2.75) software by Applied Imaging to detect the ScFISH probes on metaphase chromosomes, while capturing the probe signal it has an option in the software to increase the exposure time of the camera . Usually, we have to increase the exposure time of the camera to be able to see the ScFISH probes.

Currently, we are working on developing an automated microscopy system, for that I need to figure out, how to increase the exposure time of the camera using the following system configuration.

Operating system : Windows NT
ICPCI frame grabber card (Coreco Imaging Inc.,)
COHU camera ( 4912-5010)
ITEX-ICPCI (v3.1.0.0) software

Does anybody have an idea on how to control the exposure time of the camera using ITEX-ICPCI (v3.1.0.0) software. I guess it should be on the on lines of triggered acquisition, but I dont have much idea on how to do it. Please reply me with your valuable suggestions.

Thanks in advance for your help.

Regards,
Pavan Yanala
pkymw5-at-umkc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 23:11:25 2004

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Add 120 metric tons of depleted uranium spread over Kosovo in former
Yugoslavia by American forces. Sergey

At 06:56 PM 4/8/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 12 23:32:15 2004

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Charles
USA has veto in UN, if they don't like something, they veto it, so US share
complete responsibility for every exportation international law. From
another hand, I don't see much willingness from US to cooperate with UN in
many cases (like Iraq), so there is definitely double standards: US smartly
use UN to "cover up" unpopular decisions (like discrimination in export) if
it's in favor of US, otherwise they simply ignore UN resolutions,
international laws and perform on their own. Your posting is too
politically correct to be interesting. I am sorry. This communication
reminds to me the worse time at Soviet Union, when you have to be very
politically correct... what is happening with freedom of speech in this
country and does this country is trying to reproduce mistakes of USSR? In
the beginning of this discussion, I was trying to express the opinion, that
our forum should be out of politics, nobody supports me, so I decided to
express my opinion as a person who could compare and who has a freedom to
see things free from political correctness ) I am not a US citizen). If
this forum is going to be an arena for political correctness, I'll leave
this place immediately, I had enough in USSR. Sergey

At 08:44 PM 4/11/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 01:57:18 2004

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Hello,

we have an inverted microscope Zeiss Axiovert 200 and use the POCMini System
from Zeiss. In general we use it with glass slides with a diameter of 30mm
to observe cells. The device reaches the adjusted temperature very quickly
is very stable during measurements.

Regards,
Mario

Mario Brameshuber
Single Dye Tracing
Institute for Biophysics
Johannes Kepler University of Linz
Altenbergerstra?e 69, 4040 Linz
Austria
phone: +43 732 2468 9288

-----Ursprungliche Nachricht-----
Von: drk-at-SHCC.org [mailto:drk-at-SHCC.org]
Gesendet: Mittwoch, 07. April 2004 19:09
An: Microscopy-at-sparc5.microscopy.com
Betreff: Heated stage for LM

----------------------------------------------------------------------------
--
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hello,

We have Leica inverted (DMIRE2) and upright
(DMRXA2) microscopes in our Confocal facility that we would
like to add live cell imaging capabilities to. At the
moment, a heating stage would be adequate. If you are
using such a stage (even on a different brand
microscope) and are really happy with it, would you please
share the manufacturer with me?

Thank you in advance,

Doug

----------------------
Douglas R. Keene
Associate Investigator
Micro-Imaging Center
Shriners Hospital for Children
3101 S.W. Sam Jackson Park Road
Portland, Oregon 97239-3009
phone: 503-221-3434
FAX: 503-412-6894

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 07:45:18 2004

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Colleagues

While this started out as a discussion on the problems getting
Osmium due to various exportation rules (which I had no
problem with discussing), it is now starting to wander off topic.

Regardless of how one feels about politics in the world, that
subject does not belong on this forum. There are a number
of open forums on the Internet that you can us for these purposes.
This is not one of them.

It is time to end this thread , and let us return to the subject
at hand namely: Microscopy & Microanalysis.

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 08:27:23 2004

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Quoting Robert Kayton {kayton-at-ohsu.edu} :
} I have a client that is having difficulty keeping their fly heads in
} their thin sections. The chiton tends to seperate from the surrounding
} plastic. The head is taken off the fly, probosis removed and then
} processed more or less using a typical proceedure into epoxy.
}
} Robert J. Kayton, Ph.D.
} C.R.O.E.T., L606
} Oregon Health & Science Univ.
} kayton-at-ohsu.edu
} 503-494-2504-Office
} 503-703-3938-Cell
} www.ohsu.edu/croet/facilities/emicroscopy

Robert,
I have had this same problem with pupae and adults, and have tried many things
but nothing worked well. The best results were obtained by doing all the
trimming with a glass knife, taking only thin sections off the block at a time,
less pressure at the epon/cuticle interface. The cuticle at the bottom of the
block should sectioned off so that the knife hits tissue.

In that the head is "lumpy", the first sections will still tend to pop out of
the plastic. If there is a need to look at these, it is helpful to collect
the thick sections on water, either in a boat or a drop of water at the edge of
the glass knife and pick up the material with a loupe like EMS sells.
I keep the water at the top of the knife by drawing a line of finger nail polish
(old and cheap are fine) across the knife about 5 mm from the top edge. The
polish sticks much better than wax. Time must be allowed to let the polish dry,
so I do several at a time usually after I break the knives so they will be
ready when I need them.

As the material gets large enough to pick up with a hair, I just transfer that
to the slide and forget the excess plastic.

I am looking forward to others suggestions also.

Pat Connelly
Dept of Biology
Univ. of Pennsylvania
Philadelphia, PA
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 08:27:24 2004

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Quoting Robert Kayton {kayton-at-ohsu.edu} :
} I have a client that is having difficulty keeping their fly heads in
} their thin sections. The chiton tends to seperate from the surrounding
} plastic. The head is taken off the fly, probosis removed and then
} processed more or less using a typical proceedure into epoxy.
}
} Robert J. Kayton, Ph.D.
} C.R.O.E.T., L606
} Oregon Health & Science Univ.
} kayton-at-ohsu.edu
} 503-494-2504-Office
} 503-703-3938-Cell
} www.ohsu.edu/croet/facilities/emicroscopy

Robert,
I have had this same problem with pupae and adults, and have tried many things
but nothing worked well. The best results were obtained by doing all the
trimming with a glass knife, taking only thin sections off the block at a time,
less pressure at the epon/cuticle interface. The cuticle at the bottom of the
block should sectioned off so that the knife hits tissue.

In that the head is "lumpy", the first sections will still tend to pop out of
the plastic. If there is a need to look at these, it is helpful to collect
the thick sections on water, either in a boat or a drop of water at the edge of
the glass knife and pick up the material with a loupe like EMS sells.
I keep the water at the top of the knife by drawing a line of finger nail polish
(old and cheap are fine) across the knife about 5 mm from the top edge. The
polish sticks much better than wax. Time must be allowed to let the polish dry,
so I do several at a time usually after I break the knives so they will be
ready when I need them.

As the material gets large enough to pick up with a hair, I just transfer that
to the slide and forget the excess plastic.

I am looking forward to others suggestions also.

Pat Connelly
Dept of Biology
Univ. of Pennsylvania
Philadelphia, PA
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 08:33:22 2004

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I have followed with some interest the line of discussion re: osmium
tetroxide. I say some, because the discussion went from one subscriber
sharing the news that Osmium Tetroxide was going to become strictly
regulated to a great heated political debate.

I believe in freedom of speech, but I do not think the ListServer is a forum
for such discussion. Let's leave the politics out of this server and keep
to the facts. The issue of Osmium Tetroxide has been more than discussed
and unless someone has some real facts re: the regulation of it's usage,
please communicate among yourselves.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 08:48:58 2004

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I had a similar problem with fruit fly legs. Two possible solutions
(which I could not try in the study I was involved with) are 1. treating
with a chitinase or 2. taking tissue immediately after molting so the
chitin is still relatively soft. Also check out papers in Nature
184:1584, 1959 (Beckel) and Trans. Am. Micros. Soc. 74:197-201, 1955
(DeGiusti and Ezman).

Geoff

Robert Kayton wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 08:53:31 2004

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Announcing a 5 day intensive AFM short course entitled "AFM and Other
Scanned Probe Microscopies". It is being taught at N.C. State University in
Raleigh, NC by Prof. Phil Russell, Dr. Joe Griffith and others from June
21 -25, 2004.

This one-week short course on atomic force microscopy has evolved from the
numerous Scanned Probe Microscopy courses developed and taught by Prof.
Russell over the past 2 decades. It is designed for technicians, scientists,
engineers and researchers. The course includes lectures and laboratories
with hands-on time using a variety of scanning probe microscope (SPM)
systems.

For more information got to www.ncsu.edu/aif/afmcourse

Dale Batchelor, Ph.D.
N.C. State University
Analytical Instrumentation Facility
EGRC room 318C
Campus Box 7531
Raleigh, NC 27695
Office 919-515-3841
FAX 919-515-6965
E-Mail dale_batchelor-at-ncsu.edu
Website www.ncsu.edu/aif

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 13 09:34:26 2004

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I think quite a few people supported your initial attempt to keep politics
out of this forum. There are other newsgroups for that sort of thing.

Lesley Weston.

on 12/04/2004 9:51 PM, Sergey Ryazantsev at sryazant-at-ucla.edu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Charles
} USA has veto in UN, if they don't like something, they veto it, so US share
} complete responsibility for every exportation international law. From
} another hand, I don't see much willingness from US to cooperate with UN in
} many cases (like Iraq), so there is definitely double standards: US smartly
} use UN to "cover up" unpopular decisions (like discrimination in export) if
} it's in favor of US, otherwise they simply ignore UN resolutions,
} international laws and perform on their own. Your posting is too
} politically correct to be interesting. I am sorry. This communication
} reminds to me the worse time at Soviet Union, when you have to be very
} politically correct... what is happening with freedom of speech in this
} country and does this country is trying to reproduce mistakes of USSR? In
} the beginning of this discussion, I was trying to express the opinion, that
} our forum should be out of politics, nobody supports me, so I decided to
} express my opinion as a person who could compare and who has a freedom to
} see things free from political correctness ) I am not a US citizen). If
} this forum is going to be an arena for political correctness, I'll leave
} this place immediately, I had enough in USSR. Sergey
}
} At 08:44 PM 4/11/2004, you wrote:
}
}
} }
----------------------------------------------------------------------------
-} } -
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} }
} } Francisco J. Hernandez Blazquez wrote:
} } =====================================================
} } } I'm very, very worried about this topic. If this topic is treated as a
} } } political matter, it will make the life of researches that work in
} } } developmental countries, like me, extremely difficult. We depend on
} } importation
} } } to do our research and it is already hard enough to obtain some drugs
} } without
} } } the absurd regulations that emerge from time to time due to the politics
} } } ignorance and paranoid in what concerns to the scientific matters. It is
} } not
} } } rules that will stop terrorists to acquire material that may be used in
} } attacks
} } } because these people do not obey rules. They obtain their material in the
} } black
} } } market.
} } }
} } } As an example, I had to stop working with the effect of aflatoxin in
} } tropical
} } } fishes, a serious problem in Brazil, because it became almost impossible
} } to buy
} } } the product after some menace of its use by terrorist. Before the
} } application
} } } of absurd regulations by the US government, it could take six months to
} } receive
} } } the product, now it takes almost two years, after several formularies are
} } } filled. Now, I have colleagues that had to agree to received US inspectors
} } in
} } } their laboratories asking if they have contact with terrorist groups
} } because
} } } they want to buy 10 mg of aflatoxin.
} } }
} } ===============================================================
} } I would respectfully like to point out that the matter of export controls
} } over certain potentially dangerous materials is not the result of "absurd
} } regulations" by the US government but the result of consensus agreements
} } through the UN, the IAEA, IATA and other world bodies to which Brazil is
} } also a signor. These regulations may indeed be absurd, but your complaint
} } is with these world bodies, not specifically the US government!
} }
} } The people who have restricted your access to aflatoxin are the same type of
} } people who have mandated that a $30 bottle of silver paint, something no
} } more "dangerous" than a woman's fingernail polish remover, has to be shipped
} } (to certain countries, including Brazil) by air freight (for several
} } hundred dollars) as "dangerous goods" instead of via FedEx or UPS for a
} } fraction of the amount (as it could be shipped for example, to Japan or to
} } most of the EC countries).
} }
} } Beryllium TEM grids are restricted for shipment to certain countries because
} } some bureaucrat thought that some rogue nation might purchase a large enough
} } number of beryllium grids to melt down the metal and turn it into some
} } critical part for a nuclear reactor. But these are regulations not of the
} } US government but of one or more of these world bodies. The list of
} } examples is endless.
} }
} } We as an industry have let this happen because too many of us want to "stay
} } out of politics" but when we think that way, the bureaucrats who have
} } nothing better to do with their time, saddle us with these kinds of onerous
} } situations. I would suggestion we do just the opposite: We have to become
} } politically involved and lobby our legislators to bring some semblance of
} } sanity back to the shipping (and export) regulations. In our own small way
} } , we invite to our company every few years either one of our representatives
} } in Harrisburg or in Washington, DC and explain how government regulations
} } are holding us back from growing and innovating even more. It does have an
} } impact. But this is only a drop in the bucket in terms of what really has
} } to be done in terms of lobbying. Everyone has to be doing it! Worldwide.
} }
} } In the mean time, so long as researchers using these materials are not going
} } to be willing to keep such materials under some system of strict
} } accountability, with the reporting and explaining of any unaccountable
} } losses, the future would seem to be one where there will indeed be more and
} } more regulation of these materials which will add to everyone's cost of
} } doing research.
} }
} } I apologize to anyone who might think this an inappropriate topic for
} } discussion on the listserver.
} }
} } Chuck
} } ============================================
} } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } President 1-800-2424-SPI
} } SPI SUPPLIES FAX: 1-610-436-5755
} } PO BOX 656 e-mail:cgarber-at-2spi.com
} } West Chester, PA 19381-0656 USA
} } Cust.Service: spi2spi-at-2spi.com
} }
} } Look for us!
} } ########################
} } WWW: http://www.2spi.com
} } ########################
} } ============================================
}
} _____________________________________
}
} Sergey Ryazantsev Ph. D.
} Electron Microscopy
} UCLA School of Medicine
} Department of Biological Chemistry
} 10833 Le Conte Ave, Room 33-089
} Los Angeles, CA 90095
}
} Phone: (310) 825-1144 (office)
} (310) 206-1029 (Lab)
} FAX (departmental): (310) 206-5272
} mailto:sryazant-at-ucla.edu
}
}
}
}

--
Lesley Weston.

3512 W. 31st Avenue
Vancouver, B.C.
V6S 1X9

(604) 263 3122

lesley-at-vancouverbc.net

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 14 09:01:06 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwareham-at-utah.gov) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, April 12, 2004 at 16:25:49
---------------------------------------------------------------------------

Email: bwareham-at-utah.gov
Name: Beverly Wareham

Organization: Utah Veterinary Diagnostic Lab

Title-Subject: [Microscopy] [Filtered] TEM film Development

Question: I am looking for a facility that would be willing to develop Kodak 4489 film. Please include pricing and turn around time.
Thank you,
Beverly Wareham

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 14 09:02:03 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ottagonosole-at-tiscali.it) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 14, 2004 at 08:54:22
---------------------------------------------------------------------------

Email: ottagonosole-at-tiscali.it
Name: giovanni de caro, md

Organization: associazione bimbononno onlus - italia

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: We are a no profit organization devoted to youngsters education; we have founded a small volunteer operated natural sciences museum in southern Italy . Please see our website for details on our activities at :
http://web.tiscali.it/bimbononno
Recently we obtained a dismissed Leitz- AMR 1000 scanning electron microscope, which was in working
condition when turned off in november, 2003. we have the manulas and electronic schemes. We are seeking for an expert in the installation and operation of this instrument in order to help us in performing reinstallation and recalibration at our lab.

Thank you

Giovanni De Caro, MD
Director
Museo laboratorio di Scienze Naturali "S.Eugenio de Mazenod"-
Ripalimosani (Campobasso)
Italia

E-mail: ottagonosole-at-tiscali.it

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From MicroscopyL-request-at-ns.microscopy.com Wed Apr 14 14:11:28 2004

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Many people have studied drosophila tissues by TEM despite
the embedding difficulties. I have done many thin sections
of the eye and the epoxy usually separates from the eye
surface boundary. I just collected the section parts that
contain the tissue onto a grid with or without a film
support. If you need to examine areas near the surface
boundary a film support is usually necessary.

Larry Ackerman
Keck Advanced Microscopy Lab
Dept. of Biochemistry & Biophysics
University of California San Francisco
600-16th Street, Room S101, Box 2140
San Francisco, CA 94158 (for postal mail use 94143)

415-476-4441 FAX 415-514-4142

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 14 14:34:22 2004

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Well, I got caught unexpectedly with a lab tour and was asked about cutting
thin sections. I later found out the thickness I "guesstimated" would cut
a nitrogen atom in half. So how thin can a section of organic material be
cut with a ultra-microtome? Can metals be thinned even thinner/

Thanks for the help and I promise I will not ask about osmium!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 14 18:13:35 2004

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Hello all,

I'm having a problem with my CCD camera on the TEM. When working with an
unprocessed (not gain or dark count corrected), dark (no beam on the CCD),
1024x1024 image - I get a non-linear horizontal profile of the image. In
other words, the intensity stays constant from pixels 0 - 600, then the
profile increases linearly from pixel 600 to 1024 (slope ~ 0.3 pixel
value/pixel number) from the left to the right of the image. I can rotate
the CCD on the optic axis of the TEM, and this problem persists in the same
location (increasing from left to right) regardless of the rotation of the
camera. This problem is seen in all images, but is more prevalent in images
with } 10 sec exposure time.

Has anyone ever seen this problem before? If so, how did you correct for
it?

Instruments being used: Camera is a Proscan HSC 2, 1024x1024 on axis cooled
high speed slow scan CCD camera on a LEO 912 EFTEM (120 kV with LaB6).

Any help would be SUPER!!

Thanks for your help,

William Stratton

-------------------
William G. Stratton
Research Assistant
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 02:46:11 2004

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Hi

My experience in human pathology is that we would be between 50 and 100nm -
the lower the better - say from 60 to 80nm?

Metals - no idea.

Med vänliga hälsningar/With best regards

Gareth

***Come to Stockholm in 2004 to the 26th IFBLS congress*** Take a look at
http://www.vardforbundet.se/ifbls2004

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 07:26:01 2004

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I am interested in knowing what scanner(s) and negative holders
people are using to scan 8 X 10 cm TEM negatives. We are having some
problems with our current setup.

Thank you,
Maureen Petersen
Ohio Agricultural and Research Center/OSU
Wooster, Ohio
--

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 08:26:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (karthins-at-labindia.com) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Thursday, April 15, 2004 at 03:42:37
---------------------------------------------------------------------------

Email: karthins-at-labindia.com
Name: N.S.KARTHIKEYAN

Organization: LABINDIA INSTRUMENTS(P)LTD.

Education: Undergraduate College

Location: City, State, Country

Question: what is the resolution of 35mm slr phtography and photomicrography?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 08:25:21 2004

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Hi Everybody...

We're planning to buy a TEM for our Histology lab. Does anybody know web sources for different models, comparing spesifications, prices and reviews. We're especially interested in Hitachi 7600, Jeol JEM-1011 and LEO Libra 128. Does anybody have experience with these microscopes? If you inform us, we'd be greatly appreciated.
Thanks in advance

Dr. Necat Yžlmaz

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 08:41:00 2004

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I am looking for PC-based image analysis software that can find, count and
measure particles. The particles may be either spheres or vesicles, so
the software must be able to find/measure/count both types. I would also
like the software to report actual diameters as opposed to equivalent
sphere diameter, though doing both is acceptable. Finally, I need it to
be able to do statistics on the analyses that it performs.

If you can provide the names of some software packages that meet these
criteria, as well as the company that makes it and contact information, it
would be a great help to me. Thanks!

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 08:49:53 2004

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William,

if you rotate the camera and the problem persists in the same direction, it
is most likely not the camera that is defective. When you rotate the camera,
do you also rotate the scintillator? If so, it cannot be the scintillator
either, and it must be the setup of your microscope. Is your microscope well
aligned?

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: William Stratton [mailto:wgstratton-at-wisc.edu]
Sent: Wednesday, April 14, 2004 17:08
To: Microscopy

Hello all,

I'm having a problem with my CCD camera on the TEM. When working with an
unprocessed (not gain or dark count corrected), dark (no beam on the CCD),
1024x1024 image - I get a non-linear horizontal profile of the image. In
other words, the intensity stays constant from pixels 0 - 600, then the
profile increases linearly from pixel 600 to 1024 (slope ~ 0.3 pixel
value/pixel number) from the left to the right of the image. I can rotate
the CCD on the optic axis of the TEM, and this problem persists in the same
location (increasing from left to right) regardless of the rotation of the
camera. This problem is seen in all images, but is more prevalent in images
with } 10 sec exposure time.

Has anyone ever seen this problem before? If so, how did you correct for
it?

Instruments being used: Camera is a Proscan HSC 2, 1024x1024 on axis cooled
high speed slow scan CCD camera on a LEO 912 EFTEM (120 kV with LaB6).

Any help would be SUPER!!

Thanks for your help,

William Stratton

-------------------
William G. Stratton
Research Assistant
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 09:24:00 2004

Contents Retrieved from Microscopy Listserver Archives
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Frank:

Ultra-thin sections are generally 40-120nm thick, with 60-80nm the
dominate range for most Biologicals.

There are also "super-thin" sections 4 - 20nm.

But atomic spacings are much smaller than either of these, ( personally
not being a true materials person) atomic sizes seem to range from ~ 0.028 -
0.27nm. And I believe that sucrose is 0.8nm across.

}
} Well, I got caught unexpectedly with a lab tour and was asked about cutting thin
} sections. I later found out the thickness I "guesstimated" would cut a nitrogen
} atom in half. So how thin can a section of organic material be cut with a
} ultra-microtome? Can metals be thinned even thinner/
}
} Thanks for the help and I promise I will not ask about osmium!
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 09:37:47 2004

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Hi fellow listers,

I have a user who uses our sputter coater to coat porous membranes with
gold or silver. His question is how deep the gold/silver can travel into
his membrane pores. The pores are 60 micron deep and the pore diameter is
200 nm. Is it directly proportional to the number of times he coats or is
it totally random ?

Thanks in advance.

Soumitra

*************************************************************
Soumitra Ghoshroy
College Associate Professor, Biology
Director, Electron Microscopy Lab
Box 3EML
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office), 646-3283 (lab)
Fax: 505-646-3282
e-mail:sghoshro-at-nmsu.edu
http://www.cs.nmsu.edu/~biology/Faculty%20&%20Staff/Ghoshroy/Ghoshroy.htm
http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 09:38:21 2004

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At 08:38 AM 04/15/2004 -0400, maureen petersen wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Maureen -

We are having very good luck using a Microtek ScanMaker 8700 and SilverFast
AI software. Of course the TEM film is an odd size. Therefore we use the
"one-size-fits-all" glass holder. It's a little tedious to place the
negatives properly, but I've gotten good at it. We FTP the images to those
who need them and they are really pleased with the results. Bear in mind
however that we are a diagnostic medical service and generally prints do
not have to be made. But our results are good enough to make diagnoses
directly off the monitor.

Joiner

Joiner Cartwright, Jr., Ph.D.
Director, Electron Microscope Lab
Department of Pathology
Baylor College of Medicine

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 11:36:54 2004

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We have an Epson Perfection 3200 Photo and we just put the negatives right on
the screen, because there isn't a holder that will take them. Works fine.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Joiner Cartwright, Jr., Ph.D. [mailto:joiner-at-bcm.tmc.edu]
Sent: Thursday, April 15, 2004 10:56 AM
To: maureen petersen; Microscopy-at-MSA.Microscopy.Com

At 08:38 AM 04/15/2004 -0400, maureen petersen wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Maureen -

We are having very good luck using a Microtek ScanMaker 8700 and SilverFast
AI software. Of course the TEM film is an odd size. Therefore we use the
"one-size-fits-all" glass holder. It's a little tedious to place the
negatives properly, but I've gotten good at it. We FTP the images to those
who need them and they are really pleased with the results. Bear in mind
however that we are a diagnostic medical service and generally prints do
not have to be made. But our results are good enough to make diagnoses
directly off the monitor.

Joiner

Joiner Cartwright, Jr., Ph.D.
Director, Electron Microscope Lab
Department of Pathology
Baylor College of Medicine

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 11:45:21 2004

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Just about every image analysis package should be able to do what you are
asking for. Start with something free, like NIH-Image (the Java version will run
on your PC). If you need more, but still a lot less expense than a package
like Image Pro Plus, try using Photoshop with Fovea Pro or The Image Analysis
Toolkit (ReindeerGraphics.com), which can definitely measure those features and
report actual diameter (as well as inscribed circle size, circumscribed circle
size, etc., depending on how round they really are). The built-in statistics
are modest (mean, variance, skew, kurtosis, regression, etc.) but you can
always dump the data into a spreadsheet of stats program.

=======
In a message dated 4/15/04 11:15:10 AM, Brian.Kirkmeyer-at-iff.com writes:

} I am looking for PC-based image analysis software that can find, count
} and
} measure particles. The particles may be either spheres or vesicles, so
}
} the software must be able to find/measure/count both types. I would also
}
} like the software to report actual diameters as opposed to equivalent
} sphere diameter, though doing both is acceptable. Finally, I need it to
}
} be able to do statistics on the analyses that it performs.
}
} If you can provide the names of some software packages that meet these
}
} criteria, as well as the company that makes it and contact information,
} it
} would be a great help to me. Thanks!

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 12:35:19 2004

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Image Pro Plus by Media Cybernetics provides a full range of utilities for
capturing, communicating, processing, measuring, analyzing, archiving,
reporting, and printing.

Nicola Ranieri, Microscopy/Image Analysis
US FDA Forensic Chemistry Center
6751 Steger Drive
Cincinnati, Ohio 45237-3097
(513) 679-2700 X253
(513) 679-2761 FAX
nranieri-at-ora.fda.gov

-----Original Message-----
} From: Brian.Kirkmeyer-at-iff.com [mailto:Brian.Kirkmeyer-at-iff.com]
Sent: Thursday, April 15, 2004 10:01 AM
To: Microscopy-at-MSA.Microscopy.Com

I am looking for PC-based image analysis software that can find, count and
measure particles. The particles may be either spheres or vesicles, so
the software must be able to find/measure/count both types. I would also
like the software to report actual diameters as opposed to equivalent
sphere diameter, though doing both is acceptable. Finally, I need it to
be able to do statistics on the analyses that it performs.

If you can provide the names of some software packages that meet these
criteria, as well as the company that makes it and contact information, it
would be a great help to me. Thanks!

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 12:43:11 2004

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Ed,

You mention that a dedicated STEM or TEM/STEM (200-300kV) can achieve ~0.8A
resolution.

I think instead of "a" that should be "two". As far as I know, only Steve
Pennycook's and Phil Batson's dedicated STEMs have reached this figure. For TEMs
the number is similar. One would be the high-voltage FEG of Tonamura, and we took
the One-Angstrom Microscope at Berkeley to 0.78A in 2001.

Regards,
Mike

principe wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} A SEM-based STEM at 30kV can achieve subnanometer resolution (~0.8nm). This
} is typically a solid state detector that integrates with an ultra-high
} resolution SEM.
}
} A dedicated STEM or TEM/STEM (200-300kV) can achieve ~0.8A resolution.
}
} Regards,
} Ed
}
} *******************************************
} Edward Principe, Ph.D.
} LEO Electron Microscopy
} Applications Development Scientist
} principe-at-leo-usa.com
} 415-420-4299 (cell)
} 650-595-5516 (fax)
} *******************************************
}
} ----- Original Message -----
} } From: "Patton, David" {David.Patton-at-uwe.ac.uk}
} To: "michael shaffer" {michael-at-shaffer.net}
} Cc: {Microscopy-at-MSA.Microscopy.com}
} Sent: Tuesday, March 30, 2004 7:15 AM
} Subject: [Microscopy] STEM
}
} }
} }
} } --------------------------------------------------------------------------
} ----
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------------
} -----
} }
} } Does STEM (scanning transmission electron microscopy) give
} } better resolution than the best FE SEMs?
} }
} } Dave
} }
} } On Tue, 30 Mar 2004 10:13:01 -0330 michael shaffer
} } {michael-at-shaffer.net} wrote:
} }
} } }
} } }
} }
} } --------------------------------------------------------------------------
} ----
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} } --------------------------------------------------------------------------
} -----
} } }
} } } Breck Bowles writes ...
} } }
} } } } Sue Tyler wrote:-
} } } }
} } } } } Could you tell me if there is such a thing as a LM system
} } } } } that will project high quality images at high magnification
} } } } } that will also transmit to the web? I welcome all comments.
} } }
} } } } It gets technically easier with a live slide if you view on a colour
} } } } TV monitor the same feed that is going to the Net. At the simplest,
} } } } buy a webcam, yank the lens out, and your microscope eyepiece,
} } } } assuming you can find an old ...
} } }
} } } It seems to me you could employ a Nikon Coolpix setup. That is, the
} CP99x
} } } series and I believe the CP5000 provide for NTSC (and PAL) TV output.
} This
} } } video signal could then go into a video input as provided by many video
} } } input cards. Forgive me if I don't have the time to research current
} } } possibilities and manufacturers' model numbers, but the possibility has
} } } existed for some time.
} } }
} } } hth & cheerios ... shAf :o)
} } } Avalon Peninsula, Newfoundland
} } } www.micro-investigations.com
} } }
} } }
} } }
} } }
} } }
} } } This incoming email to UWE has been independently scanned for viruses
} and any virus detected has been removed using McAfee anti-virus software
} } }
} }
} } ----------------------------------------
} } Patton, David
} } Email: David.Patton-at-uwe.ac.uk
} } "University of the West of England"
} }
} }
} }
} } This email has been independently scanned for viruses and any virus
} detected has been removed using McAfee anti-virus software
} }
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 13:32:30 2004

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Hi David,

Thank you for your reply to the Ir coater question. Your email reply
brought up an issue I was trying to resolve about metal sputter coatings.
You seem to have a lot of nice paperwork handy and background on the
subject. So I have a question that I have never seen answered.

I used a small desk top sputter coater in my lab to coat samples for SEM
and it even had uses in TEM. It was not a high resolution coater but it
worked for me in TEM. It had a Au-Pd target and one could sputter a
coating onto a polymer substrate, for example. After thin sectioning the
polymer material, one could determine size of the sputtered metallic
particles. In the TEM, they looked more like bright nanoparticle spheres.

Everyone talks about fine grained Pt, Ir, Cr, etc.

So did you or anyone else on the list ever see published or determine what
particle size 'fine grained' was for Cr, Ir, W, Ta, Pt, Os, or any other
sputter coated metals or alloys that manufacturers sell with their sputter
coaters?

As you can imagine, it is not that difficult to determine these sizes in a
TEM with it's higher magnifications and levels of resolution. All you
basically need is a microtome, the proper target, and a TEM.

Any help with this question about 'fine grain sizes' would be of interest
to me.

Sincerely,

Paul Beauregard
Senior Research Associate
144 Chapel View Drive
Greensburg, PA 15601
(724) 834-2247

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 13:57:05 2004

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I second that emotion - we use the Epson Perfection 3200 Photo Scanner,
too. It works great.

Beth

} We have an Epson Perfection 3200 Photo and we just put the negatives
} right on
} the screen, because there isn't a holder that will take them. Works
} fine.
}
} Peggy Sherwood
} Lab Associate, Photopathology
} Wellman Laboratories of Photomedicine (W224)
} Massachusetts General Hospital
} 55 Fruit Street
} Boston, MA 02114
} 617-724-4839 (voice mail)
} 617-726-6983 (lab)
} 617-726-3192 (fax)
} msherwood-at-partners.org
}

} I am interested in knowing what scanner(s) and negative holders people
} are using to scan 8 X 10 cm TEM negatives. We are having some problems
} with our current setup.
}
} Thank you,
} Maureen Petersen
} Ohio Agricultural and Research Center/OSU
} Wooster, Ohio

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 16:08:57 2004

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As stated before, as good as all Image Analysis software packages will be
capable of doing this. Next to ImageJ (NIH-image) which runs in Java
written macros and also runs on Mac, and Image Pro Plus, I'd like to add one
more: Zeiss KS300/400 software, soon being replaced by the new Axiovision 4,
whcih will enable users to write programs (macros) with visual basic. Gives
you lots of open doors towards the future.
How about comparing Image Pro Plus and Zeiss-software, no idea, but both
have a price, ImageJ (or Image NIH) is free downloadable...but does not
offer backup as commercial software (allthough, there's also a good
mailinglist to exchange ideas/questions, just as for the
Axiovision/KS-software!).
Best regards,

Sven Terclavers

-----Original Message-----
} From: Brian.Kirkmeyer-at-iff.com [mailto:Brian.Kirkmeyer-at-iff.com]
Sent: Thursday, April 15, 2004 16:01 PM
To: Microscopy-at-MSA.Microscopy.Com

I am looking for PC-based image analysis software that can find, count and
measure particles. The particles may be either spheres or vesicles, so
the software must be able to find/measure/count both types. I would also
like the software to report actual diameters as opposed to equivalent
sphere diameter, though doing both is acceptable. Finally, I need it to
be able to do statistics on the analyses that it performs.

If you can provide the names of some software packages that meet these
criteria, as well as the company that makes it and contact information, it
would be a great help to me. Thanks!

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 16:14:30 2004

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Warren,

a very good point! I might have misunderstood the "persisting in the same
direction" part. Let's make this very clear:

If you have a pattern on the computer screen due to some defect or artifact,
and you rotate the camera, and afterwards the pattern is the same in size
and direction ON THE COMPUTER SCREEN, it is due to the camera system,
including optics (or fiber-optics) and phosphor screen.
If you rotate the camera and the pattern rotates also, the problem lies with
a part that was not rotated. This could be the microscope, but also the
optics or scintillator, depending on whether these parts rotate with the
camera or not.

Sorry for any confusion my earlier posting might have created.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]
Sent: Thursday, April 15, 2004 15:15
To: Mike Bode

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 16:31:11 2004

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Hi

I have carried out a number of experiments with my students during SEM
courses to try to determine the best route to use when trying to sputter
coat "into" holes.

Conventional surface coating techniques do not work. We found that the best
way to coat inside holes was to use the best vacuum that the sputter coater
could reach and "force" it to coat using whatever gas remained. A better
mean free path means "straight line" deposition and my reason for the
success!

My deduction was that under conventional sputter coating procedures we rely
upon the mean free path being poor to improve the scatter and hence the
ability to coat rough surfaces fairly evenly. When trying to deposit a coat
inside a hole the poor mean free path prevents the deposit travelling into
the hole.

I have no proof of my theory other than when students are asked to try and
coat a 2mm deep 1mm diameter hole the only way to ensure metal penetrates
the hole that they have found is using the technique set out above;
comments?

Happy sputtering

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob 07711 606967
www.emcourses.com
----- Original Message -----
} From: {sghoshro-at-NMSU.Edu}
To: "MSA Listserve" {Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, April 15, 2004 3:56 PM

I work with semiconductor devices that have rather
opposite dimensions. They are typically 1u-2u deep and
0.5u in diameter. The holes are vias between metal
interconnect layers. The vias are like wine glasses
or flat bottomed V-shape or U-shape.

What I have observed with Au is that it winds up
being a honeycomb of Au filaments rather than
an amorphous layer. The honeycomb cells are rather
consistent in dimensions from top, down holes and
at the bottom of the holes. I think it is safe to
say that all sputter coatings lie on the surface--they
do not penetrate the specimen.

If Au is coated again, there is a cross hatch of honeycombs.
Sometimes the alignment is significant and other times,
not so. I use low mT values (80-85mT) and low current
(20 mA). With better vacuum, the coating is less ballistic
since the Ar ions are not as aggressive, as I figure the
situation to be. Perhaps a plasma person could state
this more elegantly than I. But it seems that any slight
change in vacuum materially affects the characteristics of
the Au coating. And in particular, I would characterize it
more like a web than as a coating.

What I do know is that if I switch to Au/Pd (60/40) or
Pt, the coating is amorphous and cannot be easily seen. Au coating
can be seen at about 350KX. For Au/Pd or Pt, I can't
see a honeycomb at up to 500KX. However, Au/Pd and Pt
look totally different than Au alone. Au/Pd and Pt is
more granular rather than honeycomb. And it will look
this way at 350KX and greater.

Some metallurgical specimens I have imaged are very gross.
E.g., .5mm diameter, 10 mm deep. Au/Pd coating in a
Denton Desk II works fine. Tilted at 5 degrees, I can
look down the entire extent of the hole. Max mag in
this situation is { 5KX. Settings: 85mT, 20mA, 40 seconds.
This seems to be about 80A of coating (give or take).
In amorphous or aligned specimens, EDS will pick up the
coating. Either delete from peak ID or increase KV to
have it obfuscated by volumetric interaction.

For no known obvious reason, I would not use Ag. Well, it may
oxidize. For the above reasons, I would not use Au.
A high vacuum, low current sputter of Au/Pd ought to
work for this application. Please let us know how it
works out in the end.

gary g.

At 07:56 AM 4/15/2004, you wrote:

} Hi fellow listers,
}
} I have a user who uses our sputter coater to coat porous membranes with
} gold or silver. His question is how deep the gold/silver can travel into
} his membrane pores. The pores are 60 micron deep and the pore diameter is
} 200 nm. Is it directly proportional to the number of times he coats or is
} it totally random ?
}
} Thanks in advance.
}
} Soumitra
}
} *************************************************************
} Soumitra Ghoshroy
} College Associate Professor, Biology
} Director, Electron Microscopy Lab
} Box 3EML
} New Mexico State University
} Las Cruces, NM 88003
} Tel: 505-646-3268 (office), 646-3283 (lab)
} Fax: 505-646-3282
} e-mail:sghoshro-at-nmsu.edu
} http://www.cs.nmsu.edu/~biology/Faculty%20&%20Staff/Ghoshroy/Ghoshroy.htm
} http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 20:22:18 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (martha-at-uta.edu) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Thursday, April 15, 2004 at 15:21:35
---------------------------------------------------------------------------

Email: martha-at-uta.edu
Name: Martha Gracey

Organization: University of Texas at Arlington

Education: Graduate College

Location: Arlington, Texas USA

Question: I need help fixing a liquid sample of liposomes for SEM. The cells have no additive in the control and a protein added to the experimental line. After looking at these, I will then have to add a gold antibody for SEM again. Can you help direct me to a reference. I tried air dting and exposing to Osmium vapors and got lousy results.
Thanks
Martha

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 20:35:23 2004

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Hi, Brian-

} I am looking for PC-based image analysis software that can find, count and
} measure particles. The particles may be either spheres or vesicles, so
} the software must be able to find/measure/count both types. I would also
} like the software to report actual diameters as opposed to equivalent
} sphere diameter, though doing both is acceptable. Finally, I need it to
} be able to do statistics on the analyses that it performs.

We have analySIS from Soft Imaging System. It can do all you ask and then
some; it's really powerful. Today I was trying to show someone how to do
some analyses with the free ImageJ, which is really great for the
price, plus they could do it at their own computer. However, they were
unwilling to write or manage macros, and we were having trouble getting it
to identify, count and measure the cells we wanted, so I went back to
analySIS. Problem solved.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 15 21:05:44 2004

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The best sections I ever was able to made weres 10 nm thick proven by
independent methods. It was a sections from ribosomal crystals parallel to
the crystallographic planes (it was another story how to do it). I guess
10 nm is a limit for biological samples embedded into the plastic by
conventional technique. I would imagine, someone could do thinner
sections of uniform material like metal or even plastic (frozen?). I would
think, the limit here would be their stability for manipulation - how to
mount them on EM grid and made flat... You definitely could not cut atom
in half, because "cutting" is actually splitting between atoms (forces
between atoms are weaker than inside). Thickness of sections depends more
from the knife than ultra-microtome (if instrument is in perfect shape of
coarse). Diatome knifes are certified down to 20 nm I believe. Instrument
itself more responsible for reproducibility - how many sections of similar
thickness you may produce in the row. You may produce very good thin
section even on the very old hardly used instrument; you may produce 20
sections of the same quality in the row only on the very good, stable
machine... No osmium tetroxide for while, but still, if somebody
have problems with that stuff, let me know.... Have a great day. Sergey

At 07:41 AM 4/15/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 16 10:21:47 2004

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Hi Phil,

It's a mailinglist I started myself, as comparing to the ImageJ mailinglist.
I announced the existence of it here, but only once, and indeed, maybe I
should've done it more! Although, Zeiss knows of it, even some people from
Zeiss are members and we are having a discussion to move the mailinglist to
a Zeiss-server, in combination of an online download-page, where you can
download all (small) macro's Zeiss, I and maybe others, have written
ourselves. If you need advice or a macro, just write a message to:
KS300-at-topica.com after subscription. To subscribe:
KS300-subscribe-at-topica.com

That's all! Hope to see you soon as a 'member' :-) And don't worry about
tons of emails, this list is actually not that often used, but I must say,
every question has been answered and solved...

Best regards,

Sven

-----Original Message-----
} From: Philip Oshel [mailto:peoshel-at-wisc.edu]
Sent: Friday, April 16, 2004 16:01 PM
To: Sven.Terclavers-at-med.kuleuven.ac.be

LEHIGH MICROSCOPY SCHOOL

Lehigh University, Bethlehem, PA U.S.A.
June 6-18, 2004

* Scanning Electron Microscopy and X-ray Microanalysis

* Introduction to SEM and EDS for the New SEM Operator

* Analytical Electron Microscopy Analysis for TEM Specimens

* Atomic Force Microscopy and Other Scanned Probe Microscopes

* Characterization of Nanostructures

* Focused Ion Beam Instrumentation and Applications

* Problem Solving with SEM and X-ray Microanalysis

* Quantitative X-ray Microanalysis of Bulk Specimens and Particles

* Particle Characterization, Preparation, Microscopy, and Analysis

See course descriptions at:
{http://www.lehigh.edu/microscopy} www.lehigh.edu/microscopy

For more information contact
Sharon Coe at 610.758.5133
{mailto:Sharon.coe-at-Lehigh.edu} Sharon.coe-at-Lehigh.edu

********************************
Sharon L. Coe
Events Coordinator
Lehigh Microscopy School
5 East Packer Avenue
Bethlehem, PA 18015
610-758-5133 (phone)
610-758-4244 (fax)
{mailto:slc6-at-lehigh.ed} slc6-at-lehigh.ed
{http://www.lehigh.edu/microscopy} www.lehigh.edu/microscopy

********************************

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 16 11:06:38 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jjwolo-at-uic.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, April 16, 2004 at 10:49:29
---------------------------------------------------------------------------

Email: jjwolo-at-uic.edu
Name: John J. Wolosewick

Organization: University of Illinois at Chicago

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am trying to find a copy of the instruction manual for an Olympus Inverted Microscope Models IM, IM-2 (early 80's models). Anything would be helpful. The Olympus company has not responded to my e-mails.

Thanks so much.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 16 11:18:12 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi Martha
The problem with liposomes is that when you dehydrate in alcohols,
they dissolve so normal preparation techniques do not work.

The best approach you can take with SEM is to use cryo-SEM. We have a
cryo stage on a our field emission SEM and have used it for all sorts
of lipids and waxes that could not be looked at conventionally. The
sample has to be "cracked open" and the surface water sublimated off.

As for the immunogold treatment, we have been having some success
with using immunononogold and then gold enhancement. Then using the
backscatter detector to pick up the gold deeper in the cells. Using
a mix of the secondary electron detector and the backscatter
detector, you can see the gold even if it is inside cells because the
backscatter detector reaches deeper than the secondary electron
detector.

Both these techniques will be taught at the third International Cryo
EM course here in June. (see the website http://www.emlab.ubc.ca )

You might want to consider plunge freezing and cryo TEM. We will also
have a Vitrobot and a Leica plunge freezer at the cryo course. We
have a TEM with a cryo stage. You can bring your own sample of
liposomes and try out all the techniques including hgih pressure
freezing. If you check out the poster you will see a picture taken
at last year's course of some hela cells which were infected with
chlamidia, high pressure frozen, cracked open and looked at with cryo
SEM.
Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 16 15:36:12 2004

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Maureen,

We recently started using Epson Perfection 3200 Photo flatbed scanner and just
like Beth we are quite happy with its performance. We use the negative holder
that came with the scanner for scanning TEM negatives.

Soumitra

No financial interest in Epson, just a happy user.

Quoting maureen petersen {petersen.67-at-osu.edu} :

}
}
} -----------------------------------------------------------------------------
-
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------------
--
}
} I am interested in knowing what scanner(s) and negative holders
} people are using to scan 8 X 10 cm TEM negatives. We are having some
} problems with our current setup.
}
} Thank you,
} Maureen Petersen
} Ohio Agricultural and Research Center/OSU
} Wooster, Ohio
} --
}
}

Soumitra Ghoshroy Ph.D
College Associate Professor, Biology
Director, Electron Microscopy Lab
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office)
505-646-3283 (lab)
Fax: 505-646-3282

From MicroscopyL-request-at-ns.microscopy.com Sat Apr 17 09:04:30 2004

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Hello everybody...

I'm really appreciated for your kindly helps. All messages really helped us very much.

Best Regards

Dr. Necat Yžlmaz

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 18 08:21:50 2004

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I would like to find out whether Image-Pro Plus or another software package
allows you to obtain the real sphere diameter from a microtomed section.
Since the microtome does not necessarily cut the sphere at the largest
section, a correction needs to be applied. I looked into stereology, but it
would be nice to have this included in the software together with the
count/measure/statistics of the particles. If this is not included in the
software, is it accurate enough to use the following equation: d_actual=(4 x
d_measured)/PI ?

Thank you!

Steven Swier
Institute of Materials Science
University of Connecticut.

_________________________________________________________________
Vraag van de week: Welk soort project zou jij financieel ondersteunen?
http://www.msn.be/microsoft/potential/default.asp

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 18 10:37:09 2004

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In a message dated 4/18/04 10:49:26 AM, stevenswier-at-hotmail.com writes:

} I would like to find out whether Image-Pro Plus or another software package
}
} allows you to obtain the real sphere diameter from a microtomed section.
}
} Since the microtome does not necessarily cut the sphere at the largest
}
} section, a correction needs to be applied. I looked into stereology, but
} it
} would be nice to have this included in the software together with the
} count/measure/statistics of the particles. If this is not included in the
}
} software, is it accurate enough to use the following equation: d_actual=(4
} x
} d_measured)/PI ?
}

Fovea Pro (www.reindeergraphics.com) does include the stereological
measurements and calculations for spheres seen in section, and you can even run the
Photoshop-compatible plugins within Image Pro Plus. Be aware, however, that this
method (inherently) depends critically on several assumptions:
1) that the particles are in fact spheres - surprisingly small deviations
have major influences on the results
2) that the sections are thin,and you do not have "overprojection" problems
3) that small polar caps are visible (or that you can specify the extent to
which they are not)
4) that you have lots of data, because the propagation of errors tends to
(greatly) magnify the statistical fluctuations due to counting.

The sphere unfolding technique was very popular back in the 60's, but modern
wisdom places instead an emphasis on newer stereological techniques that
emphasize the design of specimen preparation techniques that avoid the sources of
bias and produce superior results. Read "Practical Stereology, 2nd Edition" by
Russ and Dehoff, or "Unbiased Stereology" by Howard and Reed, for more details
(or look up papers by Cruz-Orive in past issues of the Journal of Microscopy).

And lastly, no, your equation is wrong and won't work anyway.

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 18 19:51:03 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Gary Gaugler wrote:
====================================================================
.............What I do know is that if I switch to Au/Pd (60/40) or Pt, the
coating is amorphous and cannot be easily seen. Au coating can be seen at
about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
However, Au/Pd and Pt look totally different than Au alone. Au/Pd and Pt is
more granular rather than honeycomb. And it will look this way at 350KX and
greater.
====================================================================
Could you tell us the measurement used to conclude it is an amorphous
coating? So far as I know, one does see a grain, even with Pt or Au/Pd
irrrespective of the brand of sputter coater used.

Chuck

============================================
Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 18 20:53:08 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (johnpell-at-temple.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, April 18, 2004 at 19:54:26
---------------------------------------------------------------------------

Email: johnpell-at-temple.edu
Name: John Pell

Organization: Temple University

Title-Subject: [Microscopy] [Filtered] artifacts and blunders/Royal Rife

Question: I am an undergraduate student of biology at Temple University working on a pet research project on Royal Rife's microscopes for a microscopy class. I noticed a post on the Microscopy Listserve under the subject "artifacts and blunders" that contained an oblique reference to Rife. I would like to have more information characterizing Rife's blunders and the types of optical artifacts he saw through his scopes. Most of the websites with information about Rife are maintained by individuals or organizations concerned with mythologizing Rife's miraculous discovery of a cure for cancer using "vibrational energy." A critical discussion of the optical principles Rife may have used or misused does not seem to be a priority for them. If someone would point me towards such a discussion, or some of the information that could be used to construct such a discussion, I would be much obliged.

Thanks,

John Pell

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Apr 18 22:16:49 2004

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Using an FEI Sirion SFEG, the coating is amorphous.
The "measurement" is looking at the image via the SEM.
Plain Au is honeycombed. Would you like a sample of
this? See what you can see at 350KX. What would you
use to do this yourself? Let's compare images.
If it would be productive, of course.

How do we define amorphous versus non-amorphous
at this mag? This is further complicated by the
manner in which the coating is deposited. There
are way too many variables. Perhaps I simplify
the topic.

So, what do you want to see? I can produce pix
at 350KX of Au and Au/Pd coatings. If these are
a big surprise to you, I can provide specimen images.
Alternatively, show me what you have at this same
mag. Produce Au and Au/Pd and Pt images. That pretty well
covers the normal sputter coating environment.

I am always open to new views on this subject.

gary g.

At 07:12 PM 4/18/2004, you wrote:

} -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
}
} Gary Gaugler wrote:
} ====================================================================
} .............What I do know is that if I switch to Au/Pd (60/40) or Pt, the
} coating is amorphous and cannot be easily seen. Au coating can be seen at
} about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
} However, Au/Pd and Pt look totally different than Au alone. Au/Pd and Pt is
} more granular rather than honeycomb. And it will look this way at 350KX and
} greater.
} ====================================================================
} Could you tell us the measurement used to conclude it is an amorphous
} coating? So far as I know, one does see a grain, even with Pt or Au/Pd
} irrrespective of the brand of sputter coater used.
}
} Chuck
}
} ============================================
} Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} President 1-800-2424-SPI
} SPI SUPPLIES FAX: 1-610-436-5755
} PO BOX 656 e-mail:cgarber-at-2spi.com
} West Chester, PA 19381-0656 USA
} Cust.Service: spi2spi-at-2spi.com
}
} Look for us!
} ########################
} WWW: http://www.2spi.com
} ########################
} ============================================

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 07:12:25 2004

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Gary

If you are truely producing amorphous Au this would
be very significant. I must admit to being somewhat
skeptical.

An image of a near feature less "surface" is not sufficient
evidence to call something amorphous.

The best way to answer this question would be to prepare
a TEM cross-section. Then using either HREM or Electron Diffraction from
the coating you could verify if the coating is crystalline
or not.

Nestor

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 08:33:51 2004

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Contamination control of airborne dust, although not of concern for massive
samples or non-trace analysis, is of concern often enough at our
laboratory: Particularly with unknowns and when we are micromanipulating a
one-of-a-kind particle that can be confused with contaminants; when using
filtration procedures for trace quantities of particulate samples that
involve the filtering of large volumes of air; when conducting ultra-trace
component analysis within a microgram of a powder; or when developing
certain standard reference materials. Unwanted dust can add many days to
sample preparation or analysis, or can jeopardize a sample or an analysis,
making it an expensive problem if it occurs. For these reasons we
sometimes use cleanrooms and contamination control protocols with specially
trained staff, sometimes learning what is needed the hard way.

How prevalent is the need for contamination control at other facilities,
knowing there will be differences in environments and analytical goals? It
would be interesting if others would care to share experiences about the
significance of ambient dust in specimens, and what approaches to control
seem adequate for their particular case.

Thanks,
Cynthia Zeissler
Analytical Microscopy Group, NIST
Gaithersburg MD

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 08:38:57 2004

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I've been tasked with pulling together sensible specifications for a new
computer to capture digital images from our pol scope. Many options appear
to be straight forward:
More RAM, - 512 MB seems to be enough.
More HD storage, - As Daisy use to say, you can never be too rich,
too thin or have enough storage. I think 120GB is enough.
CD burner at 48X seems enough

but which monitor?
Should I look for a fast response time, say 16ms, to help me focus?
Are flat screens better for viewing than the more traditional monitors?
Do I need more then 17 inch diagonal screen?
Is the integrated Intel 3D Extreme Graphics video card a good choice for
photomicrography?

Any suggestions for a good driver to capture my images? I intend to use
photoshop to do any post imaging processing that needed, but I would like
to be able to do a little tweaking to maximize my images when I capture
them.

I have also inhered a Microimaging Video system and a RGB Automatic Camera,
but I have no instructions or user manual. If anyone knows a web site or
has a copy they would like to share I would be grateful!

Any advice, opinions or alternative suggestions are welcome!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 08:49:35 2004

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Hello all,

Thank you for all of your tips. I got some great responses with some really
good ideas to solve this problem.

To clear up some questions: All images that I see this problem with are
acquired when the beam is off (no intensity on the CCD), the images are also
raw (not dark count or gain corrected). The problem is not with an artifact
present in all CCD images, but rather the horizontal line profile of the
image (a measure of the average pixel value across the image horizontally)
increases from left to right.

What the solution may be: From responses I've received it may be that the
scintallator may have corroded from prolonged exposure to
condensation/contamination within the TEM column. We're going to try and
clean it off to rid ourselves of the problem.

Thanks again!

William Stratton

-------------------
William G. Stratton
Research Assistant
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 10:41:38 2004

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Nestor:

Indeed, amorphous likely means different things
to different folks and in different situations.
From a metallurgical or atomic standpoint, it
would mean that it lacks a definitive or distinct
crystalline structure--i.e., no lattice. On the
other hand, amorphous could mean that it is shapeless,
of no definite form or organization or methodical
arrangement.

OK, does this mean no form or organization at the
eye ball level? At the magnifying glass level?
LM, SEM, TEM level? I think that I "see" the
problem of definition and ability to define it.

The general consensus seems to be one of grains.
A honey comb shaped coating of Au would have the
metal portions containing or consisting of grains
of Au. Thus, the honey comb has organization and
methodical arrangement--not amorphous. And the
Au metal would have grains--not amorphous. Therefore,
sputtered Au is not amorphous.

Now to discuss Au/Pd. This material sputters
totally differently than Au alone. The coating
is like a layer of grains of sand. These dots,
if you will, may touch one another in places and
not in others. Unlike reflowed metal, the dots
are distinct and quite 3-D. Is this an amorphous
layer? If each dot was one grain, and each grain
was not touching each other grain, is the coating
amorphous or not? Does continuity play into the
definition?

At damascene vias, the ILD is definitely amorphous.
These areas etch totally differently than areas
away from the vias. It's interesting to see that
areas away from vias exhibit some degree of
amorphousness. Why the via areas are more strongly
amorphous, I do not yet know. This is something
I am working on at the moment.

If I can find some Au and Au/Pd pix that I can
post, I will do so. I have the pix somewhere and
I have specimens (all over the place). If there
is interest, I will work on getting them.

gary g.

At 05:34 AM 4/19/2004, you wrote:
} Gary
}
} If you are truely producing amorphous Au this would
} be very significant. I must admit to being somewhat
} skeptical.
}
} An image of a near feature less "surface" is not sufficient
} evidence to call something amorphous.
}
} The best way to answer this question would be to prepare
} a TEM cross-section. Then using either HREM or Electron Diffraction from
} the coating you could verify if the coating is crystalline
} or not.
}
}
} Nestor
}
}
}
} } -------------------------------------------------------------------------
} -----
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------
} ------
} }
} } Using an FEI Sirion SFEG, the coating is amorphous.
} } The "measurement" is looking at the image via the SEM.
} } Plain Au is honeycombed. Would you like a sample of
} } this? See what you can see at 350KX. What would you
} } use to do this yourself? Let's compare images.
} } If it would be productive, of course.
} }
} } How do we define amorphous versus non-amorphous
} } at this mag? This is further complicated by the
} } manner in which the coating is deposited. There
} } are way too many variables. Perhaps I simplify
} } the topic.
} }
} } So, what do you want to see? I can produce pix
} } at 350KX of Au and Au/Pd coatings. If these are
} } a big surprise to you, I can provide specimen images.
} } Alternatively, show me what you have at this same
} } mag. Produce Au and Au/Pd and Pt images. That pretty well
} } covers the normal sputter coating environment.
} }
} } I am always open to new views on this subject.
} }
} } gary g.
} }
} }
} } At 07:12 PM 4/18/2004, you wrote:
} }
} } } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} } }
} } } Gary Gaugler wrote:
} } } ====================================================================
} } } .............What I do know is that if I switch to Au/Pd (60/40) or Pt, the
} } } coating is amorphous and cannot be easily seen. Au coating can be seen at
} } } about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
} } } However, Au/Pd and Pt look totally different than Au alone. Au/Pd and
} Pt is
} } } more granular rather than honeycomb. And it will look this way at
} 350KX and
} } } greater.
} } } ====================================================================
} } } Could you tell us the measurement used to conclude it is an amorphous
} } } coating? So far as I know, one does see a grain, even with Pt or Au/Pd
} } } irrrespective of the brand of sputter coater used.
} } }
} } } Chuck
} } }
} } } ============================================
} } } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } } President 1-800-2424-SPI
} } } SPI SUPPLIES FAX: 1-610-436-5755
} } } PO BOX 656 e-mail:cgarber-at-2spi.com
} } } West Chester, PA 19381-0656 USA
} } } Cust.Service: spi2spi-at-2spi.com
} } }
} } } Look for us!
} } } ########################
} } } WWW: http://www.2spi.com
} } } ########################
} } } ============================================

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 10:45:03 2004

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Hi John:

I had never heard of Rife until some guy got on this list last year
raving about why all of us so-called scientists had ignored Rife's
contributions to science/microscopy/medicine.When I asked him what
exactly Rife's contributions were, I got a few websites (long since
deleted) but no real evidence or references in the literature. I did
read one website which I suspect a Google search could bring up. Once I
waded through 5-6 pages of unsubstantiated claims, I did find some
discussion of his microscope. While the complexity of the instrument was
somewhat impressive, the images it delivered were not. I think the
"optical principles" involved were largely products of Rife's imagination.
My general impression of the reaction of working scientists to
people like Rife is one of dismissal. Since the evidence offered is
usually imaginary or artifactual, those who work in the field in
question don't bother to refute the "evidence" (most of us have better
things to do). Unfortunately, this leads the gulible to accuse the
scientific community of a conspiracy since it can't "refute" the work of
the soon to be demi-god. The web has made the propagation of theories
about Rife much easier.
Good luck with your project.

Geoff

by way of MicroscopyListserver wrote:

} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (johnpell-at-temple.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, April 18, 2004 at 19:54:26
} ---------------------------------------------------------------------------
}
} Email: johnpell-at-temple.edu
} Name: John Pell
}
} Organization: Temple University
}
} Title-Subject: [Microscopy] [Filtered] artifacts and blunders/Royal Rife
}
} Question: I am an undergraduate student of biology at Temple University working on a pet research project on Royal Rife's microscopes for a microscopy class. I noticed a post on the Microscopy Listserve under the subject "artifacts and blunders" that contained an oblique reference to Rife. I would like to have more information characterizing Rife's blunders and the types of optical artifacts he saw through his scopes. Most of the websites with information about Rife are maintained by individuals or organizations concerned with mythologizing Rife's miraculous discovery of a cure for cancer using "vibrational energy." A critical discussion of the optical principles Rife may have used or misused does not seem to be a priority for them. If someone would point me towards such a discussion, or some of the information that could be used to construct such a discussion, I would be much obliged.
}
} Thanks,
}
} John Pell
}
}
} ---------------------------------------------------------------------------
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 10:55:22 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have to agree with Nestor.

We recently produces a very thin coating of Ni and TiO2 that was sputtered simultaneously using a Edwards sputtering system. According to other publications these should be Polycrystalline. In the Tecnai 12 the diffraction the pattern was amorphous. We were pleased since the polycrystalline samples we proved can be introduced by beam damage (Remove C1 aperature) and that introduced a polycrystalline sample. Beautiful artefact. Still were not convinced that the film was amorphous. The sample was examined at fei Netherlands on the Technai G2 equipped with a FEG gun, a beauty. It proven to be nano crystals. We are still waiting for the final data set from fei. I would not be surprised if the Gold film follows the same logic.

-----Original Message-----
} From: Nestor J. Zaluzec [mailto:zaluzec-at-microscopy.com]
Sent: Monday, April 19, 2004 2:35 PM
To: microscopy-at-ns.microscopy.com

Gary

If you are truely producing amorphous Au this would
be very significant. I must admit to being somewhat
skeptical.

An image of a near feature less "surface" is not sufficient
evidence to call something amorphous.

The best way to answer this question would be to prepare
a TEM cross-section. Then using either HREM or Electron Diffraction from
the coating you could verify if the coating is crystalline
or not.

Nestor

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 11:38:15 2004

Contents Retrieved from Microscopy Listserver Archives
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TEM Analyst Position
---------------------
A position is open for a Transmission Electron Microscopy Analyst in the Process Characterization Group at International SEMATECH in Austin, Texas.

Our group provides technical support to research and development projects at International SEMATECH (www.sematech.org). The analyst would interface with engineers and project managers, determine analytical plans, conduct analyses, and interpret and present data. The work involves characterization of materials systems new to the semiconductor industry and there is significant opportunity to do interesting and publishable science. Our business plan allows significant opportunities for collaboration and visibility within the industry as well as the materials and microscopy academic communities.

Our toolset includes two 300 keV TEM's (one FEG, one LaB6), with SUTW-EDX, GIF, multiple HAADF-STEM and CCD cameras. Our sample preparation toolset includes several PIPS and Duomill tools as well as 2 FEI FIB systems.

This is a temporary position (1 year renewable contract) with benefits. Preference made to qualified persons willing to work off-shift.

Interested parties should reply offline to Brendan.Foran-at-Sematech.Org
-------------------

Sincerely,
Brendan
-----------------------------------------------
Brendan Foran, Ph.D.
Senior Member Technical Staff
Transmission Electron Microscopy Group Leader
Process Characterization Lab- ATDF
International SEMATECH
phone (512) 356-3936
-----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 11:41:30 2004

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Frank,

I would definitely add more RAM---at least a gigabyte, I would think.
Some of the images I work with are over 140MB and a few images running
in Photoshop can gobble memory like there's no tomorrow. And if you're
doing video, it's even worse. I would also get the highest speed
processor I could afford. The 2.8 gigahertz processors are fairly
reasonable, and since I built my computer I think the 3.0+ GHZ
processors are starting to come down. In terms of the monitor, I'm told
that CRT's still have a thin edge over flat panels for image quality,
plus a huge advantage in price, but the flats are getting better all the
time. BIG monitors are definitely nicer, though, and that's where CRTs
can save large amounts of money over flat panels. Finally, I would
consider a DVD or combo burner to increase storage capacity for your
images. Big files fill up a CD pretty quickly.

Hope this helps. Good luck.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

-----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
Sent: Monday, April 19, 2004 8:35 AM
To: microscopy-at-msa.microscopy.com

I've been tasked with pulling together sensible specifications for a new
computer to capture digital images from our pol scope. Many options
appear to be straight forward:
More RAM, - 512 MB seems to be enough.
More HD storage, - As Daisy use to say, you can never be too rich,
too thin or have enough storage. I think 120GB is enough.
CD burner at 48X seems enough

but which monitor?
Should I look for a fast response time, say 16ms, to help me focus? Are
flat screens better for viewing than the more traditional monitors? Do I
need more then 17 inch diagonal screen? Is the integrated Intel 3D
Extreme Graphics video card a good choice for photomicrography?

Any suggestions for a good driver to capture my images? I intend to use
photoshop to do any post imaging processing that needed, but I would
like to be able to do a little tweaking to maximize my images when I
capture them.

I have also inhered a Microimaging Video system and a RGB Automatic
Camera, but I have no instructions or user manual. If anyone knows a
web site or has a copy they would like to share I would be grateful!

Any advice, opinions or alternative suggestions are welcome!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 13:52:35 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Get the fastest P4 you can afford. 2.66GHz or
3GHz. Get at least 1GB DDR RAM. The motherboard
will likely have three DIMM slots, so put in
three 512MB PC2700 DDR DIMMs--1.5GB. Its FSB
should handle these.

Put in two hard drives. Dual 120G is good.
Set up D: as Photoshop's scratch disk. This way
PS will work very fast since it does not have to
use C: for work and scratch. Plus, I tend to keep
data on D: and programs on C:. This way, backup
is done mostly of D:.

For optical, I think that optimum is Plextor Premium
along with Panasonic DVR-106D DVD-R/RW-CD-R/RW.
If you don't get the DVD burner, get a DVD-ROM drive
at least. The DVD burner is excellent for big backups.
Also get Roxio's newest Version 7 burning software. It
is a major improvement over Version 6. The 106D
will write 4X DVDs. And it also becomes a backup
burner for CDs.

I'd recommend not using on-board video. If it fails,
you are dead. Get an Nvidea/ASUS GeForce FX5200 8X
AGP 128MB. Fast and offloads CPU a lot. Integrated
usually means on-board rather than a separate board.
If separate, it is probably OK.

Also, go with WindowsXP Pro over Win2K Pro. XP is
a new OS rather than an update of 2K. Very stable
and reliable. 2K is good too but XP is later
and has more features.

Flat screen CRTs are my favorite. I use a Sony
Multiscan E500 21". There are newer models. For
images, it is great. For my camera capture system,
I use Samsung 191t TFT/LCD. PS7 and image processing
is done on the CRT system. If you will have only
one system, I recommend CRT. The 21" units are
HEAVY! Refresh rate is 80Hz. No flicker.

gary g.

At 06:34 AM 4/19/2004, you wrote:

} I've been tasked with pulling together sensible specifications for a new
} computer to capture digital images from our pol scope. Many options appear
} to be straight forward:
} More RAM, - 512 MB seems to be enough.
} More HD storage, - As Daisy use to say, you can never be too rich,
} too thin or have enough storage. I think 120GB is enough.
} CD burner at 48X seems enough
}
} but which monitor?
} Should I look for a fast response time, say 16ms, to help me focus?
} Are flat screens better for viewing than the more traditional monitors?
} Do I need more then 17 inch diagonal screen?
} Is the integrated Intel 3D Extreme Graphics video card a good choice for
} photomicrography?
}
} Any suggestions for a good driver to capture my images? I intend to use
} photoshop to do any post imaging processing that needed, but I would like
} to be able to do a little tweaking to maximize my images when I capture
} them.
}
} I have also inhered a Microimaging Video system and a RGB Automatic Camera,
} but I have no instructions or user manual. If anyone knows a web site or
} has a copy they would like to share I would be grateful!
}
} Any advice, opinions or alternative suggestions are welcome!
}
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 14:06:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

William,

you need to be VERY careful if you try to do something with the Phosphor. It
can be damaged beyond repair very easily.

You mention that you get a signal from the camera with the beam off. What is
the exposure time? Usually the phosphor is covered with a thin metallic
layer to provide conductivity and block photons. One of the reasons for your
"shadow" might be an uneven thickness of this layer. What do you see if you
darken the TEM room completely and increase exposure time until you see
something?

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: William Stratton [mailto:wgstratton-at-wisc.edu]
Sent: Monday, April 19, 2004 08:11
To: Microscopy

Hello all,

Thank you for all of your tips. I got some great responses with some really
good ideas to solve this problem.

To clear up some questions: All images that I see this problem with are
acquired when the beam is off (no intensity on the CCD), the images are also
raw (not dark count or gain corrected). The problem is not with an artifact
present in all CCD images, but rather the horizontal line profile of the
image (a measure of the average pixel value across the image horizontally)
increases from left to right.

What the solution may be: From responses I've received it may be that the
scintallator may have corroded from prolonged exposure to
condensation/contamination within the TEM column. We're going to try and
clean it off to rid ourselves of the problem.

Thanks again!

William Stratton

-------------------
William G. Stratton
Research Assistant
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 15:25:24 2004

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One of our users has come to us with a sticky problem.

Her siRNA transfections look great in live cells, but after fixation and
immunostaining there are red dots everywhere, all over the coverslip
(polylysine coated), all over the cells, and in the cells.

Anybody else encounter this problem?

Thanks.
____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 20:39:25 2004

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To All:

The question about whether coatings deposited using a sputter coater are
'amorphous' or 'crystalline' seems to be in dispute here. On an atomic
level, if you can make an amorphous metal then we should be able to image it
in our high resolution TEM (JEOL 4000EX) and not find the orderly
arrangement of atoms in the layers. For gold deposited on amorphous
(definitely) silicon, we can see easily at 800kX (5MX final mag) that the
gold 'islands' of about 5nm diameter are composed of crystalline gold with
each atom being able to be identified and counted in the orderly structure.
We do the same thing at interfaces in semiconductor devices to note the
changes of atomic structure where two metal system combine. It should also
be noted that if the layer is thin enough, the diffraction pattern is hard
to find (very weak signal) but with a long enough dwell time you will
definitely see that the metal layer has atomic level crystalline structure.

The argument that seems to be being presented here is semantic, not
scientific. Whether or not a layer appears as a 'honeycomb' has nothing to
do with the fact that the structure of the 'honeycomb' is crystalline or
amorphous. For the purposes of SEM the ideal is to have an 'amorphous'
layer from the standpoint that at the magnifications involved there is no
contribution of 'ordered' structures from the coating. This has absolutely
nothing to do with whether or not the atomic level structures are
crystalline or amorphous. We routinely coat samples with whatever material
is best suited for the images we want to obtain. That might be gold, Au/Pd,
Cr, Ag, Ti or whatever else seems to work. For Auger work we even use
deposited Li to eliminate charging without contributing significantly to the
spectral data. For SEM you are striving to achieve a coating that allows
imaging of your actual sample without adding 'artifacts' that will confuse
the interpretation of your data. If that means that you deposit a
gold/palladium or chromium layer with such fine structure that your SEM
image sees only the information from your sample but doesn't present an
artifact then, by all means, call it 'amorphous'. A more distinctive
description might, however, be 'uniform' at the magnification used. By this
definition the actual atomic level crystallinity of the layer is not called
into question. If you really want to know about the atomic scale ordering
then you need to move on to HRTEM since SEM is not sufficient to see the
atomic scale features. You could also use atomic force microscopy to 'see'
the atomic structure of your surface coating.

Drew Hirt
Materials Research Laboratories, Inc.
Tel (800) 424-1776
Fax (330) 750-0776
drew-at-hirt.com
http://www.mrllab.com

on 4/19/04 11:57 AM, Gary Gaugler at gary-at-gaugler.com wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Nestor:
}
} Indeed, amorphous likely means different things
} to different folks and in different situations.
} From a metallurgical or atomic standpoint, it
} would mean that it lacks a definitive or distinct
} crystalline structure--i.e., no lattice. On the
} other hand, amorphous could mean that it is shapeless,
} of no definite form or organization or methodical
} arrangement.
}
} OK, does this mean no form or organization at the
} eye ball level? At the magnifying glass level?
} LM, SEM, TEM level? I think that I "see" the
} problem of definition and ability to define it.
}
} The general consensus seems to be one of grains.
} A honey comb shaped coating of Au would have the
} metal portions containing or consisting of grains
} of Au. Thus, the honey comb has organization and
} methodical arrangement--not amorphous. And the
} Au metal would have grains--not amorphous. Therefore,
} sputtered Au is not amorphous.
}
} Now to discuss Au/Pd. This material sputters
} totally differently than Au alone. The coating
} is like a layer of grains of sand. These dots,
} if you will, may touch one another in places and
} not in others. Unlike reflowed metal, the dots
} are distinct and quite 3-D. Is this an amorphous
} layer? If each dot was one grain, and each grain
} was not touching each other grain, is the coating
} amorphous or not? Does continuity play into the
} definition?
}
} At damascene vias, the ILD is definitely amorphous.
} These areas etch totally differently than areas
} away from the vias. It's interesting to see that
} areas away from vias exhibit some degree of
} amorphousness. Why the via areas are more strongly
} amorphous, I do not yet know. This is something
} I am working on at the moment.
}
} If I can find some Au and Au/Pd pix that I can
} post, I will do so. I have the pix somewhere and
} I have specimens (all over the place). If there
} is interest, I will work on getting them.
}
} gary g.
}
}
}
}
}
} At 05:34 AM 4/19/2004, you wrote:
} } Gary
} }
} } If you are truely producing amorphous Au this would
} } be very significant. I must admit to being somewhat
} } skeptical.
} }
} } An image of a near feature less "surface" is not sufficient
} } evidence to call something amorphous.
} }
} } The best way to answer this question would be to prepare
} } a TEM cross-section. Then using either HREM or Electron Diffraction from
} } the coating you could verify if the coating is crystalline
} } or not.
} }
} }
} } Nestor
} }
} }
} }
} } } -------------------------------------------------------------------------
} } -----
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } -------------------------------------------------------------------------
} } ------
} } }
} } } Using an FEI Sirion SFEG, the coating is amorphous.
} } } The "measurement" is looking at the image via the SEM.
} } } Plain Au is honeycombed. Would you like a sample of
} } } this? See what you can see at 350KX. What would you
} } } use to do this yourself? Let's compare images.
} } } If it would be productive, of course.
} } }
} } } How do we define amorphous versus non-amorphous
} } } at this mag? This is further complicated by the
} } } manner in which the coating is deposited. There
} } } are way too many variables. Perhaps I simplify
} } } the topic.
} } }
} } } So, what do you want to see? I can produce pix
} } } at 350KX of Au and Au/Pd coatings. If these are
} } } a big surprise to you, I can provide specimen images.
} } } Alternatively, show me what you have at this same
} } } mag. Produce Au and Au/Pd and Pt images. That pretty well
} } } covers the normal sputter coating environment.
} } }
} } } I am always open to new views on this subject.
} } }
} } } gary g.
} } }
} } }
} } } At 07:12 PM 4/18/2004, you wrote:
} } }
} } } } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} } } }
} } } } Gary Gaugler wrote:
} } } } ====================================================================
} } } } .............What I do know is that if I switch to Au/Pd (60/40) or Pt, the
} } } } coating is amorphous and cannot be easily seen. Au coating can be seen at
} } } } about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
} } } } However, Au/Pd and Pt look totally different than Au alone. Au/Pd and
} } Pt is
} } } } more granular rather than honeycomb. And it will look this way at
} } 350KX and
} } } } greater.
} } } } ====================================================================
} } } } Could you tell us the measurement used to conclude it is an amorphous
} } } } coating? So far as I know, one does see a grain, even with Pt or Au/Pd
} } } } irrrespective of the brand of sputter coater used.
} } } }
} } } } Chuck
} } } }
} } } } ============================================
} } } } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } } } President 1-800-2424-SPI
} } } } SPI SUPPLIES FAX: 1-610-436-5755
} } } } PO BOX 656 e-mail:cgarber-at-2spi.com
} } } } West Chester, PA 19381-0656 USA
} } } } Cust.Service: spi2spi-at-2spi.com
} } } }
} } } } Look for us!
} } } } ########################
} } } } WWW: http://www.2spi.com
} } } } ########################
} } } } ============================================
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 21:14:33 2004

Contents Retrieved from Microscopy Listserver Archives
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Whoa, I did not intend for this to get way
off base, out of hand, perverted, convoluted,
complicated, ...fill in the adjectives.

Post: This is the point of issue. There is a fine structure
of the coating. At low mag, it cannot be seen. At
high mag, it can be seen. Is it an "artifact?" No.
It is real. But then, we need to define an artifact
in the context of coating, et. al. As Nestor and
Charles said, it is an issue of grains. This is
bounded. We can deal with this.

If the SEM sees information of the coating, then what?
It is not an artifact. Furthermore, what does "uniform"
mean? It seems that your posting says that in
one case the coating is amorphous but in another
it is not...based on mag and artifacts. But "uniform"
is counter-amorphous... sigh.

I think we are headed towards making a mountain out
of a mole hill. Perhaps we should let this dog lay.
If not, Nestor will keep us on track. Notwithstanding,
I will do some EBSD studies later this year and report
back to the list.

gary g.

At 07:01 PM 4/19/2004, you wrote:
} To All:
}
} [snip] If that means that you deposit a
} gold/palladium or chromium layer with such fine structure that your SEM
} image sees only the information from your sample but doesn't present an
} artifact then, by all means, call it 'amorphous'. A more distinctive
} description might, however, be 'uniform' at the magnification used. By this
} definition the actual atomic level crystallinity of the layer is not called
} into question. If you really want to know about the atomic scale ordering
} then you need to move on to HRTEM since SEM is not sufficient to see the
} atomic scale features. You could also use atomic force microscopy to 'see'
} the atomic structure of your surface coating.
}
} Drew Hirt
} Materials Research Laboratories, Inc.
} Tel (800) 424-1776
} Fax (330) 750-0776
} drew-at-hirt.com
} http://www.mrllab.com
}
}
} on 4/19/04 11:57 AM, Gary Gaugler at gary-at-gaugler.com wrote:
}
} }
} }
} }
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ----------------------------------------------------------------------------
} --} -
} }
} } Nestor:
} }
} } Indeed, amorphous likely means different things
} } to different folks and in different situations.
} } From a metallurgical or atomic standpoint, it
} } would mean that it lacks a definitive or distinct
} } crystalline structure--i.e., no lattice. On the
} } other hand, amorphous could mean that it is shapeless,
} } of no definite form or organization or methodical
} } arrangement.
} }
} } OK, does this mean no form or organization at the
} } eye ball level? At the magnifying glass level?
} } LM, SEM, TEM level? I think that I "see" the
} } problem of definition and ability to define it.
} }
} } The general consensus seems to be one of grains.
} } A honey comb shaped coating of Au would have the
} } metal portions containing or consisting of grains
} } of Au. Thus, the honey comb has organization and
} } methodical arrangement--not amorphous. And the
} } Au metal would have grains--not amorphous. Therefore,
} } sputtered Au is not amorphous.
} }
} } Now to discuss Au/Pd. This material sputters
} } totally differently than Au alone. The coating
} } is like a layer of grains of sand. These dots,
} } if you will, may touch one another in places and
} } not in others. Unlike reflowed metal, the dots
} } are distinct and quite 3-D. Is this an amorphous
} } layer? If each dot was one grain, and each grain
} } was not touching each other grain, is the coating
} } amorphous or not? Does continuity play into the
} } definition?
} }
} } At damascene vias, the ILD is definitely amorphous.
} } These areas etch totally differently than areas
} } away from the vias. It's interesting to see that
} } areas away from vias exhibit some degree of
} } amorphousness. Why the via areas are more strongly
} } amorphous, I do not yet know. This is something
} } I am working on at the moment.
} }
} } If I can find some Au and Au/Pd pix that I can
} } post, I will do so. I have the pix somewhere and
} } I have specimens (all over the place). If there
} } is interest, I will work on getting them.
} }
} } gary g.
} }
} }
} }
} }
} }
} } At 05:34 AM 4/19/2004, you wrote:
} } } Gary
} } }
} } } If you are truely producing amorphous Au this would
} } } be very significant. I must admit to being somewhat
} } } skeptical.
} } }
} } } An image of a near feature less "surface" is not sufficient
} } } evidence to call something amorphous.
} } }
} } } The best way to answer this question would be to prepare
} } } a TEM cross-section. Then using either HREM or Electron Diffraction from
} } } the coating you could verify if the coating is crystalline
} } } or not.
} } }
} } }
} } } Nestor
} } }
} } }
} } }
} } } } -------------------------------------------------------------------------
} } } -----
} } } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } } -------------------------------------------------------------------------
} } } ------
} } } }
} } } } Using an FEI Sirion SFEG, the coating is amorphous.
} } } } The "measurement" is looking at the image via the SEM.
} } } } Plain Au is honeycombed. Would you like a sample of
} } } } this? See what you can see at 350KX. What would you
} } } } use to do this yourself? Let's compare images.
} } } } If it would be productive, of course.
} } } }
} } } } How do we define amorphous versus non-amorphous
} } } } at this mag? This is further complicated by the
} } } } manner in which the coating is deposited. There
} } } } are way too many variables. Perhaps I simplify
} } } } the topic.
} } } }
} } } } So, what do you want to see? I can produce pix
} } } } at 350KX of Au and Au/Pd coatings. If these are
} } } } a big surprise to you, I can provide specimen images.
} } } } Alternatively, show me what you have at this same
} } } } mag. Produce Au and Au/Pd and Pt images. That pretty well
} } } } covers the normal sputter coating environment.
} } } }
} } } } I am always open to new views on this subject.
} } } }
} } } } gary g.
} } } }
} } } }
} } } } At 07:12 PM 4/18/2004, you wrote:
} } } }
} } } } } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} } } } }
} } } } } Gary Gaugler wrote:
} } } } } ====================================================================
} } } } } .............What I do know is that if I switch to Au/Pd (60/40) or
} Pt, the
} } } } } coating is amorphous and cannot be easily seen. Au coating can be
} seen at
} } } } } about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
} } } } } However, Au/Pd and Pt look totally different than Au alone. Au/Pd and
} } } Pt is
} } } } } more granular rather than honeycomb. And it will look this way at
} } } 350KX and
} } } } } greater.
} } } } } ====================================================================
} } } } } Could you tell us the measurement used to conclude it is an amorphous
} } } } } coating? So far as I know, one does see a grain, even with Pt or Au/Pd
} } } } } irrrespective of the brand of sputter coater used.
} } } } }
} } } } } Chuck
} } } } }
} } } } } ============================================
} } } } } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } } } } President 1-800-2424-SPI
} } } } } SPI SUPPLIES FAX: 1-610-436-5755
} } } } } PO BOX 656 e-mail:cgarber-at-2spi.com
} } } } } West Chester, PA 19381-0656 USA
} } } } } Cust.Service: spi2spi-at-2spi.com
} } } } }
} } } } } Look for us!
} } } } } ########################
} } } } } WWW: http://www.2spi.com
} } } } } ########################
} } } } } ============================================
} }
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 21:28:32 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mmckillip-at-smurfitlcom) from on Monday, April 19, 2004 at 11:39:07
---------------------------------------------------------------------------

Email: mmckillip-at-smurfitlcom
Name: M McKillip

Organization: Smurfit Stone Container Corp

Title-Subject: [Microscopy] [Filtered] MListserver:Embedding polymer films

Question: Is there a method to enhance polymer film bonding to a Poly/Bed 812 embedding medium. Frequently the thin films release from the embedding medium during microtoming.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 22:22:17 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Gary:

My intent was to try to put this into some kind of reasonable perspective.
An 'artifact' in SEM is anything induced by the sample prep that is not
representative of the actual sample you are studying. The whole point of
development in coating systems has historically been to reduce the artifacts
that are induced. The argument about whether to use gold (the age-old
standard) or gold-palladium addresses the fact that gold alone produces
grains (structures) that are visible at relatively low magnifications (let's
say about 20kX). With Au-Pd you can get to higher magnifications before
this becomes a problem. Are they really there in your image? Yes. Are
they representative of your sample? No. That's why they are called
'artifacts'. If you are seeing the coating then, yes, there is a fine
structure of the coating, whether it is 'grains' or 'honeycombs' or anything
else. The goal of the coating is that there is no fine structure that can
be misinterpreted as a characteristic of the actual sample. Again, none of
this discussion has anything to do with 'crystallinity' and the use of
'amorphous' is apparently ambiguous in this case. I suggested 'uniform'
but, again, all of your discussions so far have been aimed at suggesting
that the 'smooth', 'uniform' and 'essentially invisible' coating on your
sample is 'amorphous'. This is an attempt to get to the basic issue and
leave out the semantics and confusion that seem to have crept in.

Drew Hirt
Materials Research Laboratories, Inc.
Tel (800) 424-1776
Fax (330) 750-0776
drew-at-hirt.com
http://www.mrllab.com

on 4/19/04 10:35 PM, Gary Gaugler at gary-at-gaugler.com wrote:

} Whoa, I did not intend for this to get way
} off base, out of hand, perverted, convoluted,
} complicated, ...fill in the adjectives.
}
} Post: This is the point of issue. There is a fine structure
} of the coating. At low mag, it cannot be seen. At
} high mag, it can be seen. Is it an "artifact?" No.
} It is real. But then, we need to define an artifact
} in the context of coating, et. al. As Nestor and
} Charles said, it is an issue of grains. This is
} bounded. We can deal with this.
}
} If the SEM sees information of the coating, then what?
} It is not an artifact. Furthermore, what does "uniform"
} mean? It seems that your posting says that in
} one case the coating is amorphous but in another
} it is not...based on mag and artifacts. But "uniform"
} is counter-amorphous... sigh.
}
} I think we are headed towards making a mountain out
} of a mole hill. Perhaps we should let this dog lay.
} If not, Nestor will keep us on track. Notwithstanding,
} I will do some EBSD studies later this year and report
} back to the list.
}
} gary g.
}
}
} At 07:01 PM 4/19/2004, you wrote:
} } To All:
} }
} } [unsnip]

The question about whether coatings deposited using a sputter coater are
'amorphous' or 'crystalline' seems to be in dispute here. On an atomic
level, if you can make an amorphous metal then we should be able to image it
in our high resolution TEM (JEOL 4000EX) and not find the orderly
arrangement of atoms in the layers. For gold deposited on amorphous
(definitely) silicon, we can see easily at 800kX (5MX final mag) that the
gold 'islands' of about 5nm diameter are composed of crystalline gold with
each atom being able to be identified and counted in the orderly structure.
We do the same thing at interfaces in semiconductor devices to note the
changes of atomic structure where two metal system combine. It should also
be noted that if the layer is thin enough, the diffraction pattern is hard
to find (very weak signal) but with a long enough dwell time you will
definitely see that the metal layer has atomic level crystalline structure.

The argument that seems to be being presented here is semantic, not
scientific. Whether or not a layer appears as a 'honeycomb' has nothing to
do with the fact that the structure of the 'honeycomb' is crystalline or
amorphous. For the purposes of SEM the ideal is to have an 'amorphous'
layer from the standpoint that at the magnifications involved there is no
contribution of 'ordered' structures from the coating. This has absolutely
nothing to do with whether or not the atomic level structures are
crystalline or amorphous. We routinely coat samples with whatever material
is best suited for the images we want to obtain. That might be gold, Au/Pd,
Cr, Ag, Ti or whatever else seems to work. For Auger work we even use
deposited Li to eliminate charging without contributing significantly to the
spectral data. For SEM you are striving to achieve a coating that allows
imaging of your actual sample without adding 'artifacts' that will confuse
the interpretation of your data. If that means that you deposit a
} } gold/palladium or chromium layer with such fine structure that your SEM
} } image sees only the information from your sample but doesn't present an
} } artifact then, by all means, call it 'amorphous'. A more distinctive
} } description might, however, be 'uniform' at the magnification used. By this
} } definition the actual atomic level crystallinity of the layer is not called
} } into question. If you really want to know about the atomic scale ordering
} } then you need to move on to HRTEM since SEM is not sufficient to see the
} } atomic scale features. You could also use atomic force microscopy to 'see'
} } the atomic structure of your surface coating.
} }
} } Drew Hirt
} } Materials Research Laboratories, Inc.
} } Tel (800) 424-1776
} } Fax (330) 750-0776
} } drew-at-hirt.com
} } http://www.mrllab.com
} }
} }
} } on 4/19/04 11:57 AM, Gary Gaugler at gary-at-gaugler.com wrote:
} }
} } }
} } }
} } }
} }
----------------------------------------------------------------------------
-} } -
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } ----------------------------------------------------------------------------
} } --} -
} } }
} } } Nestor:
} } }
} } } Indeed, amorphous likely means different things
} } } to different folks and in different situations.
} } } From a metallurgical or atomic standpoint, it
} } } would mean that it lacks a definitive or distinct
} } } crystalline structure--i.e., no lattice. On the
} } } other hand, amorphous could mean that it is shapeless,
} } } of no definite form or organization or methodical
} } } arrangement.
} } }
} } } OK, does this mean no form or organization at the
} } } eye ball level? At the magnifying glass level?
} } } LM, SEM, TEM level? I think that I "see" the
} } } problem of definition and ability to define it.
} } }
} } } The general consensus seems to be one of grains.
} } } A honey comb shaped coating of Au would have the
} } } metal portions containing or consisting of grains
} } } of Au. Thus, the honey comb has organization and
} } } methodical arrangement--not amorphous. And the
} } } Au metal would have grains--not amorphous. Therefore,
} } } sputtered Au is not amorphous.
} } }
} } } Now to discuss Au/Pd. This material sputters
} } } totally differently than Au alone. The coating
} } } is like a layer of grains of sand. These dots,
} } } if you will, may touch one another in places and
} } } not in others. Unlike reflowed metal, the dots
} } } are distinct and quite 3-D. Is this an amorphous
} } } layer? If each dot was one grain, and each grain
} } } was not touching each other grain, is the coating
} } } amorphous or not? Does continuity play into the
} } } definition?
} } }
} } } At damascene vias, the ILD is definitely amorphous.
} } } These areas etch totally differently than areas
} } } away from the vias. It's interesting to see that
} } } areas away from vias exhibit some degree of
} } } amorphousness. Why the via areas are more strongly
} } } amorphous, I do not yet know. This is something
} } } I am working on at the moment.
} } }
} } } If I can find some Au and Au/Pd pix that I can
} } } post, I will do so. I have the pix somewhere and
} } } I have specimens (all over the place). If there
} } } is interest, I will work on getting them.
} } }
} } } gary g.
} } }
} } }
} } }
} } }
} } }
} } } At 05:34 AM 4/19/2004, you wrote:
} } } } Gary
} } } }
} } } } If you are truely producing amorphous Au this would
} } } } be very significant. I must admit to being somewhat
} } } } skeptical.
} } } }
} } } } An image of a near feature less "surface" is not sufficient
} } } } evidence to call something amorphous.
} } } }
} } } } The best way to answer this question would be to prepare
} } } } a TEM cross-section. Then using either HREM or Electron Diffraction from
} } } } the coating you could verify if the coating is crystalline
} } } } or not.
} } } }
} } } }
} } } } Nestor
} } } }
} } } }
} } } }
} } } } } -------------------------------------------------------------------------
} } } } -----
} } } } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } } } To Subscribe/Unsubscribe --
} } } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } } } -------------------------------------------------------------------------
} } } } ------
} } } } }
} } } } } Using an FEI Sirion SFEG, the coating is amorphous.
} } } } } The "measurement" is looking at the image via the SEM.
} } } } } Plain Au is honeycombed. Would you like a sample of
} } } } } this? See what you can see at 350KX. What would you
} } } } } use to do this yourself? Let's compare images.
} } } } } If it would be productive, of course.
} } } } }
} } } } } How do we define amorphous versus non-amorphous
} } } } } at this mag? This is further complicated by the
} } } } } manner in which the coating is deposited. There
} } } } } are way too many variables. Perhaps I simplify
} } } } } the topic.
} } } } }
} } } } } So, what do you want to see? I can produce pix
} } } } } at 350KX of Au and Au/Pd coatings. If these are
} } } } } a big surprise to you, I can provide specimen images.
} } } } } Alternatively, show me what you have at this same
} } } } } mag. Produce Au and Au/Pd and Pt images. That pretty well
} } } } } covers the normal sputter coating environment.
} } } } }
} } } } } I am always open to new views on this subject.
} } } } }
} } } } } gary g.
} } } } }
} } } } }
} } } } } At 07:12 PM 4/18/2004, you wrote:
} } } } }
} } } } } } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} } } } } }
} } } } } } Gary Gaugler wrote:
} } } } } } ====================================================================
} } } } } } .............What I do know is that if I switch to Au/Pd (60/40) or
} } Pt, the
} } } } } } coating is amorphous and cannot be easily seen. Au coating can be
} } seen at
} } } } } } about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
} } } } } } However, Au/Pd and Pt look totally different than Au alone. Au/Pd and
} } } } Pt is
} } } } } } more granular rather than honeycomb. And it will look this way at
} } } } 350KX and
} } } } } } greater.
} } } } } } ====================================================================
} } } } } } Could you tell us the measurement used to conclude it is an amorphous
} } } } } } coating? So far as I know, one does see a grain, even with Pt or Au/Pd
} } } } } } irrrespective of the brand of sputter coater used.
} } } } } }
} } } } } } Chuck
} } } } } }
} } } } } } ============================================
} } } } } } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } } } } } President 1-800-2424-SPI
} } } } } } SPI SUPPLIES FAX: 1-610-436-5755
} } } } } } PO BOX 656 e-mail:cgarber-at-2spi.com
} } } } } } West Chester, PA 19381-0656 USA
} } } } } } Cust.Service: spi2spi-at-2spi.com
} } } } } }
} } } } } } Look for us!
} } } } } } ########################
} } } } } } WWW: http://www.2spi.com
} } } } } } ########################
} } } } } } ============================================
} } }
} } }
} } }
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 19 22:37:59 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I'm in violent agreement with you. What is of
concern to me is that as I/we move to extreme
sub-micron dimensions such as 0.18u and below,
how does the coating affect what we see and
can present?

The problem is that at 0.5u and larger, the
coatings are not all that significant. However,
for extreme sub-micron feature sizes, I'm worried
about the coating. At what point does the coating
just exist and then become an artifact and then
cloud the specimen? Heisenberg uncertainty plays
into this...perhaps.

At 350KX and above, Au is not invisible...IMO.
Au/Pd is visible but looks different. Pt is
pretty much invisible. Os seems like a very
ideal coating. At 90nm, what is a good coating???

As semiconductor feature sizes continue to reduce,
how does this affect our procedures for analyzing them?
How do we analyze the specimens without having to
explain coatings? If we have to explain them, it
puts our findings into question...or argumentation
enters into the picture. This is not good.

gary g.

At 08:44 PM 4/19/2004, you wrote:
} Gary:
}
} My intent was to try to put this into some kind of reasonable perspective.
} An 'artifact' in SEM is anything induced by the sample prep that is not
} representative of the actual sample you are studying. The whole point of
} development in coating systems has historically been to reduce the artifacts
} that are induced. The argument about whether to use gold (the age-old
} standard) or gold-palladium addresses the fact that gold alone produces
} grains (structures) that are visible at relatively low magnifications (let's
} say about 20kX). With Au-Pd you can get to higher magnifications before
} this becomes a problem. Are they really there in your image? Yes. Are
} they representative of your sample? No. That's why they are called
} 'artifacts'. If you are seeing the coating then, yes, there is a fine
} structure of the coating, whether it is 'grains' or 'honeycombs' or anything
} else. The goal of the coating is that there is no fine structure that can
} be misinterpreted as a characteristic of the actual sample. Again, none of
} this discussion has anything to do with 'crystallinity' and the use of
} 'amorphous' is apparently ambiguous in this case. I suggested 'uniform'
} but, again, all of your discussions so far have been aimed at suggesting
} that the 'smooth', 'uniform' and 'essentially invisible' coating on your
} sample is 'amorphous'. This is an attempt to get to the basic issue and
} leave out the semantics and confusion that seem to have crept in.
}
} Drew Hirt
} Materials Research Laboratories, Inc.
} Tel (800) 424-1776
} Fax (330) 750-0776
} drew-at-hirt.com
} http://www.mrllab.com
}
}
}
} on 4/19/04 10:35 PM, Gary Gaugler at gary-at-gaugler.com wrote:
}
} } Whoa, I did not intend for this to get way
} } off base, out of hand, perverted, convoluted,
} } complicated, ...fill in the adjectives.
} }
} } Post: This is the point of issue. There is a fine structure
} } of the coating. At low mag, it cannot be seen. At
} } high mag, it can be seen. Is it an "artifact?" No.
} } It is real. But then, we need to define an artifact
} } in the context of coating, et. al. As Nestor and
} } Charles said, it is an issue of grains. This is
} } bounded. We can deal with this.
} }
} } If the SEM sees information of the coating, then what?
} } It is not an artifact. Furthermore, what does "uniform"
} } mean? It seems that your posting says that in
} } one case the coating is amorphous but in another
} } it is not...based on mag and artifacts. But "uniform"
} } is counter-amorphous... sigh.
} }
} } I think we are headed towards making a mountain out
} } of a mole hill. Perhaps we should let this dog lay.
} } If not, Nestor will keep us on track. Notwithstanding,
} } I will do some EBSD studies later this year and report
} } back to the list.
} }
} } gary g.
} }
} }
} } At 07:01 PM 4/19/2004, you wrote:
} } } To All:
} } }
} } } [unsnip]
}
} The question about whether coatings deposited using a sputter coater are
} 'amorphous' or 'crystalline' seems to be in dispute here. On an atomic
} level, if you can make an amorphous metal then we should be able to image it
} in our high resolution TEM (JEOL 4000EX) and not find the orderly
} arrangement of atoms in the layers. For gold deposited on amorphous
} (definitely) silicon, we can see easily at 800kX (5MX final mag) that the
} gold 'islands' of about 5nm diameter are composed of crystalline gold with
} each atom being able to be identified and counted in the orderly structure.
} We do the same thing at interfaces in semiconductor devices to note the
} changes of atomic structure where two metal system combine. It should also
} be noted that if the layer is thin enough, the diffraction pattern is hard
} to find (very weak signal) but with a long enough dwell time you will
} definitely see that the metal layer has atomic level crystalline structure.
}
} The argument that seems to be being presented here is semantic, not
} scientific. Whether or not a layer appears as a 'honeycomb' has nothing to
} do with the fact that the structure of the 'honeycomb' is crystalline or
} amorphous. For the purposes of SEM the ideal is to have an 'amorphous'
} layer from the standpoint that at the magnifications involved there is no
} contribution of 'ordered' structures from the coating. This has absolutely
} nothing to do with whether or not the atomic level structures are
} crystalline or amorphous. We routinely coat samples with whatever material
} is best suited for the images we want to obtain. That might be gold, Au/Pd,
} Cr, Ag, Ti or whatever else seems to work. For Auger work we even use
} deposited Li to eliminate charging without contributing significantly to the
} spectral data. For SEM you are striving to achieve a coating that allows
} imaging of your actual sample without adding 'artifacts' that will confuse
} the interpretation of your data. If that means that you deposit a
} } } gold/palladium or chromium layer with such fine structure that your SEM
} } } image sees only the information from your sample but doesn't present an
} } } artifact then, by all means, call it 'amorphous'. A more distinctive
} } } description might, however, be 'uniform' at the magnification
} used. By this
} } } definition the actual atomic level crystallinity of the layer is not
} called
} } } into question. If you really want to know about the atomic scale ordering
} } } then you need to move on to HRTEM since SEM is not sufficient to see the
} } } atomic scale features. You could also use atomic force microscopy to
} 'see'
} } } the atomic structure of your surface coating.
} } }
} } } Drew Hirt
} } } Materials Research Laboratories, Inc.
} } } Tel (800) 424-1776
} } } Fax (330) 750-0776
} } } drew-at-hirt.com
} } } http://www.mrllab.com
} } }
} } }
} } } on 4/19/04 11:57 AM, Gary Gaugler at gary-at-gaugler.com wrote:
} } }
} } } }
} } } }
} } } }
} } }
} ----------------------------------------------------------------------------
} -} } -
} } } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } } To Subscribe/Unsubscribe --
} } } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } }
} } }
} ----------------------------------------------------------------------------
} } } --} -
} } } }
} } } } Nestor:
} } } }
} } } } Indeed, amorphous likely means different things
} } } } to different folks and in different situations.
} } } } From a metallurgical or atomic standpoint, it
} } } } would mean that it lacks a definitive or distinct
} } } } crystalline structure--i.e., no lattice. On the
} } } } other hand, amorphous could mean that it is shapeless,
} } } } of no definite form or organization or methodical
} } } } arrangement.
} } } }
} } } } OK, does this mean no form or organization at the
} } } } eye ball level? At the magnifying glass level?
} } } } LM, SEM, TEM level? I think that I "see" the
} } } } problem of definition and ability to define it.
} } } }
} } } } The general consensus seems to be one of grains.
} } } } A honey comb shaped coating of Au would have the
} } } } metal portions containing or consisting of grains
} } } } of Au. Thus, the honey comb has organization and
} } } } methodical arrangement--not amorphous. And the
} } } } Au metal would have grains--not amorphous. Therefore,
} } } } sputtered Au is not amorphous.
} } } }
} } } } Now to discuss Au/Pd. This material sputters
} } } } totally differently than Au alone. The coating
} } } } is like a layer of grains of sand. These dots,
} } } } if you will, may touch one another in places and
} } } } not in others. Unlike reflowed metal, the dots
} } } } are distinct and quite 3-D. Is this an amorphous
} } } } layer? If each dot was one grain, and each grain
} } } } was not touching each other grain, is the coating
} } } } amorphous or not? Does continuity play into the
} } } } definition?
} } } }
} } } } At damascene vias, the ILD is definitely amorphous.
} } } } These areas etch totally differently than areas
} } } } away from the vias. It's interesting to see that
} } } } areas away from vias exhibit some degree of
} } } } amorphousness. Why the via areas are more strongly
} } } } amorphous, I do not yet know. This is something
} } } } I am working on at the moment.
} } } }
} } } } If I can find some Au and Au/Pd pix that I can
} } } } post, I will do so. I have the pix somewhere and
} } } } I have specimens (all over the place). If there
} } } } is interest, I will work on getting them.
} } } }
} } } } gary g.
} } } }
} } } }
} } } }
} } } }
} } } }
} } } } At 05:34 AM 4/19/2004, you wrote:
} } } } } Gary
} } } } }
} } } } } If you are truely producing amorphous Au this would
} } } } } be very significant. I must admit to being somewhat
} } } } } skeptical.
} } } } }
} } } } } An image of a near feature less "surface" is not sufficient
} } } } } evidence to call something amorphous.
} } } } }
} } } } } The best way to answer this question would be to prepare
} } } } } a TEM cross-section. Then using either HREM or Electron Diffraction
} from
} } } } } the coating you could verify if the coating is crystalline
} } } } } or not.
} } } } }
} } } } }
} } } } } Nestor
} } } } }
} } } } }
} } } } }
} } } } } }
} -------------------------------------------------------------------------
} } } } } -----
} } } } } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} } } } } } To Subscribe/Unsubscribe --
} } } } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } } } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } } } }
} -------------------------------------------------------------------------
} } } } } ------
} } } } } }
} } } } } } Using an FEI Sirion SFEG, the coating is amorphous.
} } } } } } The "measurement" is looking at the image via the SEM.
} } } } } } Plain Au is honeycombed. Would you like a sample of
} } } } } } this? See what you can see at 350KX. What would you
} } } } } } use to do this yourself? Let's compare images.
} } } } } } If it would be productive, of course.
} } } } } }
} } } } } } How do we define amorphous versus non-amorphous
} } } } } } at this mag? This is further complicated by the
} } } } } } manner in which the coating is deposited. There
} } } } } } are way too many variables. Perhaps I simplify
} } } } } } the topic.
} } } } } }
} } } } } } So, what do you want to see? I can produce pix
} } } } } } at 350KX of Au and Au/Pd coatings. If these are
} } } } } } a big surprise to you, I can provide specimen images.
} } } } } } Alternatively, show me what you have at this same
} } } } } } mag. Produce Au and Au/Pd and Pt images. That pretty well
} } } } } } covers the normal sputter coating environment.
} } } } } }
} } } } } } I am always open to new views on this subject.
} } } } } }
} } } } } } gary g.
} } } } } }
} } } } } }
} } } } } } At 07:12 PM 4/18/2004, you wrote:
} } } } } }
} } } } } } } -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
} } } } } } }
} } } } } } } Gary Gaugler wrote:
} } } } } } } ====================================================================
} } } } } } } .............What I do know is that if I switch to Au/Pd (60/40) or
} } } Pt, the
} } } } } } } coating is amorphous and cannot be easily seen. Au coating can be
} } } seen at
} } } } } } } about 350KX. For Au/Pd or Pt, I can't see a honeycomb at up to 500KX.
} } } } } } } However, Au/Pd and Pt look totally different than Au alone. Au/Pd and
} } } } } Pt is
} } } } } } } more granular rather than honeycomb. And it will look this way at
} } } } } 350KX and
} } } } } } } greater.
} } } } } } } ====================================================================
} } } } } } } Could you tell us the measurement used to conclude it is an amorphous
} } } } } } } coating? So far as I know, one does see a grain, even with Pt or
} Au/Pd
} } } } } } } irrrespective of the brand of sputter coater used.
} } } } } } }
} } } } } } } Chuck
} } } } } } }
} } } } } } } ============================================
} } } } } } } Charles A. Garber, Ph. D. Ph: 1-610-436-5400
} } } } } } } President 1-800-2424-SPI
} } } } } } } SPI SUPPLIES FAX: 1-610-436-5755
} } } } } } } PO BOX 656 e-mail:cgarber-at-2spi.com
} } } } } } } West Chester, PA 19381-0656 USA
} } } } } } } Cust.Service: spi2spi-at-2spi.com
} } } } } } }
} } } } } } } Look for us!
} } } } } } } ########################
} } } } } } } WWW: http://www.2spi.com
} } } } } } } ########################
} } } } } } } ============================================
} } } }
} } } }
} } } }
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 03:17:16 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Frank,
Your new computer should have a minimum of one gigabyte RAM. Imaging
processing applications are memory hungry.
A digital video capture card maintains the integrity of your data. If
you convert digital to analog and back to digital loss of image quality
may occur. ATI Radion makes a good combined video-capture card, some
people prefer a separate capture card. This will also have the fast
connections should you upgrade your camera at some time in the future.
Two hard drives allow you to keep your programs and applications
separate from large image and other data files. This speeds up your
system and decreases maintenance (like defragmenting). It makes backup
easier and your files are on a separate device if your 'C' drive fails.
DVD burners have come down in price (under $200.) and can store over
4gB . Sony just released their 4th generation 8X DVD burners. They
developed the DVD format and have a reputation for reliability. (Be
aware that there are two DVD formats, "+" and "-". Most current brands
and models can use both types of media.)

Bob Carter
2000 Bayshore Road
Lopez Island, WA 98261

-----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
Sent: Monday, April 19, 2004 6:35 AM
To: microscopy-at-msa.microscopy.com

I've been tasked with pulling together sensible specifications for a new
computer to capture digital images from our pol scope. Many options
appear to be straight forward:
More RAM, - 512 MB seems to be enough.
More HD storage, - As Daisy use to say, you can never be too rich,
too thin or have enough storage. I think 120GB is enough.
CD burner at 48X seems enough

but which monitor?
Should I look for a fast response time, say 16ms, to help me focus? Are
flat screens better for viewing than the more traditional monitors? Do I
need more then 17 inch diagonal screen? Is the integrated Intel 3D
Extreme Graphics video card a good choice for photomicrography?

Any suggestions for a good driver to capture my images? I intend to use
photoshop to do any post imaging processing that needed, but I would
like to be able to do a little tweaking to maximize my images when I
capture them.

I have also inhered a Microimaging Video system and a RGB Automatic
Camera, but I have no instructions or user manual. If anyone knows a
web site or has a copy they would like to share I would be grateful!

Any advice, opinions or alternative suggestions are welcome!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 08:31:08 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Does anyone have a fixation procedure to recommend for E. coli? These cells
are being used as a control for some more hazardous strains and must be
chemically fixed in a containment hood prior to being brought to our
facility.

The E. coil cells were fixed using 2.5% glut + 2% PAF in 0.1M Cacodylate
buffer, pH 7.4, (with added 1mM CaCl2, 2mM MgCl2.6H20, 0.25% NaCl)
followed by osmium post-fix, ETOH dehydration and embedding in 812 generic
resin or 812 generic:spurr mixture. This has produced cells with obvious
collapse of the plasma membrane at the poles of the cells. The pulling away
of the plasma membrane from the cell wall gives the initial appearance of
large vacuoles at either end of the cell. Other bacteria strains, such as
listeria, have been well preserved using this protocol.

However, E. coli cells that were fixed in the same primary fix-buffer
combination and then plunge frozen do not show the same artifact. In this
case the cells were freeze-substituted in acetone-osmium and then embedded
in Spurr resin. I was surprised at the difference since both samples were
initially fixed identically. This seems to indicate that the difference
might not be related to osmolarity of the primary fix as I initially
suspected.

I might note that these cells were grown in liquid culture. The above
protocol works fine with cells grown on agar.

Older references suggest using acrolein for primary fixation. I prefer to
not use this chemical due to itąs hazardous nature. Other older references
utilize vernal-acetate buffer which is also no longer desirable due to itąs
classification as a restricted substance requiring special permissions to
purchase.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 09:06:40 2004

Contents Retrieved from Microscopy Listserver Archives
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Frank

I don't know if you made this clearer at an earlier stage, but a major factor in handling and storage will be the resolution and quality of images that you capture from your microscope. There will be great difference between a 1 mega pixel image captured/stored in JPEG format and 5-6 mega pixel image captured/stored in TIF or RAW format - a factor of 50x or more.

If you are after bigger formats then DVD writers must be a better prospect than CD writers especially as they should be able to write to CDs as well. But if you're archiving to these disks you would need to consider that none are considered as archival quality. I think most experts suggest that for 5-10 year storage you should maintain at least one duplicate CD or DVD disks ie if one goes wrong after use then check the unused backup.

I would also point out that there are really 5 DVD formats (DVD+R, DVD-R, DVD+RW, DVD-RW and DVD RAM). Although it is the slowest of the 5 formats, DVD RAM does guarantee 100,000x writes compared with 1,000x for the others so it should be the nearest to archival. I believe this is because of a more meticulous error checking system. At present I think Iomega and LG are the only manufacturers of writers for all of the formats. But the big problem is that because DVD RAM disks are more expensive and slower, they are less popular in the West (a bit more popular in Japan I think). So if you used a system like that you may want RAM for internal use and say DVD+R for customers or other users.

I hope I have got all my facts correct and haven't just muddied the waters.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
University of Sunderland
Tyne & Wear
UK

e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Bob Carter {bob-at-rockisland.com}

Perhaps "the answer" is to use a microscope that allows high-resolution
imaging of your structures without any coating, through proper choice of low
voltage and/or Variable Pressure imaging conditions ( in VP mode,
nitrogen/air ionized by the secondaries generated by the primary beam acts
as both the neutralizing gas and as an "internal scintillator"). Through
both improved low-voltage imaging resolution and VP mode, high-resolution
secondary electron imaging on uncoated "charge challenged" samples is
achievable on the latest generation secondary electron microscopes.

Regards,
Ed

***********************
Edward L. Principe, Ph.D.
Applications Development Scientist
Zeiss SMT, Inc.
(formerly LEO Electron Microscopy)
*****************************
----- Original Message -----
} From: "Gary Gaugler" {gary-at-gaugler.com}
To: "Materials Research Laboratories, Inc." {mrllab-at-raex.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Monday, April 19, 2004 8:59 PM

Hello Microscopists !

First I looked on the MSA website for electron microscopy service labs
in the Cleveland, Ohio metropolitan area - and even with Google. All
to no avail. So now I'm beating the drums on the Microscopy Listserver.

The specimens will be some broken wheel bolts - about the size
you'd have holding your car's wheels on. Mebbe 9/16 inch diameter
and an inch and a half long. Both fractography and metallographically
prepared cross sections. Mebbe microhardness, too. Ability to EDX
or WDS carbon would be a plus. This would be a common-ground
examination as part of a legal case. We're trying to piggyback the
lab work onto the on-site exam; hence the need for a lab in the
Cleveland area. Don't be bashful. I'll submit results to the firm
that's organizing the party through my own counsel/client.

Best regards,
George Langford, Sc.D.
Amenex Associates, Inc.
http://wwww.amenex.com/

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 12:07:39 2004

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debbie

pick your favourite fixation method. the bacterium will be inactivated
by formaldehyde, formaldehyde:glutaraldehyde, or glutaraldehyde. this
has always worked for us, anyway

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 12:08:10 2004

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Hi Debby,
All the bacteria that I have done like a lower pH. (was microscopist for
Microbiology Dept at
Univ. of Illinois and looked at all the bugs that came in the Dept for
various types of research)
That is why veronal acetate buffer was used for so long because it
buffers well at pHs of 6.8 or
so. It however, as you pointed out, is now restricted. We get a
different appearance of the walls
when we do a strictly Os fix and one involving both G and Os especially
obvious in the Gram
Negative bacteria. The traditional "Kellenberger" method puts Os
directly in the liquid growth
media and pellets the bugs down then resuspends them in fresh Os. It
appears you cannot do
that however because of the necessary pre-treatment for safety purposes.
We get fairly good
preservation however using either Os only or both G and Os. We always
do an en bloc UA
stain after the Osmium because of the free nucleic acids which stain
nicely. I assume you are
putting the bugs in agar? Perhaps you might want to send me an image.
Have you peeked at the
bugs in SEM to see what their surface looks like with a simple G, Os,
dehydration, and CPD or
freeze drying run? That would also give you an idea of how crenulated
the surface might be
expected to be.
Don't know if any of the above helped, but just thought I would toss in
my two cents.

Good Luck,
Judy

Debby Sherman wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
} Does anyone have a fixation procedure to recommend for E. coli? These cells
} are being used as a control for some more hazardous strains and must be
} chemically fixed in a containment hood prior to being brought to our
} facility.
}
} The E. coil cells were fixed using 2.5% glut + 2% PAF in 0.1M Cacodylate
} buffer, pH 7.4, (with added 1mM CaCl2, 2mM MgCl2.6H20, 0.25% NaCl)
} followed by osmium post-fix, ETOH dehydration and embedding in 812 generic
} resin or 812 generic:spurr mixture. This has produced cells with obvious
} collapse of the plasma membrane at the poles of the cells. The pulling away
} of the plasma membrane from the cell wall gives the initial appearance of
} large vacuoles at either end of the cell. Other bacteria strains, such as
} listeria, have been well preserved using this protocol.
}
} However, E. coli cells that were fixed in the same primary fix-buffer
} combination and then plunge frozen do not show the same artifact. In this
} case the cells were freeze-substituted in acetone-osmium and then embedded
} in Spurr resin. I was surprised at the difference since both samples were
} initially fixed identically. This seems to indicate that the difference
} might not be related to osmolarity of the primary fix as I initially
} suspected.
}
} I might note that these cells were grown in liquid culture. The above
} protocol works fine with cells grown on agar.
}
} Older references suggest using acrolein for primary fixation. I prefer to
} not use this chemical due to it1s hazardous nature. Other older references
} utilize vernal-acetate buffer which is also no longer desirable due to it1s
} classification as a restricted substance requiring special permissions to
} purchase.
}
} Debby
}
} Debby Sherman, Manager Phone: 765-494-6666
} Life Science Microscopy Facility FAX: 765-494-5896
} Purdue University E-mail: dsherman-at-purdue.edu
} S-052 Whistler Building
} 170 S. University Street
} West Lafayette, IN 47907
} http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 13:13:57 2004

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George ,
Try Smithers in Akron (330-762-7441
ARDL also in Akron at 330-794-660
Noveon between Akron and Cleveland at 216-447-5000.

Good luck

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

"George
Langford, To: Microscopy-at-MSA.Microscopy.com
Sc.D." cc: "George Langford, Sc.D." {amenex-at-amenex.com}
{amenex-at-amene Subject: [Microscopy] Commercial SEM labs in the
x.com} Cleveland, OH area ?

04/20/2004
11:48 AM
Please
respond to
"George
Langford,
Sc.D."

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Hello Microscopists !

First I looked on the MSA website for electron microscopy service labs
in the Cleveland, Ohio metropolitan area - and even with Google. All
to no avail. So now I'm beating the drums on the Microscopy Listserver.

The specimens will be some broken wheel bolts - about the size
you'd have holding your car's wheels on. Mebbe 9/16 inch diameter
and an inch and a half long. Both fractography and metallographically
prepared cross sections. Mebbe microhardness, too. Ability to EDX
or WDS carbon would be a plus. This would be a common-ground
examination as part of a legal case. We're trying to piggyback the
lab work onto the on-site exam; hence the need for a lab in the
Cleveland area. Don't be bashful. I'll submit results to the firm
that's organizing the party through my own counsel/client.

Best regards,
George Langford, Sc.D.
Amenex Associates, Inc.
http://wwww.amenex.com/

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 13:33:38 2004

Contents Retrieved from Microscopy Listserver Archives
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Although we have always kept OsO4 wrapped up to protect it from light
because someone somewhere said that it was light sensitive, now I'm
wondering if that is indeed true or not. I personally cannot really
remember if it is, or if this is just a superstition. How do you people
store your OsO4, and is it really light sensitive or not?

Garry

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 14:04:23 2004

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Last week I posted an inquiry regarding an instruction manual for an older
model Olympus microscope, and noted that Olympus America had not responded
to my e-mails from their web site. Thanks to those who responded, and I
must add that Olympus America responded immediately to my posting on this
microscopy site. In fact, Olympus provided three
e-mail responses, phone calls, a manual, some needed technical information
and additional support links. They were terrific. Good job.

John J. Wolosewick, Ph.D.
Department of Anatomy and Cell Biology M/C 512
University of Illinois at Chicago
808 S. Wood Street
Chicago, Illinois 60612

jjwolo-at-uic.edu 312-996-6022

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 16:35:04 2004

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Materials Research Laboratories, Inc.
290 North Bridge Street
Struthers, OH 44471
800 424-1776
http://www.mrllab.com/

}
} George ,
} Try Smithers in Akron (330-762-7441
} ARDL also in Akron at 330-794-660
} Noveon between Akron and Cleveland at 216-447-5000.
}
} Good luck
}
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}
}
}
} "George
} Langford, To: Microscopy-at-MSA.Microscopy.com
} Sc.D." cc: "George Langford, Sc.D." {amenex-at-amenex.com}
} {amenex-at-amene Subject: [Microscopy] Commercial SEM labs in the
} x.com} Cleveland, OH area ?
}
} 04/20/2004
} 11:48 AM
} Please
} respond to
} "George
} Langford,
} Sc.D."
}
}
}
}
}
}
}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
}
} Hello Microscopists !
}
} First I looked on the MSA website for electron microscopy service labs
} in the Cleveland, Ohio metropolitan area - and even with Google. All
} to no avail. So now I'm beating the drums on the Microscopy Listserver.
}
} The specimens will be some broken wheel bolts - about the size
} you'd have holding your car's wheels on. Mebbe 9/16 inch diameter
} and an inch and a half long. Both fractography and metallographically
} prepared cross sections. Mebbe microhardness, too. Ability to EDX
} or WDS carbon would be a plus. This would be a common-ground
} examination as part of a legal case. We're trying to piggyback the
} lab work onto the on-site exam; hence the need for a lab in the
} Cleveland area. Don't be bashful. I'll submit results to the firm
} that's organizing the party through my own counsel/client.
}
} Best regards,
} George Langford, Sc.D.
} Amenex Associates, Inc.
} http://wwww.amenex.com/
}
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 16:58:31 2004

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Quoting Garry Burgess {GBurgess-at-exchange.hsc.mb.ca} :
} Although we have always kept OsO4 wrapped up to protect it from light
} because someone somewhere said that it was light sensitive, now I'm
} wondering if that is indeed true or not. I personally cannot really
} remember if it is, or if this is just a superstition. How do you people
} store your OsO4, and is it really light sensitive or not?
}
} Garry
+++++++++++++
Garry,
I store the OsO4 in the refrigerator and I KNOW that the light is off because
there is no light bulb in there!

Pat Connelly
Dept. of Biology
Univ. of Pennsylvania

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 16:58:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Quoting Garry Burgess {GBurgess-at-exchange.hsc.mb.ca} :
} Although we have always kept OsO4 wrapped up to protect it from light
} because someone somewhere said that it was light sensitive, now I'm
} wondering if that is indeed true or not. I personally cannot really
} remember if it is, or if this is just a superstition. How do you people
} store your OsO4, and is it really light sensitive or not?
}
} Garry
+++++++++++++
Garry,
I store the OsO4 in the refrigerator and I KNOW that the light is off because
there is no light bulb in there!

Pat Connelly
Dept. of Biology
Univ. of Pennsylvania

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 20:47:01 2004

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Debby
I did not have problems with E.coli fixation using 1.5% GA in PBS 1-2h on
ice. Your fixation looks over killing to me (for how long, overnight I
guess?). I don't see any reason to use formaldehyde for EM if antigenity is
not a critical issue. Usually people use formaldehyde for immuno-EM in
combination with low GA concentration (so formaldehyde partially
substitute GA) . Over fixation by itself may cause the shrinkage and other
artefacts. Sergey.

At 06:52 AM 4/20/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 23:20:26 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (pamarone-at-bdsinternational.com) from on Tuesday, April 20, 2004 at 06:39:53
---------------------------------------------------------------------------

Email: pamarone-at-bdsinternational.com
Name: Pam Marone

Organization: Pharmaceutical

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have any information or references regarding staining/labelling for SEM? I would like to follow a liposome-based structure through the digestive tract, through its metabolism and would like to have a technique for labelling such a structure. Thank you

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From MicroscopyL-request-at-ns.microscopy.com Tue Apr 20 23:21:03 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (curtlane2003-at-yahoo.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, April 20, 2004 at 22:41:46
---------------------------------------------------------------------------

Email: curtlane2003-at-yahoo.com
Name: curt lane

Organization: lane assoc.

Title-Subject: [Microscopy] [Filtered] MListserver:sem service labs

Question: I am trying to get a list of sem service labs currently operating in northern california. thank you

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 06:05:27 2004

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George ,

We do outside SEM work and we are located in Euclid. You can visit our
website at www.atclabs.com for more information. We have 2 SEM digitally
equipped with PGT systems which helps us to produce more presentable photos
EDS and WDS analysis. We also have a full metallography, chemistry,
mechanical, and X-ray labs.
For more information please contact Joe Radisek at 216-692-5456 e-mail:
Radisek-at-argo-tech.com or myself.

Regards,

Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

                    "George

                    Langford,            To:
Microscopy-at-MSA.Microscopy.com
                    Sc.D."               cc:     "George Langford, Sc.D."
{amenex-at-amenex.com}
                    {amenex-at-amene        Subject: [Microscopy]
Commercial SEM labs in the
                    x.com}                Cleveland, OH area
?



04/20/2004
                    11:48
AM
                    Please

                    respond
to

"George
                    Langford,


Sc.D."






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From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 09:11:39 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (le_thiec-at-nancy.inra.fr) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 21, 2004 at 08:28:31
---------------------------------------------------------------------------

Email: le_thiec-at-nancy.inra.fr
Name: Le Thiec

Organization: INRA

Title-Subject: [Microscopy] [Filtered] MListserver: WDS and cryo

Question: Dear all

I would like to analyse the element composition of biological samples also I am looking for a scanning electron microscope (field emission will be better) with cryo system and WDS system. it will be possible for me to go everywhere in the world. If you know a laboratory which has a SEM with WDS and cryo, please contact me. Thank you in advances.
Didier

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From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 09:11:12 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (fremingt-at-fhcrc.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 21, 2004 at 08:43:33
---------------------------------------------------------------------------

Email: fremingt-at-fhcrc.org
Name: Franque Remington

Organization: Fred Hutchinson Cancer Research Center

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have sucessful results fixing and processing samples of conidia of aspergillus for sem? We have tried many methods, but instead of being round, they have places where the walls seem to have indented. We have tried 2% gluteraldehyde fixation, with and without post-fixing in osmium. We have dehydrated in both alcohols and acetone and used HMDS and nothing changes the result.

Any help would be appreciated.

F. Remington
fremingt-at-fhcrc.org
Fred Hutchinson Cancer Research Center

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From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 09:57:24 2004

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Hi there,

Due to the dissolution of a lab, 13 steel histology knives are
available for free to any educational and/or non-profit
organization/lab/personnel. They are not available to any commercial
outlet.

Description
- 12 specimens, 12 cm blades, most likely stainless steel, date from
approximately 1940-1960, Each in box. Look decent, most likely will
require some sharpening, though they are sharp to the finger.

- 1 ca 18 cm blade, otherwise like above.

Knives are provided on a first come - first served basis. There is no
limit on number of knives per address. If you have questions, please
send me a direct (i.e., non-listserver) e-mail. Thanks for your
interest.

Daniel Geiger
--
***************************************************************************************

Daniel L. Geiger, Ph.D.
Research Associate Santa Barbara Museum of Natural History
Adjunct Assistant Professsor, University of Southern California, Los Angeles

Mailing Address:
Molecular Systematics Lab, Natural History Museum of Los Angeles County
900 Exposition Blvd., Los Angeles, CA 90007, USA
phone: (213) 763 3431 fax: (213) 748 4432
NEW e-mail geiger-at-vetigastropoda.com
NEW www http://www.vetigastropoda.com

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 11:30:57 2004

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Try vapor fixing in osmium vapor. Put you material in a small container (I
use a glass Petri dish sealed with double parafilm) with a few drops of 4%
osmium tetroxide. Leave it for about 72 hours at RT in a hood, then air
dry. Aspergillus conidia tend to dimple a bit naturally, but this will
stabilize them as well as,any method, and better than most.
Robert

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 12:07:47 2004

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Hi,

After many years of living with osmicated 'fridges, I tried an experiment by keeping the osmium tetroxide at the back of the chemical hood at room temperature.

We only keep about 50ml at a time and the chemical hood is always on, so there didn't seem to be any vapour hazard (unlike the smelly 'fridge).

After 5 years of doing this, I can say that there seems to be no harm in keeping 2% osmium tetroxide at room temperature and in full light every day. Now keep the osmium tetroxide in full light and at room temperature and we have the added bonus of a clean fridge.

Hope this is useful.

PS. Thanks Nestor.

Regards,

Paul Webster.

Paul Webster, Ph.D.
House Ear Institute
2100 West Third Street
Los Angeles
CA 90057
phone (213) 273 8026
fax (213) 413 6739
email: pwebster-at-hei.org

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 12:35:05 2004

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Hi Gary,

This is a quote from Advanced Inorganic Chemistry, 2nd Ed. by Cotton
and Wilkinson on page 1005 under tetroxides. This is a well known book.
"Above ~180°, RuO4 can explode, giving RuO2 and O2, and it is decomposed
slowly by light; OsO4 is more stable in both respects."
The later statement suggests or implies that OsO4 can also be
decomposed by light because it does NOT say, "; OsO4 is very stable and
does not decompose or explode."

So I always wrapped OsO4 in Al foil as a minimum and kept all of it in
a glass container tray is case of a broken ampoule. OsO4 ampoules are not
something you want out in the open on a bench anyway.
For potential RuO4 spills, use a crystallizing dish lined and padded
on the bottom with paper towels.
Unsaturated corn oil is recommended for OsO4 but it's a mess to clean
up. Yuk!

The article in the Sept-Oct 2002 issue of Microscopy Today on page 20
would indicate that the reaction rates are indeed quite different. I sent
you an email reprint of the discussion of some of the chemistry of Os and
Ru and their reaction indicators in this article.

Paul Beauregard
Senior Research Associate
Microscopy and Image Analysis

At 01:54 PM 04/20/04 -0500, Garry Burgess wrote:
}
}
} ---------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 15:04:29 2004

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Hi:

I would like to remind researchers that osmium made up in distilled water is
very stable at room temperature. However, if some of you make up a 1% in
buffer and store as such then definitely refrigerate your solution because
reduces at a faster rate. We have noticed this in our laboratory and now
only make up 2% aqueous and dilute with an equal amount of buffer when we
need it. We store it in the hood in a glass stoppered 100 ml wide mouth
bottle which is enclosed in a small bell jar.

Karen Bentley

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

-----Original Message-----
} From: Webster, Paul [mailto:PWebster-at-hei.org]
Sent: Wednesday, April 21, 2004 1:29 PM
To: MSA listserver submission (E-mail)
Cc: Nestor-at-Zaluzec.Com; Zaluzec-at-aaem.amc.anl.gov

Hi,

After many years of living with osmicated 'fridges, I tried an experiment by
keeping the osmium tetroxide at the back of the chemical hood at room
temperature.

We only keep about 50ml at a time and the chemical hood is always on, so
there didn't seem to be any vapour hazard (unlike the smelly 'fridge).

After 5 years of doing this, I can say that there seems to be no harm in
keeping 2% osmium tetroxide at room temperature and in full light every day.
Now keep the osmium tetroxide in full light and at room temperature and we
have the added bonus of a clean fridge.

Hope this is useful.

PS. Thanks Nestor.

Regards,

Paul Webster.

Paul Webster, Ph.D.
House Ear Institute
2100 West Third Street
Los Angeles
CA 90057
phone (213) 273 8026
fax (213) 413 6739
email: pwebster-at-hei.org

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 18:12:25 2004

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William;
If you see this problem with the beam off, it is certainly NOT
your phosphor causing the problem. This noise is typical of a CCD
readout when the CCD is a frame read-out, not an interline readout and
when thermal noise is excessive due to a failure of the cooling system.

John Mardinly
Intel

-----Original Message-----
} From: William Stratton [mailto:wgstratton-at-wisc.edu]
Sent: Monday, April 19, 2004 7:11 AM
To: Microscopy

Hello all,

Thank you for all of your tips. I got some great responses with some
really
good ideas to solve this problem.

To clear up some questions: All images that I see this problem with are
acquired when the beam is off (no intensity on the CCD), the images are
also
raw (not dark count or gain corrected). The problem is not with an
artifact
present in all CCD images, but rather the horizontal line profile of the
image (a measure of the average pixel value across the image
horizontally)
increases from left to right.

What the solution may be: From responses I've received it may be that
the
scintallator may have corroded from prolonged exposure to
condensation/contamination within the TEM column. We're going to try
and
clean it off to rid ourselves of the problem.

Thanks again!

William Stratton

-------------------
William G. Stratton
Research Assistant
University of Wisconsin - Madison

1509 University Avenue
Madison, WI 53706
Office: 608-265-6391
Fax: 608-262-8353
wgstratton-at-wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 19:36:20 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (jlflow2-at-uky.edu) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Wednesday,
April 21, 2004 at 16:07:08
---------------------------------------------------------------------------

Email: jlflow2-at-uky.edu
Name: Jen Flowers

Organization: University of Kentucky, Dept. of Plant Pathology

Education: Graduate College

Location: Lexington, KY, USA

Question: Hi, I am looking for a contact that is familiar with
viewing conifer tissue using confocal microscopy. I plan on looking
at a fungal pathogen growing through pine tissue for part of my
dissertation research. Any help would be greatly appreciated

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From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 19:47:38 2004

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Hello,
Anyone have a Med 020 sputter coater/evaporator I could get some training
on? We bought a used unit and the manual doesn't have a very good section
on how to procedureally use it.
Thanks, any advice appreciated.

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 21 23:21:36 2004

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Hi All,

Just a quick email to say thank you to all who answered my earlier posting
and who gave of their time and knowledge. After much fiddling with my
obselete PC I finally got some software working and managed to export my
images.

Regards
George

George Theodossiou
Physicist / Electron Microscopist

AMCOR Research and Technology
Ph: +61 3 9490 6135
Fax: +61 3 9499 4295
Mobile: 0409 568 840
email: George.Theodossiou-at-amcor.com.au

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this message is prohibited. If you have received this message in error
please notify AMCOR immediately.
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From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 00:00:32 2004

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Hi:
I would need a gun for a Zeiss 109 TEM. If you have one or now of anyone who
has please let me know.
Thank you,
Peter Jordan/EMSI

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 10:13:53 2004

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Hi Jen
We had a project which looked at a fungus infecting pine.

The fungus was transfected with GFP. The pine autofluoresced in the
red and the green. We ballanced up the autofluorescence and then with
the software on the Bio-Rad Radiance subtracted the red from the
green just leaving the fungus GFP in the green which we could then
overlay with the red autofluorescence. This was published as "The use
of the green fluorescent protein as a biomarker for sapstain fungi"
by S.Lee, S.H. Kim and C. Breuil For. Path. 32 (2002) 153-161

The Bio-Rad Radiance worked very well on this project but if you
have access to a spectral imaging system, you can also eliminate the
autofluorescence using software.

Elaine

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--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 12:57:20 2004

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Folks -

I am looking to acquire (beg, borrow, purchase)
a Philips (now FEI) multiple sample holder
PW6598 for a CM12-TEM. It allows for three
TEM grids to inserted at the same time.

Any suggestions would be appreciated.

thanks and regards,

Jim

*********************************************************
Dr. Jim Quinn james.quinn-at-sunysb.edu
Materials Science 631-632-6663 FAX:8052
SUNY at Stony Brook http://www.matscieng.sunysb.edu/
Stony Brook, New York 11794 - 2275
*********************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 14:18:28 2004

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I have never fixed human tissue overnight in Osmium Tetroxide, or even left
it in lower concentration alcohols, for fear of ultrastructural details
being leached away during the night, but lately I'm left wondering if
perhaps one could get away with fixing animal [human] tissue in 1% Osmium
Tetroxide overnight in the fridge. Prior to this, we've always fixed in
Osmium for half an hour to an hour.

Does anyone have any experience with overnight fixation of animal tissue in
1% Osmium Tetroxide in water overnight? It would be a great time saver to
me if I knew for certain that this wouldn't adversely affect the
ultrastructure of the tissue.

Garry

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 14:38:54 2004

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Try checking the booklet Identification of Common Aspergillus Species by Dr. Maren A. Klich , mycologist from our facility, published by Centraalbureau voor Schimmelcultures, Utrecht (2002). Different species were imaged in a XL 30 ESEM using either 3% glutaraldehyde in 0.05m cacodylate buffer, ethanol dehydration, and CPD or 2% Osmium vapor fixation and either air-drying or freeze-drying. Most images of conidia and ascospores were adequate, but we had less success with preserving structure on the conidial heads. Now that we have the Peltier cold stage accessory, I intend to image different Aspergillus species uncoated in wet mode under various vacuum conditions. As "they" say "one size does not fit all"!

Bruce F. Ingber, Biologist
Electron Microscopy
USDA-ARS, SRRC
1100 Robert E. Lee Blvd.
New Orleans, LA 70124
bingber-at-srrc.ars.usda.gov
504-286-4270 phone
504-286-4419 fax

} } } "Robert Simmons" {rsimmons-at-gsu.edu} 04/21/04 11:52AM } } }
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Try vapor fixing in osmium vapor. Put you material in a small container (I
use a glass Petri dish sealed with double parafilm) with a few drops of 4%
osmium tetroxide. Leave it for about 72 hours at RT in a hood, then air
dry. Aspergillus conidia tend to dimple a bit naturally, but this will
stabilize them as well as,any method, and better than most.
Robert

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (fremingt-at-fhcrc.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 21, 2004 at 08:43:33
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Email: fremingt-at-fhcrc.org
Name: Franque Remington

Organization: Fred Hutchinson Cancer Research Center

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have sucessful results fixing and processing samples of conidia of aspergillus for sem? We have tried many methods, but instead of being round, they have places where the walls seem to have indented. We have tried 2% gluteraldehyde fixation, with and without post-fixing in osmium. We have dehydrated in both alcohols and acetone and used HMDS and nothing changes the result.

Any help would be appreciated.

F. Remington
fremingt-at-fhcrc.org
Fred Hutchinson Cancer Research Center

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 14:48:30 2004

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Hi all,

I'm trying the Nikon software ACT-1 that manages the Nikon DXM1200 digital
camera. The software has room for only 8 custom scales. I want to set
predefined scales for all stops in my stereo zoom, and all objectives in my
compound microscope, which makes much more than 8.

Have you figured out a workaround for this? I will appreciate any help!

Cheers, Martin

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370
fax +54 11 4982-4494

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 15:59:05 2004

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Hi Garry,
We routinely leave our tissues in 75% alcohol overnight in the
refrigerator. It doesn't shrink or
swell the tissue. Perhaps if one is interested in lipids it might be an
issue but we have compared
it with tissues that are done straight through, and don't see a
difference in animal or plant tissue.
When we leave it in osmium overnight however we get maceration of the
tissue. We actually use
that fact to clean the cytoplasmic stuff out of cells for cryofracturing
for SEM.
Now that we do microwaving however we can do the entire process in one
short morning.
Good Luck,
Judy

Judy Murphy
Microscopy Technology Center
San Joaquin Delta College
5151 Pacific Ave
Stockton, CA 95201
209-954-5284
209-954-5600
jmurphy-at-deltacollege.edu

Garry Burgess wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I have never fixed human tissue overnight in Osmium Tetroxide, or even left
} it in lower concentration alcohols, for fear of ultrastructural details
} being leached away during the night, but lately I'm left wondering if
} perhaps one could get away with fixing animal [human] tissue in 1% Osmium
} Tetroxide overnight in the fridge. Prior to this, we've always fixed in
} Osmium for half an hour to an hour.
}
} Does anyone have any experience with overnight fixation of animal tissue in
} 1% Osmium Tetroxide in water overnight? It would be a great time saver to
} me if I knew for certain that this wouldn't adversely affect the
} ultrastructure of the tissue.
}
} Garry
}
} This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 22 17:58:58 2004

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Our lab always fixed in 2.5% Glutaraldehyde overnite.
We have fixed fat specimens in OsO4. What type(s) of
specimens does your lab work with?
Sara
Garry Burgess {GBurgess-at-exchange.hsc.mb.ca} wrote:

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Society of America

I have never fixed human tissue overnight in Osmium
Tetroxide, or even left
it in lower concentration alcohols, for fear of
ultrastructural details
being leached away during the night, but lately I'm
left wondering if
perhaps one could get away with fixing animal [human]
tissue in 1% Osmium
Tetroxide overnight in the fridge. Prior to this,
we've always fixed in
Osmium for half an hour to an hour.

Does anyone have any experience with overnight
fixation of animal tissue in
1% Osmium Tetroxide in water overnight? It would be a
great time saver to
me if I knew for certain that this wouldn't adversely
affect the
ultrastructure of the tissue.

Garry

This e-mail and/or any documents in this transmission
is intended for the address(s) only and may contain
legally privileged or confidential information. Any
unauthorized use, disclosure, distribution, copying or
dissemination is strictly prohibited. If you receive
this transmission in error, please notify the sender
immediately and return the original.

__________________________________
Do you Yahoo!?
Yahoo! Photos: High-quality 4x6 digital prints for 25˘
http://photos.yahoo.com/ph/print_splash

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 02:16:05 2004

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Hi all,
I am looking for single crystal Quartz and Sapphire substrate, having a
very high optical purity.
I need those for single molecule / nanoparticle fluorescence microscopy
experiments at low temperature.
Does any-body know of a company (or companies) that makes them in
various dimensions and thickness and
with a proven optical purity.
(I tried to get some info from Marketech International Inc., but they've
ignored my email messages thus far)
I would appreciate any help.
Thanks,
Eli

--
***************************************
Eli Rothenberg
Institute of Chemistry, the Farkas Center for Light Induced Processes
and the Center for Nanoscience and Nanotechnology
The Hebrew University of Jerusalem
Jerusalem 91904, Israel
TEL.:972-2-6586814
FAX: 972-2-5618033
http://chem.ch.huji.ac.il/~nano/
****************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 03:34:36 2004

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Hi,

I've been playing around with Max Sidorow's CTFexplorer and I'm finding
it hard to see the
advantage of FEG microscopes for structural biology.

At 61000-times magnification I can't see any major difference between
the Tecnai 20T and
the Tecnai F20T for example.

Only at magnifications beyond 300000 is the F20T clearly superior (due
to better spatial
coherence).

Am I (or is CTFexplorer) missing something relevant?

The CTFexplorer can be found at http://clik.to/ctfexplorer.

Upon request I can also send a Word file with the CTF-plots.

Philip

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 06:56:34 2004

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Eli, have you tried Goodfellow at www.goodfellow.com?
They might be able to help you.

Ed Komarnicki
MacDermid Inc.

eli rothenberg {elir-at-chem.ch.huji.ac.il}
04/23/04 03:37 AM

To
microscopy {Microscopy-at-MSA.Microscopy.Com}
cc

Subject
Quartz and Sapphire substrates.

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Hi all,
I am looking for single crystal Quartz and Sapphire substrate, having a
very high optical purity.
I need those for single molecule / nanoparticle fluorescence microscopy
experiments at low temperature.
Does any-body know of a company (or companies) that makes them in
various dimensions and thickness and
with a proven optical purity.
(I tried to get some info from Marketech International Inc., but they've
ignored my email messages thus far)
I would appreciate any help.
Thanks,
Eli

--
***************************************
Eli Rothenberg
Institute of Chemistry, the Farkas Center for Light Induced Processes
and the Center for Nanoscience and Nanotechnology
The Hebrew University of Jerusalem
Jerusalem 91904, Israel
TEL.:972-2-6586814
FAX: 972-2-5618033
http://chem.ch.huji.ac.il/~nano/
****************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 08:57:44 2004

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Hi,

(a plain-text reply without plots for the benefit of the microscopy
list-server)

} From your plots it seems that you need a FEG to reach resolutions beyond
about 3 A,
But I can’t see any great advantage up to about 5 A resolution.
Is that correct? (and what is all the excitement about then?)

Philip

-----Original Message-----
} From: Lucken, Uwe [mailto:uwl-at-nl.feico.com]
Sent: 23 April 2004 15:03
To: Philip Koeck; 3dem-at-ucsd.edu; microscopy-at-sparc5.microscopy.com
Cc: Max.Sidorov-at-Amd.Com

It might be safer to leave the tissue in buffer overnight after the initial
aldehyde fixation, rather than in OsO4. As you say, the OsO4 step would only
add 30-60 minutes in the morning.

Lesley Weston.

on 22/04/2004 12:39 PM, Garry Burgess at GBurgess-at-exchange.hsc.mb.ca wrote:

}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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--} -
}
}
} I have never fixed human tissue overnight in Osmium Tetroxide, or even left
} it in lower concentration alcohols, for fear of ultrastructural details
} being leached away during the night, but lately I'm left wondering if
} perhaps one could get away with fixing animal [human] tissue in 1% Osmium
} Tetroxide overnight in the fridge. Prior to this, we've always fixed in
} Osmium for half an hour to an hour.
}
} Does anyone have any experience with overnight fixation of animal tissue in
} 1% Osmium Tetroxide in water overnight? It would be a great time saver to
} me if I knew for certain that this wouldn't adversely affect the
} ultrastructure of the tissue.
}
} Garry
}
} This e-mail and/or any documents in this transmission is intended for the
} address(s) only and may contain legally privileged or confidential
} information. Any unauthorized use, disclosure, distribution, copying or
} dissemination is strictly prohibited. If you receive this transmission in
} error, please notify the sender immediately and return the original.
}

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 10:24:44 2004

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"Microanalysis - A New Tool in Combating Terrorism" by Dennis Ward of
the Federal Bureau of Investigation will be the keynote presentation at
the Spring meeting of the Central States Microscopy and Microanalysis
Society on Friday, May 7 at the University of Missouri, Columbia. Other
presentations include "Scanning Probe Microscopy Under Controlled
Environments" by Dr. Shije Wu of Molecular Imaging Corporation,
"Explosives and Explosives Residue Identification" by William Randle of
the Missouri State Highway Patrol Crime Laboratory, and additional talks
on microscopy applications in the biological and materials sciences.
There will also be a poster display area and vendors' exhibits.

This event is hosted by the UMC Electron Microscopy Core Facility and
will begin at 8 a.m. on May 7th, 2004 in the Adams Conference Center of
the College of Veterinary Medicine. Morning and afternoon snack breaks
are included and registration is FREE! A catered lunch will be
available for $10.00 per person (reservations required), and we ask that
those wanting lunch please let us know ASAP (!!!) so we can get a firm
number to give to the caterer.

For more information, directions, and registration forms please contact
me at the address below.

Hope to see you there!

Randy Tindall, President
Central States Microscopy and Microanalysis Society
Web: http://treefrog.cvm.uiuc.edu/~lam/csmms/

Electron Microscopy Core
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 10:54:49 2004

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Philip;

I would also add that for x-ray or EELS microanalysis, which
some biologists - albeit a few(!) carry out and actually call
"structural biology, FEGs can be important since one obtains a far
higher electron flux per unit area than with LaB6 thus improving
precision of measuements. In some cases of detection and mapping of
rather low subcellular contents in small regions (in membranes for
example) it can be crucial.

Peter

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--
Peter Ingram
Sr. Physicist
Adj. Professor of Pathology,
Duke University Medical Center
Box 90319
LaSalle Street Extension
DURHAM NC USA 27708-0319

Tel: (919) 660-2695
Fax: (919) 660-2671
e-mail: p.ingram-at-cellbio.duke.edu
http://152.3.54.107/AEM_LAB.html

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 12:57:01 2004

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----- Original Message -----
} From: pamarone-at-bdsinternational.com (by way of
MicroscopyListserver)

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (david.mahoney-at-baesystems.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, April 23, 2004 at 11:28:27
---------------------------------------------------------------------------

Email: david.mahoney-at-baesystems.com
Name: Dave Mahoney

Organization: BAE SYSTEMS

Title-Subject: [Microscopy] [Filtered] New SEM

Question: Iím not sure members can comment on equipment but Iím currently in the market for a new SEM I have narrowed he choices down to JEOL model JSM-6460LV or a Hitachi S-3600N. If anyone has any comments, good or bad, on reliability, performance, image quality, and service issues all comments would be greatly appreciated.
Thank you
BAE SYSTEMS
Dave Mahoney
250 Knotter Drive
Cheshire, CT 06489

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From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 17:02:12 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (skoval-at-uwo.ca) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, April 23, 2004 at 15:54:21
---------------------------------------------------------------------------

Email: skoval-at-uwo.ca
Name: Susan Koval

Organization: University of Western Ontario

Title-Subject: [Microscopy] [Filtered] MListserver: Philips EM300 parts

Question: I am looking for replacement lens for an old, but still needed,
Philips EM300. Specifically, I need the intermediate and
projector lens coils and housings. If anyone has an EM300
they are using for replacement parts, and can provide the
above items, please contact me.

skoval-at-uwo.ca

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From MicroscopyL-request-at-ns.microscopy.com Fri Apr 23 17:42:52 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rinaldop-at-uol.com.br) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, April 23, 2004 at 17:34:05
---------------------------------------------------------------------------

Email: rinaldop-at-uol.com.br
Name: Rinaldo Pires dos Santos

Organization: UFRGS - Porto Alegre - RS - Brazil

Title-Subject: [Microscopy] [Filtered] Problems when dehydrate plant tissues

Question: I am working with the ultrastructure of the gametophyte and sporophyte of Frullania brasiliensis (a folious hepatophyte). After the aldehyde and osmium fixation, when I dehydrate with alcohol or acetone (10, 30, 50, 70, 90, 100; 15-30 minutes each), the samples shrink. Some sugestion?
Thank you.
Rinaldo P. Santos

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From MicroscopyL-request-at-ns.microscopy.com Sat Apr 24 18:50:40 2004

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Hello all,

First the good news:

In addition to state of the art "scopes" from API, AutoQuant,
Bio-Rad, III, Nikon, Perkinelmer, and Zeiss students at the 2004 UBC
Live-cell course can expect to use several really new 3D microscope
systems:

1. Olympus will bring their new Fluoview 1000 and also a new disk scanner
(www.olympusamerica.com/seg_section/seg_product.asp?p=5&sc=1&product=962)

2. Visitech are planning to bring their new Vt"eye" AOD video-rate
confocal system (www.vt-eye.info/) as well as a Yokogawa-based system.

3. Jenalab will bring their DERMALINSPECT 2-photon in-situ optical
biopsy system
(www.jenlab.de/english/products/Derma_Inspect/derma_inspect.html).

and

4. LaVisionBiotech will be bring their TrimScope, high-speed
multifocal, multiphoton microscope.
(www.lavisionbiotec.de/start_product.html)

Now, some more good news:

Several of the students who were originally accepted to attend the
UBC Live-Cell Course have now found that they will not be able to
attend after all.

This means that we now have room for about 3 more students.

If you are interested, please go to: (www.3dcourse.ubc.ca) and look
around. The application form can be found at
(www.3dcourse.ubc.ca/application.htm)

Cheers,

Jim Pawley
--
**********************************************
Prof. James B. Pawley, Ph. 608-263-3147
Room 223, Zoology Research Building,
FAX 608-265-5315
1117 Johnson Ave., Madison, WI, 53706
JBPAWLEY-at-WISC.EDU
3D Microscopy of Living Cells Course, June 12-24, 2004, UBC, Vancouver Canada
Info: www.3dcourse.ubc.ca/ Applications due by March 15, 2004

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 06:47:51 2004

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Hi all,

could anyone please suggest and explain reasonable values for the minimum number of points to be grouped as a grain as well as for the minimum misorientation between two points in EBSD/OIM.

Regards.

Andreas Meyer.

&-] ############################### &-]

Moritz Andreas Meyer
Dipl.-Ing (FH) MSc.
Sr. Materials Analyst SEM
Materials Analysis Department

AMD Saxony LLC & Co. KG
Wilschdorfer Landstraße 101
D-01099 Dresden

Tel. +49 351 277 4149
Fax. +49 351 277 9 4149
E-Mail. moritz-andreas.meyer-at-amd.com

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 08:04:19 2004

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Hi Morgan and all,

We have contacted Nikon, and have an answer for the scales question: Sorry,
only eight.

I solved the problem writing a simple Visual Basic script for IMatch to
place scales on digital images. The script process a batch of images,
reading the scale codes between [] form the file name (it could take that
information from somewhere else).

Regards, Martin

At 02:28 AM 4/23/2004, you wrote:
} Hi Martin
}
} I don't have the answer to your problem but I also use the DXM1200 and ACT
} software. If anyone comes up with an answer could you let me know?
}
} Thanks in advance
}
} Gareth
} Med vänliga hälsningar/With best regards
}
} Gareth
}
} ***Come to Stockholm in 2004 to the 26th IFBLS congress*** Take a look at
} http://www.vardforbundet.se/ifbls2004
}
} http://www.ki.se/biomedlab
} e-mail Gareth.Morgan-at-labmed.ki.se
}
} Tel +46 8 5858 1038
} Fax +46 8 5858 7730
}
} Gareth Morgan MPhil MSc FIBMS,
} Department of Laboratory Medicine (Labmed),
} Karolinska Institute,
} Karolinska University Hospital at Huddinge, F46
} SE 141 86 Stockholm
} Sweden
}
} OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
} för klinisk patologi och cytologi.
}
} NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
} Clinical Histo- and Cytopathology Laboratory.
}

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370
fax +54 11 4982-4494

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 09:59:15 2004

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Hi again,

I think I have to be a bit more specific. The question is whether a FEG
is worth the extra investment for the
sort of work we are planning.

On the one hand we image individual proteins with a magnification of
20K- 50K and defocus between 1000 nm
and 2000 nm. There we want to get resolutions between 5 and 10 Angstrom.
Judging from Uwe’s plot that
shouldn’t be a problem with a LaB6.

On the other hand we image 2D crystals at about 60K magnification aiming
at a resolution of about 2 to 3 Angstrom.
Here we work much closer to focus (500 nm), which should improve the
envelope of the LaB6 quite a bit.
(It would be nice, Uwe, if you could send me a plot for 500 nm defocus
for comparison. I can’t reproduce your plots
with the parameters you give.)

For these two types of application, is there any point in investing in a
FEG?
} From what I’ve seen so far there doesn’t seem to be.

Yours sincerely,

Philip

-----Original Message-----
} From: max.sidorov-at-spansion.com [mailto:max.sidorov-at-spansion.com]
Sent: 23 April 2004 18:42
To: uwl-at-nl.feico.com; Philip.Koeck-at-biosci.ki.se; 3dem-at-ucsd.edu;
microscopy-at-sparc5.microscopy.com

Hi,

I would like to build an eyepiece with a c-mount thread.
I already have the eyepiece but without lens.
But when I look through it I only can
see part of what I can see through a 10x eyepiece. I have no
vignetting. The image looks nice. But it looks
like magnified.

Can anybody tell me which kind of lens I have to insert into
my eyepiece in order to see aproximately what I can see with
a 10x WF eyepiece.

Anneliese Schmaus

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 11:25:00 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all,

I wonder if you have recommendations for limits in the length of image file
names. For example, it happened to me that during ftp transfers some long
file names were truncated to 64 characters + extension.

I always tried to limit the most important information in the first 6 or 8
characters, but this cannot always be done.

May be you know of a practical name size that will work safely in most
cases using windows - mac - ftp - linux - internet - etc.

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370
fax +54 11 4982-4494

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 13:22:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Ramirez,

We had the same problem in our lab, during transfer from pc to a Mac-network
(everyone works with Macs, except Microscopy...). I had to reduce the
filenames to 27 characters, but by using codes, it's always possible to
trace back some photos. Here's the text I sent around in the lab for users
of the mciroscopes, hope it helps you out!
Best regards,

Sven Terclavers
____________________________________________________________________________
____________
Scoobidoo is the Microscopy-server which is used to archive images. Here
you can find out how to save and archive your image-files.

Every microscope user gets a personal folder on the server to store his/her
images. Some folders are already created, if you don't have one yet, please
contact me. Within this folder, you have to create subfolders according to
the tissue you're taking photos of followed by the year, e.g. folder 'Sven
Terclavers', subfolders 'Heart_2002', 'Limb_2002', 'Heart_2003' etc.

In these folders you can now store your images (preferably in High Quality
JPEG-format, at least 300 dpi) of the corresponding tissue. To be able to
quickly find the data about a photo (microscope, magnification, dye, …) we
can use 27 characters (without the format-extension) to name the photos. So
from now one, please always use the next configuration to store image-files:

RRRRRRmmmmTTssssDDD_Mxxxaaa.zzz

RRRRRR = description of the research (MMI, AB , PlGF, …)
mmmm = mouse number
TT = mouse type (WT, HO, HE)
ssss = slide and/or coupe-number
DDD = dye (you will find a list of abbreviations on the last page)
M = microscope (Z [Zeiss], L [Leica], C [Confocal])
xxx = magnification
aaa = number of the photo (in case you take more than one photo of a tissue)
zzz = file-format (preferably JPEG)

· e.g. MMI1306HO0416TBM_Z40x002.jpg
o MMI = Mouse myocard infarct
o 1306 = mouse number
o HO = homozygot
o 0416 = slide 04, coupe 16
o TBM = thrombomodulin staining
o Z40x = Zeiss, 40x magnification
o 002 = second image

The first part of the name makes it possible to find the slide in case a new
photo has to be taken. With the second part, followed after the underscore,
it is possible to find what microscope and magnification was used to be able
to add a scale bar afterwards. In some situations, when working on the
Leica-microscope, you might need to add more characters to the magnification
(because of the extra 2 magnification-lenses). Then you can use the extra
characters from the research-description RRRRRR, mouse-number or
photo-number.
____________________________________________________________________________
___________

-----Original Message-----
} From: Martin Ramirez [mailto:ramirez-at-amnh.org]
Sent: Monday, April 26, 2004 18:27 PM
To: microscopy-at-msa.microscopy.com

Hi all,

I wonder if you have recommendations for limits in the length of image file
names. For example, it happened to me that during ftp transfers some long
file names were truncated to 64 characters + extension.

I always tried to limit the most important information in the first 6 or 8
characters, but this cannot always be done.

May be you know of a practical name size that will work safely in most
cases using windows - mac - ftp - linux - internet - etc.

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370
fax +54 11 4982-4494

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 15:02:14 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mocherla-at-eng.fsu.edu) from
http://www.msa.microscopy.com/Ask-A-Microscopist.html on Monday,
April 26, 2004 at 12:53:13
---------------------------------------------------------------------------

Email: mocherla-at-eng.fsu.edu
Name: supriya

Organization: Florida State University

Education: Graduate College

Location: Tallahassee, Florida,

Question: I would like to observe liposomes under TEM. I found a
paper which talks about using cryo-TEM ( Ref: Almgren et al, 2000.
The procedure described there is a bit difficult. Can anybody help me
in getting this real straight by using TEM or SEM.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 15:03:21 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (cjreinbold-at-bcsew.edu) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Monday,
April 26, 2004 at 14:42:39
---------------------------------------------------------------------------

Email: cjreinbold-at-bcsew.edu
Name: Corbett

Organization: The Blood Center

Education: Graduate College

Location: Milwaukee, WI, USA

Question: Dear Microscopist,

The problem I'm having is the presence of a dark ring in the center
of field. The instrument we're using is a Zeiss Axioskop upright with
Plan-Neofluar 100X/1.30 oil ojective, with a mercury bulb having
approx. 87hrs for FITC fluorescence. The sample is a cultured cell
line using Falcon 8 well slides and using antiquench for mounting. I
have performed the easy steps of cleaning and aligning with no
clearing of the problem. Any suggestions with this problem are
welcomed.
CR-

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 16:27:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello,
What common fluorophores will serve as electron donors to HRP with
result of a precipitate that is both colored and fluorescent? I recall
a discussion on this site long ago but have not been able to find it in
the archives. Will Nile Red serve for this purpose?

Thanks,
Glen
Glen MacDonald
Core for Communication Research
Virginia Merrill Bloedel Hearing Research Center
Box 357923
University of Washington
Seattle, WA 98195-7923 USA
(206) 616-4156
glenmac-at-u.washington.edu

************************************************************************
******
The box said "Requires Windows 95 or better", so I bought a Macintosh.
************************************************************************
******

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 17:18:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

You can also download a variety of different types of batch file renaming
software from www.tucows.com

cheers,
Rosmeary

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

} From: "Sven Terclavers" {Sven.Terclavers-at-med.kuleuven.ac.be}
} Reply-To: {Sven.Terclavers-at-med.kuleuven.ac.be}
} Date: Mon, 26 Apr 2004 20:20:54 +0200
} To: "Martin Ramirez" {ramirez-at-amnh.org} , {microscopy-at-msa.microscopy.com}
} Subject: [Microscopy] RE: length of file names
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Ramirez,
}
} We had the same problem in our lab, during transfer from pc to a Mac-network
} (everyone works with Macs, except Microscopy...). I had to reduce the
} filenames to 27 characters, but by using codes, it's always possible to
} trace back some photos. Here's the text I sent around in the lab for users
} of the mciroscopes, hope it helps you out!
} Best regards,
}
} Sven Terclavers
} ____________________________________________________________________________
} ____________
} Scoobidoo is the Microscopy-server which is used to archive images. Here
} you can find out how to save and archive your image-files.
}
} Every microscope user gets a personal folder on the server to store his/her
} images. Some folders are already created, if you don't have one yet, please
} contact me. Within this folder, you have to create subfolders according to
} the tissue you're taking photos of followed by the year, e.g. folder 'Sven
} Terclavers', subfolders 'Heart_2002', 'Limb_2002', 'Heart_2003' etc.
}
} In these folders you can now store your images (preferably in High Quality
} JPEG-format, at least 300 dpi) of the corresponding tissue. To be able to
} quickly find the data about a photo (microscope, magnification, dye, …) we
} can use 27 characters (without the format-extension) to name the photos. So
} from now one, please always use the next configuration to store image-files:
}
} RRRRRRmmmmTTssssDDD_Mxxxaaa.zzz
}
} RRRRRR = description of the research (MMI, AB , PlGF, …)
} mmmm = mouse number
} TT = mouse type (WT, HO, HE)
} ssss = slide and/or coupe-number
} DDD = dye (you will find a list of abbreviations on the last page)
} M = microscope (Z [Zeiss], L [Leica], C [Confocal])
} xxx = magnification
} aaa = number of the photo (in case you take more than one photo of a tissue)
} zzz = file-format (preferably JPEG)
}
} · e.g. MMI1306HO0416TBM_Z40x002.jpg
} o MMI = Mouse myocard infarct
} o 1306 = mouse number
} o HO = homozygot
} o 0416 = slide 04, coupe 16
} o TBM = thrombomodulin staining
} o Z40x = Zeiss, 40x magnification
} o 002 = second image
}
} The first part of the name makes it possible to find the slide in case a new
} photo has to be taken. With the second part, followed after the underscore,
} it is possible to find what microscope and magnification was used to be able
} to add a scale bar afterwards. In some situations, when working on the
} Leica-microscope, you might need to add more characters to the magnification
} (because of the extra 2 magnification-lenses). Then you can use the extra
} characters from the research-description RRRRRR, mouse-number or
} photo-number.
} ____________________________________________________________________________
} ___________
}
}
}
}
}
} -----Original Message-----
} } From: Martin Ramirez [mailto:ramirez-at-amnh.org]
} Sent: Monday, April 26, 2004 18:27 PM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy] length of file names
}
}
}
}
} ----------------------------------------------------------------------------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ----------------------------------------------------------------------------
} ---
}
} Hi all,
}
} I wonder if you have recommendations for limits in the length of image file
} names. For example, it happened to me that during ftp transfers some long
} file names were truncated to 64 characters + extension.
}
} I always tried to limit the most important information in the first 6 or 8
} characters, but this cannot always be done.
}
} May be you know of a practical name size that will work safely in most
} cases using windows - mac - ftp - linux - internet - etc.
}
}
}
} Martín J. Ramírez
} División Aracnología
} Museo Argentino de Ciencias Naturales
} Av. Angel Gallardo 470
} C1405DJR Buenos Aires
} Argentina
} tel +54 11 4982-8370
} fax +54 11 4982-4494
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Apr 26 18:10:07 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Supriya,

I used to do a lot of TEM of liposomes a few years back, and we always used
fairly simple negative staining protocols, in which the liposomes are mixed
with an electron-dense stain, applied to a grid, the excess is wicked off, and
the remaining thin film of solution is allowed to air-dry. You can use uranyl
acetate, phosphotungstic acid, phosphomolybdic acid or others to stain.

We used glow-discharged carbon films on grids to make the carbon "wettable."
Otherwise, the film is hydrophobic and won't spread the staining solution
properly.

There are lots of recipes out there; consult any good resource that discusses
negative staining of viruses, bacteria, proteins, lipoproteins, etc. For
example, see:

{http://www.urmc.rochester.edu/research/emimg/negstain.html}

Good luck!

Bob Chiovetti
RMC/Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 02:18:27 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

In biology we use the microscope quite differently than material
scientists generally do. We never work at Scherzer defocus and we try to
get as close as possible to the information limit by averaging and
CTF-correction based on the weak phase / weak amplitude object
approximation. I think that should get rid of delocalization. You can
look up the method for example at
http://ncmi.bcm.tmc.edu/~stevel/EMAN/doc/.

By resolution I don't mean point resolution. The resolution we aim at is
close to the information limit at the highest underfocus we used to take
the images. We can only achieve this resolution in the final average
(actually a 3D model) but not in an individual image.
For that sort of imaging the FEG does have advantages because the
information limit is better (but I'm not sure whether the advantages are
big enough to justify the higher price). Max Sidorow shows that nicely
at http://clik.to/ctfexplorer (click on "science behind it").

To clarify: We have to use high defocus because we need good contrast
transfer at very low spatial frequencies to be able to see the protein
molecules.

We use film and scan it with 7 micron pixels.

-----Original Message-----
} From: A.Chuvilin [mailto:andrey.chuvilin-at-tu-ilmenau.de]
Sent: 27 April 2004 03:00
To: Philip Koeck

Hi,

Here is a website which deals with cross-platform compatible files -
file naming issues:

http://www.imagemontage.com/Docs/FileNames.html

Windows-NT does not like to have a "." (period) at the end of a file
name and cannot access files with "/" (forward slash) anywhere in the
file name, so you will have to deal with this when exchanging files from
Mac to Windows.

There is a program available which deals with the conversion of Mac
filenames to the MS-Windows standard:

http://peccatte.karefil.com/software/MacNames/MacNamesEN.htm

There are some restrictions on filenames in Unix/Linux, but it is a
possible intermediary to store files which you have to exchange between
Mac and MS-Windows.

Here is some information on the filenames on Linux:

http://farside.ph.utexas.edu/teaching/329/lectures/node12.html

I thought that since WinNT, the "MS-DOS" derived operating systems could
also handle long filenames ?

I use a Linux-system with SAMBA to exchange files between systems, it
makes the Linux-server act like an NT/W2000/XP-server (it is free):

http://samba.anu.edu.au/samba/

If you install Netatalk on the same Linux-system, you can excahnge files
between MS-Windows and Macintosh (Netatalk is also free):

http://netatalk.sourceforge.net/

Regards,

Peter Van Osta

Director Imaging
MAIA SCIENTIFIC (formerly Union Biometrica NV)
Cipalstraat 3
B-2440 Geel
Belgium
Tel.: +32-(0)14 570 620
Fax.: +32-(0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company

====================================================================================
} } ----------------------------------------------------------------------------
} } --
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 07:12:46 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I think it's time to get this question out of the way once and for all.

The point that Henning makes indicates that CTF explorer is unrealistic
since such low convergence angles require very long exposure times. That
means CTF explorer can be quite misleading if you use it to judge the
suitability of a microscope for structural biology.

On the other hand I don't think Hennings simulation at
http://www.amp.ucdavis.edu/index.php?p=download do a LaB6-instrument
complete justice.
If I type in parameters for a Philips CM120 at 1500 nm defocus, using
0.7 mrad convergence angle the plot shows an information limit of about
16 Angstrom. With our old CM120 I have recorded images of carbon film at
45K magnification, 1500 nm defocus and 1 second exposure time where the
CTF shows oscillations out to beyond 10 Angstrom. That certainly isn't
the limit for that microscope either, since the filament wasn't
especially new at the time and I recorded quite a small area on a 1K CCD
camera.
Maybe the convergence angle for a LaB6 should be a bit smaller than 0.7
mrad.

What would really settle it for me is some experimental data.

Does anybody have a direct comparison between a FEG and a LaB6 that are
otherwise equivalent, for example images of carbon film taken around 50K
magnification and 1500 nm defocus with identical settings for exposure
time, apertures etc? Maybe the same with a well-used LaB6 filament to
see how quickly a LaB6 deteriorates?
The EM manufacturers ought to have data like that!? Or does anybody know
of a publication?

Philip

-----Original Message-----
} From: Henning Stahlberg [mailto:HStahlberg-at-ucdavis.edu]
Sent: 26 April 2004 19:38
To: Philip Koeck
Cc: 3dem-at-ucsd.edu

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi,

Here is a website which deals with cross-platform compatible files -
file naming issues:

http://www.imagemontage.com/Docs/FileNames.html

Windows-NT does not like to have a "." (period) at the end of a file
name and cannot access files with "/" (forward slash) anywhere in the
file name, so you will have to deal with this when exchanging files from
Mac to Windows.

There is a program available which deals with the conversion of Mac
filenames to the MS-Windows standard:

http://peccatte.karefil.com/software/MacNames/MacNamesEN.htm

There are some restrictions on filenames in Unix/Linux, but it is a
possible intermediary to store files which you have to exchange between
Mac and MS-Windows.

Here is some information on the filenames on Linux:

http://farside.ph.utexas.edu/teaching/329/lectures/node12.html

I thought that since WinNT, the "MS-DOS" derived operating systems could
also handle long filenames ?

I use a Linux-system with SAMBA to exchange files between systems, it
makes the Linux-server act like an NT/W2000/XP-server (it is free):

http://samba.anu.edu.au/samba/

If you install Netatalk on the same Linux-system, you can excahnge files
between MS-Windows and Macintosh (Netatalk is also free):

http://netatalk.sourceforge.net/

Regards,

Peter Van Osta

Director Imaging
MAIA SCIENTIFIC (formerly Union Biometrica NV)
Cipalstraat 3
B-2440 Geel
Belgium
Tel.: +32-(0)14 570 620
Fax.: +32-(0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company

====================================================================================
} } ----------------------------------------------------------------------------
} } --
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 08:44:51 2004

Contents Retrieved from Microscopy Listserver Archives
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} Ask your Zeiss rep to take a careful look at the collcting lens that
} brings the light from the Hg lamp house into the microscope body.
} We have had the one on our Axiovert become fogged (the coatings
} become slightly opaque from the heat of the lamp). I've been told
} that the problem has been solved in recent years, but if your
} microscope is 5 or 6 years old, this may be the problem.

Lee
****************************
} The problem I'm having is the presence of a dark ring in the center
} of field. The instrument we're using is a Zeiss Axioskop upright
} with Plan-Neofluar 100X/1.30 oil ojective, with a mercury bulb
} having approx. 87hrs for FITC fluorescence. The sample is a cultured
} cell line using Falcon 8 well slides and using antiquench for
} mounting. I have performed the easy steps of cleaning and aligning
} with no clearing of the problem. Any suggestions with this problem
} are welcomed.
} CR-
}
}
} ---------------------------------------------------------------------------

--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 09:17:51 2004

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Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Title-Subject: [Microscopy] [Filtered] Light Microscope Repair

Question: We have a LEICA Ergoplan light microscope in need of
repair. The DIC no longer works. Can anyone suggest a repair
service company? We are located in Newark, DE.

Thanks

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From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 09:21:35 2004

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Hi,

In biology we use the microscope quite differently than material
scientists generally do. We never work at Scherzer defocus and we try to
get as close as possible to the information limit by averaging and
CTF-correction based on the weak phase / weak amplitude object
approximation. I think that should get rid of delocalization. You can
look up the method for example at
http://ncmi.bcm.tmc.edu/~stevel/EMAN/doc/.

By resolution I don't mean point resolution. The resolution we aim at is
close to the information limit at the highest underfocus we used to take
the images. We can only achieve this resolution in the final average
(actually a 3D model) but not in an individual image.
For that sort of imaging the FEG does have advantages because the
information limit is better (but I'm not sure whether the advantages are
big enough to justify the higher price). Max Sidorow shows that nicely
at http://clik.to/ctfexplorer (click on "science behind it").

To clarify: We have to use high defocus because we need good contrast
transfer at very low spatial frequencies to be able to see the protein
molecules.

We use film and scan it with 7 micron pixels.

-----Original Message-----
} From: A.Chuvilin [mailto:andrey.chuvilin-at-tu-ilmenau.de]
Sent: 27 April 2004 03:00
To: Philip Koeck

On Thu, 22 Apr 2004, Judy Murphy wrote:
} Now that we do microwaving however we can do the entire process in one
} short morning.

Yea, just rub it in that you've got the wonderful microwave system!!!

I'm just kidding--sort of : )--but I also wanted to thank you for the
great 'practical' information that you have shared with the list.

Karen Bovard
Omaha NE

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 15:00:03 2004

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On Apr 26, 2004, at 6:45 AM, Philip Koeck wrote:

} I think I have to be a bit more specific. The question is whether a FEG
} is worth the extra investment for the
} sort of work we are planning.
}
} On the one hand we image individual proteins with a magnification of
} 20K- 50K and defocus between 1000 nm
} and 2000 nm. There we want to get resolutions between 5 and 10
} Angstrom.
} Judging from Uwe’s plot that
} shouldn’t be a problem with a LaB6.
}
} On the other hand we image 2D crystals at about 60K magnification
} aiming
} at a resolution of about 2 to 3 Angstrom.
} Here we work much closer to focus (500 nm), which should improve the
} envelope of the LaB6 quite a bit.
} (It would be nice, Uwe, if you could send me a plot for 500 nm defocus
} for comparison. I can’t reproduce your plots
} with the parameters you give.)
}
} For these two types of application, is there any point in investing in
} a
} FEG?
}
Dear Philip,
There has certainly been a lot of single-particle work done using a
LaB6 filament; however, little of it has had as good as 1 nm resolution
in the 3D reconstructions. Of course, there are other issues, such as
alignment, that play a role in limiting resolution. One thing to keep
in mind is that the better the envelope function, the higher the S/N
ratio in the images, so, although you might be able to obtain useful
images with the resolution range of interest using a LaB6, you might be
better able to determine structures with the better S/N from the FEG.
I.e., a FEG will produce better data. On the other hand, you are
surely comparing getting the FEG vs. getting something else--other
equipment, more post-docs, etc.--and I cannot make this judgment for
you.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 18:36:00 2004

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Dear Anneliese,

The problem you describe is a common one and is due to the "camera factor". There are a number of issues,including the length of your phototube and the size of the detector (chip) in your camera.

Rather than trying to re-engineer the system, I would suggest that you call
a. Your local microscope rep, to see if he has a 0.5x (or similar) projection eyepiece to go in your phototube or
b. A company such as OPTEM or Diagnostic Instruments, both of whom make great phototubes which might also solve the problem. I think you will probably find both of them listed at www.microscopy.info

Hope this is helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

~-at-~-at-~~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-

At 05:44 PM 4/26/04 +0200, Klughammer wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 18:36:00 2004

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Dear Anneliese,

The problem you describe is a common one and is due to the "camera factor". There are a number of issues,including the length of your phototube and the size of the detector (chip) in your camera.

Rather than trying to re-engineer the system, I would suggest that you call
a. Your local microscope rep, to see if he has a 0.5x (or similar) projection eyepiece to go in your phototube or
b. A company such as OPTEM or Diagnostic Instruments, both of whom make great phototubes which might also solve the problem. I think you will probably find both of them listed at www.microscopy.info

Hope this is helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education
125 Paridon Street, Suite 102
Springfield, MA 01118
PH: 413-746-6931 FX: 413-746-9311 Web: www.MicroscopyEducation.com

~-at-~-at-~~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-

At 05:44 PM 4/26/04 +0200, Klughammer wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 22:07:49 2004

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Dear Fellow Microscopists,

In our lab we want to switch from the conventional (heated rod) to
electron beam evaporation of carbon. I remember seeing some time ago
information on the web or on this list about a simple homebrew electron
beam evaporator. The unit looked fairly small. I tried finding the info
again but with no success. If someone has a link or other pointer -
please help.
We cannot justify spending money on a new electron beam evaporation
system. I hope it will be possible to modify our current vacuum
evaporator. It is of the old JEOL type with bell jar and diffusion pump
system. The model is JEOL JEE-400.
I will highly appreciate any information/advice/experience about such
modification.
Information about small commercial electron beam evaporation systems is
also welcome.

With regards,

Radostin Danev

-----------------------------------------------------
Radostin Danev, Ph.D.
Laboratory of Nano-Structure Physiology
Center for Integrative Bioscience
Okazaki National Research Institutes
tel: +81-564-59-5563
fax: +81-564-59-5554
e-mail: rado-at-nips.ac.jp
-----------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Apr 27 23:24:48 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rstark18-at-bellsouth.net) from
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Tuesday, April 27, 2004 at 17:35:40
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Email: rstark18-at-bellsouth.net
Name: Ronnie Stark

Title-Subject: [Microscopy] [Filtered] MListserver:RCA emu4 electron microscope

Question: Is anyone out there still using an RCA EMU4 electron
microscope. I (actually, a friend of mine) have one in working order,
and many extra parts. We have boards a-e,etc. If anyone is interested
in the scope or parts for it, please email me. Thanks, Ronnie

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Hi all

I am working on the phase transformation aspects of an alpha+beta titanium
alloy. I would like to study the formation of Widmanstatten alpha and
serrated alpha using ATEM and HRTEM. I would like to get suggestions as to
what are the signatures for these products to look for and also the journal
articles/books to read about them.

Thanks and regards
Mythili R

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 28 12:05:55 2004

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Hello,
I am attempting to bring an LKB 2128 IV ultramicrotome back into service
and would like to have the original documentation. Please contact me if you
can provide copies of the operator and/or service manuals. The thermal arm
feed indicator lamp is lit continually and the reset does not seem to be
working. I would also appreciate any user comments about this machine:
reliability, ease of use? It seems a bit gimmicky. I am experienced with
operating and servicing the LKB I, III and V microtomes.
Thank you.
Jim

James S. Romanow
The University of Connecticut
Physiology and Neurobiology Department
Electron Microscopy Facility
Unit 3242
BSP Building, Room G06
91 North Eagleville Road
Storrs, CT 06269-3242

860 486-2914 voice
860 486-6369 fax
james.romanow-at-uconn.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Apr 28 18:27:03 2004

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Hi listserver,
I am recently working with the ultrastructure of the
sporophyte and gametophyte of Frullania brasiliensis, a
Marchantiophyta (Hepatophyta). I am fixing the samples in a
mixture of glutaraldehyde and formaldeyde an post fixing in
osmium tetroxide. However, during the dehydration, the
samples suffer shrink, mainly the young sporophytes. I used
ethanol or acetone (10, 30, 50, 70, 90, 90, 100, 100 steps,
15 minutes each) without success. I also used acidified DMP
(dimetoxypropane), also with bad results. Do you have some
suggestion to avoid this problem? Which the recommended
protocol for the study of delicate bryophytes under TEM and
SEM?
Sincerely,
Prof. Rinaldo Pires dos Santos
*****************************************************
Prof. Dr. Rinaldo Pires dos Santos
Lab. de Anatomia Vegetal
Dept. de Botânica - UFRGS
Av. Bento Gonçalves, 9500 - Bloco IV - Prédio 43423 - Sala 208
91501-970 - Porto Alegre - RS
Brazil
Fone:+55 51 33167758 - Fax: +55 51 33167670
E-mail: rinaldop-at-uol.com.br

---
Acabe com aquelas janelinhas que pulam na sua tela.
AntiPop-up UOL - É grátis!
http://antipopup.uol.com.br

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 00:19:42 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (WWiggins-at-Carolinas.org) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, April 28, 2004 at 14:16:09
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Email: WWiggins-at-Carolinas.org
Name: Winston Wiggins

Organization: Carolinas HealthCare System

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Are there any labs, commercial or otherwise, in the Carolinas or vicinity that does immunogold for type I collagen - quickly and painlessly?

Winston W. Wiggins, Supervisor
Cannon Electron Microscopy Lab
Carolinas Medical Center
P.O. Box 32861; Charlotte, NC 28232-2861
Ship to: 1000 Blythe Blvd; Charlotte, NC 28203
Ofc:704-355-1267 ; Lab:704-355-7220 ; Fax 704-355-0589
E-mail: Winston.Wiggins-at-CarolinasHealthCare.org {mailto:WWiggins-at-Carolinas.org}

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From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 02:25:09 2004

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hello microscopists (for sure better than me ;-) ) !

please, Can someone tell me what is exactly immunogold, and its function
in SEM or FESEM ?

thank you in advance...

Sylvain MAURY, in FRANCE

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 05:36:07 2004

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Hi,

does anyone know who sells sputter coaters for 300 mm wafers for SEM sample preparation ?

Thanx.

Andreas M.

&-] ############################### &-]

Moritz Andreas Meyer
Dipl.-Ing (FH) MSc.
Sr. Materials Analyst SEM
Materials Analysis Department

AMD Saxony LLC & Co. KG
Wilschdorfer Landstraße 101
D-01099 Dresden

Tel. +49 351 277 4149
Fax. +49 351 277 9 4149
E-Mail. moritz-andreas.meyer-at-amd.com

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 06:53:41 2004

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Hi,

You can find information about immunogold on the website of Aurion:

http://www.aurion.nl/

Regards,

Peter Van Osta

P.S. I have no commercial interest in the company.

========================================
sylvain maury wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} hello microscopists (for sure better than me ;-) ) !
}
} please, Can someone tell me what is exactly immunogold, and its function
} in SEM or FESEM ?
}
} thank you in advance...
}
} Sylvain MAURY, in FRANCE

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 08:45:47 2004

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hello (second time)

sorry but the website www.aurion.nl is not working well.

So I must precise my applications in FESEM : i'm currently doing
observations of prepared samples (polished, coated...or not) of
microelectronics (Si, AsGa, ULSI/VLSI,).

What is immunogold ?
How can immunogold be useful for my applications ? is there an interest
for me to look for this item ?

I read it's used for biomedical and biology SEM applications...

Thanx for answers.

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 11:23:22 2004

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On Apr 29, 2004, at 6:45 AM, sylvain maury wrote:

} So I must precise my applications in FESEM : i'm currently doing
} observations of prepared samples (polished, coated...or not) of
} microelectronics (Si, AsGa, ULSI/VLSI,).
}
} What is immunogold ?
} How can immunogold be useful for my applications ? is there an interest
} for me to look for this item ?
}
} I read it's used for biomedical and biology SEM applications...
}
} Thanx for answers.
}
Dear Sylvain,
Immunogold is formed from an antibody molecule that is chemically
bonded to a small--~5 nm--bead of gold. Different size gold beads can
be used allowing one to distinguish between different antibodies that
can be used simultaneously. The immunogold staining method allows one
to determine the locations of specific molecules that react with
antibodies, so it is useful for biological specimens. However, since
simple compounds generally do not react with antibodies, and since the
microelectronics samples you are investigating consist of large areas
that have the same composition, immunogold is not likely to be of any
use to you (unless you are trying to detect macromolecular species
adhering to the surface of your specimens).
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 11:46:32 2004

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Sylvain: I've been doing materials and semiconductor SEM for 20+ years
and never once have I had a need for immunogold. In fact, even if I
wanted to use it for some obscure reason, I don't think I could due to
the materials and the chemistry involved. So that's one less thing for
you to worry about.

sylvain maury wrote:

} ------------------------------------------------------------------------------
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--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 12:39:12 2004

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Try Emitech.

http://www.emitech.co.uk/sputtercoating.html

K695X for 12" wafers.

gary g.

At 03:35 AM 4/29/2004, you wrote:

} Hi,
}
} does anyone know who sells sputter coaters for 300 mm wafers for SEM
} sample preparation ?
}
} Thanx.
}
} Andreas M.
}
} &-] ############################### &-]
}
} Moritz Andreas Meyer
} Dipl.-Ing (FH) MSc.
} Sr. Materials Analyst SEM
} Materials Analysis Department
}
} AMD Saxony LLC & Co. KG
} Wilschdorfer Landstraße 101
} D-01099 Dresden
}
} Tel. +49 351 277 4149
} Fax. +49 351 277 9 4149
} E-Mail. moritz-andreas.meyer-at-amd.com

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 13:23:19 2004

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I am trying to do some freeze substitution using uranyl acetate in
anhydrous acetone. There are lots of references in the literature where
individuals use UA at concentrations of 0.1, 0.2, 0.5, 1.0 or even 2% in
acetone. I tried to make up a batch yesterday and barely any went into
solution. I doubt I achieved even 0.1% solubility. Any insights into this
problem would be appreciated. Thanks, Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 15:33:38 2004

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Fellow microscopists:

I recently read about a product - plastic cell culture dishes which do
not polarize light to the same extent as the conventional ones and can
therefore be used for DIC. Unfortunately, I do not remember the name of
the company(ies) that manufacture these. Could anyone please tell me. I
would appreciate hearing from the companies themselves.

Thank you
Judy

Judy Trogadis
Bio-Imaging Coordinator
St. Michael's Hospital, 7Queen
30 Bond St.
Toronto, ON M5B 1W8
Canada
ph: 416-864-6060 x6337
pager: 416-685-9219
fax: 416-864-6043
trogadisj-at-smh.toronto.on.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 16:03:55 2004

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For those planning on attending the May 7th meeting of the Central
States Microscopy and Microanalysis Society, here is a link to the
current schedule, updated parking information, and directions:
http://www.biotech.missouri.edu/emc/csmms.htm.

Be there!

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Thu Apr 29 17:03:27 2004

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tom

in an early life, when i was more A-compulsive, i tried to dehydrate
with UA in the dehydrant. my normal choice is acetone. i found that i
could get 2% UA in 10%. by values above 50% the solubility of UA was
virtually 0. solubility in EtOH was worse.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 01:55:25 2004

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Hello, Everyone,

I need to estimate the local temperature in the beam
area of the thin TEM sample (inorganic)when doing
micro/nano-diffraction or HREM imaging. We use normal
specimen holder. Does anybody have some ideas of it?

Thanks, wish you all a nice weekend.

-juha

__________________________________
Do you Yahoo!?
Win a $20,000 Career Makeover at Yahoo! HotJobs
http://hotjobs.sweepstakes.yahoo.com/careermakeover

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 02:25:50 2004

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Hello everyone !

For this time, i haven't got any question to ask.

All I want is to greatly thank all the people on the microscopy
community MSA for answering and sharing their knowledge. When i sent my
first message, i thought nobody would answer my questions, but i was
nicely surprised when i received answers from many people who work in
the same way of interest.

i'm happy to see that microscopy VIPs ;-) , are very nice persons and
that everyone is always in a good mood to help beginners like me.

Thank you all again.

Sylvain MAURY, a young SEM french student in Failure Analysis (not so
young, after all)

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 04:45:09 2004

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Čçďđŕňĺíî ÎŇ (Izprateno Ot) : microscopy-at-sparc5.microscopy.com
Äî (Do): embrd_bg-at-cablebg.net

.. č ĺ ńúń ńëĺäíčňĺ ńęóćĺáíč äŕííč:
.. i e sus slednite sluzhebni danni:

---
MAILFROM: microscopy-at-sparc5.microscopy.com
Received: from unknown (HELO cablebg.net) (81.198.116.105)
by mail.interbgc.com with SMTP; 30 Apr 2004 09:45:09 -0000
} From: microscopy-at-sparc5.microscopy.com
To: embrd_bg-at-cablebg.net

I have run into a problem here that Amray/KLA tech support has not had a
chance to figure out.

I had 2 researchers yesterday capturing digital images off our 1810 with
the included image control/nybblenet package. Unfortunately they
inadvertently turned off the data bar in the software and thus have no idea
as to the scale of their images. I know there is info placed in the tiff
header file that records instrument settings, and I have tried several
packages that have some ability to mine the header, but none have been able
to dig out the Amray specific stuff. There are about 200 images involved and
2 of the samples cannot be reshot. To make matters worse, one of the
researchers has to fly off back home today.

Anyone know how to mine out the header data so that I can at least
calculate or better yet regenerate the databar. HELP

Scott Whittaker
Laboratories of Analytical Biology
Smithsonian Institution
National Museum of Natural History
PO Box 37012 MRC104
Washington DC 20013-7012
202-357-1651

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 10:10:31 2004

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Paul,
I had similar or worst experiences with dissolving UA in acetone. I
also could not get it to go in completely in water either. It depended on
the particular bottle(s) of UA.

However, I recently got some of the certified depleted UA from EMS and it
went in without even stirring! Then I was at another facility that hauled
out some ancient UA that hadn't been used in years. It also went into water
with minimal agitation. One good thing is that when you find a good bottle
it will last for many years.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 4/29/04 5:02 PM, "paul r hazelton" {paul_hazelton-at-umanitoba.ca} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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}
} tom
}
} in an early life, when i was more A-compulsive, i tried to dehydrate
} with UA in the dehydrant. my normal choice is acetone. i found that i
} could get 2% UA in 10%. by values above 50% the solubility of UA was
} virtually 0. solubility in EtOH was worse.
}
} paul
}
} Paul R. Hazelton, PhD
} Electron Microscope Unit
} University of Manitoba
} Department of Medical Microbiology
} 531 Basic Medical Sciences Building
} 730 William Avenue
} Winnipeg, Manitoba, Canada, R3E 0W3
} e-mail: paul_hazelton-at-umanitoba.ca
} Phone:204-789-3313
} Pager:204-931-954
} Cell:204-781-1502
} Fax:204-789-3926
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 11:14:40 2004

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I am looking for someone who has an SEM with a heating stage.

Please contact me off list.

Mark Germani, Ph.D.
MicroMaterials Research, Inc.
136 Shore Drive, #200
Burr Ridge, IL 60527

(630) 325-8170
(630) 325-8178 fax

mgermani-at-micromaterialsresearch.com
www.MicroMaterialsResearch.com

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 11:19:13 2004

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I have been testing a variety of backscatter detectors recently under
conditions of relatively high beam current, longer integration times, and
high amplifier gain. It would appear many of the BSED and amplifiers can
approach better precision than assumed by many current frame stores. That
is, BEI better than 0.1Z -at- Z=30 should be better than 1 part in 255, and
more worthy than 8bit frame stores.

However, it also seems I cannot assume I can back off on amplifier gain,
acquire a greater dynamic range (Z), and assume the same precision (i.e.,
0.1Z is no longer maintained). Under these same conditions, with gain set
for full dynamic range (e.g., Z=10-30), can I evaluate the resulting
histogram distribution from a homogeneous phase (e.g., Ti metal), and
calculate, or otherwise relate the distribution to digital bit depth? I
imagine some type of relationship between the noise distribution and atomic
number resolution(?)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 13:22:09 2004

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Debby

it may depend upon the lot. i have some old stuff from TAAB (that goes
back a way) that works beautifully, while i have a bottle from EMS which
has been iffy, and i like them. now, however, i have to find out which
bottle was used by the student made the last aqueous batch for negative
stain, because it precipitated. of course, if it is who i suspect, she
also tried to adjust the pH to 7.0 since we do that for PTA.

it was the better soluble material that did not go into solution in 10%
EtOH or 50% acetone. either way, including UA in the dehydrant after en
bloc fixation/staining did not make any difference in the final product
so i stopped doing it on the basis that it was a questionable step which
only contributed to the waste disposal and time/work for solution
preparation problems.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 15:49:40 2004

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You are absolutely correct. I had a bottle bought 9 months ago that does
not dissolve well while a new bottle from a different lot does great...

I have used it in 100% acetone for FS and in water or methanol for routine
staining.

Debby

On 4/30/04 1:21 PM, "paul r hazelton" {paul_hazelton-at-umanitoba.ca} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Debby
}
} it may depend upon the lot. i have some old stuff from TAAB (that goes
} back a way) that works beautifully, while i have a bottle from EMS which
} has been iffy, and i like them. now, however, i have to find out which
} bottle was used by the student made the last aqueous batch for negative
} stain, because it precipitated. of course, if it is who i suspect, she
} also tried to adjust the pH to 7.0 since we do that for PTA.
}
} it was the better soluble material that did not go into solution in 10%
} EtOH or 50% acetone. either way, including UA in the dehydrant after en
} bloc fixation/staining did not make any difference in the final product
} so i stopped doing it on the basis that it was a questionable step which
} only contributed to the waste disposal and time/work for solution
} preparation problems.
}
} paul
}
}
} Paul R. Hazelton, PhD
} Electron Microscope Unit
} University of Manitoba
} Department of Medical Microbiology
} 531 Basic Medical Sciences Building
} 730 William Avenue
} Winnipeg, Manitoba, Canada, R3E 0W3
} e-mail: paul_hazelton-at-umanitoba.ca
} Phone:204-789-3313
} Pager:204-931-954
} Cell:204-781-1502
} Fax:204-789-3926
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Apr 30 16:17:38 2004

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List members,

I would like to hear from individuals who have experience with the three
possible FESEM gun types; cold cathode, thermal assisted cold cathode and
Schottky. I understand the theoretical differences but want practical
information such as:
# beam hours before tip change
Downtime related to gun/vacuum problems
Stability
Flashing routine for CC
Anything else of relevance

I would love to hear from those who have experience with both CC and
Schottky who can do an objective comparison of performance...especially in a
multi-user facility. Please answer off-line if you would be willing to
provide information about specific instruments. I want to avoid any
references on the list to specific vendors products that may not be
complimentary. I am sure all would love to have you send the very positive
replies to the list if you so desire.

Also, comments on diffusion pump/rotary pump or turbo pump/scroll pump
systems for high end FESEMs would also be helpful. Specific information
would be:
Reliability
Noise
Pumping speed
Does it really matter which system if you are not in a clean room situation?
Etc.

Many thanks in advance,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Sat May 1 08:58:08 2004

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Colleagues

The April Archives are now on-line.

http://www.microscopy.com/MicroscopyListserver

Nestor
Your Friendly Neighborhood SysOop

From MicroscopyL-request-at-ns.microscopy.com Sat May 1 08:59:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (esem1-at-traceevidence.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, May 1, 2004 at 08:36:12
---------------------------------------------------------------------------

Email: esem1-at-traceevidence.org
Name: David Spence

Organization: Southwestern Institute of Forensic Sciences

Title-Subject: [Microscopy] [Filtered] MListserver:Looking For Used SEM, EDS and Coating Equipment

Question: I am looking for used SEM, EDS, sputter/carbon coater and related equipment. If you have or know of any equipment that is serviceable and available for haul-off or very inexpensive, please let me know. I am specifically looking for an older quality SEM with a motorized stage that is suitable for automated gunshot residue analysis.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 13:14:45 2004

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Dear Colleagues,

I am involved with a consortium that is being partially funded by the
NSF-ATE program. The main project involves the development of 3-D
images related to various science, math, engineering and technology
areas (from molecules to organs to CAD/architecture) so that they can
be projected (stereographic projection). Each institution
participating in the project will have a 3-D theatre built so that
SMET classes can be brought in for demonstrations of course specific
images (the theatre will house a Barco 3-D projector driven by a SGI
UNIX-based workstation and a special screen that retains
polarization). Students and faculty from the partner institutions
will also be trained in a residential program at Brookhaven National
Lab by their 3-D Visualization Team.

Since I have been teaching TEM and SEM courses at NCC for almost 20
years, I thought that it would be an interesting project to render
student and my own SEM & TEM images for 3-D projection. I have seen
many threads on 3-D imaging on this listserver and I would appreciate
some advice on where to begin. Initially, I am supposed to identify
some software applications that would be suitable for rendering 3-D
images of my micrographs. I am aware of some of the applications that
are used at BNL for their 3-D theatre such as OpenDX, Open GL and
Visualization ToolKit (VTK).

Can anyone suggest an application (UNIX based ideally) that I might
get started with? As a novice in this area I realize that the concept
of 3-D imaging and stereographic projection are probably two entirely
different principles. I would appreciate any references (articles,
books, websites) that will help me to understand the concepts.

Thanks for any assistance you can provide!

Steve
--
Stephen J. Beck
Professor
Bio-Imaging Center/Electron Microscopy
Department of Biology
Nassau Community College
Garden City, NY 11530
Voice Mail: (516) 572-7829
Email: {becks-at-sunynassau.edu}
URL: {http://www.sunynassau.edu/webpages/biology/becks.htm}

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 15:13:18 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (yuansheng-sun-at-uiowa.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Sunday, May 2, 2004 at 14:45:18
---------------------------------------------------------------------------

Email: yuansheng-sun-at-uiowa.edu
Name: Yuansheng Sun

Organization: University of Iowa

Education: Graduate College

Location: Iowa city, IA, USA

Question: Dear Madam or Sir:

I am doing a project on deconvolution for 3D phase contrast microscopy. As you know, it is very hard to measure a real psf. So I am wondering how to construct a theoretical psf based on the experimental parameters. Could you give me some infomation on this like some books or papers or technology documents. Thanks!
best from yuansheng

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 16:07:25 2004

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I have been using ImageJ and the VolumeJ plugin (for surface
rendering) to generate 3D anaglyphs (red/green stereo) as animations.
As has been mentioned in this group before, ImageJ is a free program
that has been ported from NIH-Image to the Java platform so that it
will work on almost any machine. You can get more information on
ImageJ at http://rsb.info.nih.gov/ij/

You can download a couple of the anaglyphs at
http://astro.temple.edu/~jbs/research/Anaglyphs. Remember that you
will need red/green glasses to get the full effect.

Joel

The images were originally obtained as z-series with a Leica confocal
microscope.

Date sent: Sun, 02 May 2004 14:17:59 -0400
} From: Steve Beck {becks-at-sunynassau.edu}

I second Joel's suggestion of ImageJ/VolumeJ. You might also want to take a look at VisBio (http://www.loci.wisc.edu/VisBio). VisBio is a open-source JAVA based image analysis tool for multidimensional biological image data. Features include measurement, volume rendering, and arbitrary image stack slicing. Integration with ImageJ is under development.

best regards,
kevin

Kevin W. Eliceiri
Laboratory for Optical and Computational Instrumentation
http://www.loci.wisc.edu
Room 271 Animal Sciences
1675 Observatory Drive
Madison, WI 53706
Phone: 608-263-6288
Fax: 608-265-3083

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 19:05:12 2004

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Dear Steve,

I guess you know about the GeoWall (http://geowall.geo.lsa.umich.edu/)
projects. This is for geologists, but quite amenable to any type of 3D
projection really. Somewhat different to the setup you're proposing,
because it's PC- or Mac-based, but same principles. There's even a company
(VRCO) that sells turnkey systems. There is a bit of background information
on the GeoWall site, but more info on some of the link sites.

cheers,
Rosemmary

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

} From: Steve Beck {becks-at-sunynassau.edu}
} Date: Sun, 02 May 2004 14:17:59 -0400
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] 3-D Imaging & Projection
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Dear Colleagues,
}
} I am involved with a consortium that is being partially funded by the
} NSF-ATE program. The main project involves the development of 3-D
} images related to various science, math, engineering and technology
} areas (from molecules to organs to CAD/architecture) so that they can
} be projected (stereographic projection). Each institution
} participating in the project will have a 3-D theatre built so that
} SMET classes can be brought in for demonstrations of course specific
} images (the theatre will house a Barco 3-D projector driven by a SGI
} UNIX-based workstation and a special screen that retains
} polarization). Students and faculty from the partner institutions
} will also be trained in a residential program at Brookhaven National
} Lab by their 3-D Visualization Team.
}
} Since I have been teaching TEM and SEM courses at NCC for almost 20
} years, I thought that it would be an interesting project to render
} student and my own SEM & TEM images for 3-D projection. I have seen
} many threads on 3-D imaging on this listserver and I would appreciate
} some advice on where to begin. Initially, I am supposed to identify
} some software applications that would be suitable for rendering 3-D
} images of my micrographs. I am aware of some of the applications that
} are used at BNL for their 3-D theatre such as OpenDX, Open GL and
} Visualization ToolKit (VTK).
}
} Can anyone suggest an application (UNIX based ideally) that I might
} get started with? As a novice in this area I realize that the concept
} of 3-D imaging and stereographic projection are probably two entirely
} different principles. I would appreciate any references (articles,
} books, websites) that will help me to understand the concepts.
}
} Thanks for any assistance you can provide!
}
} Steve
} --
} Stephen J. Beck
} Professor
} Bio-Imaging Center/Electron Microscopy
} Department of Biology
} Nassau Community College
} Garden City, NY 11530
} Voice Mail: (516) 572-7829
} Email: {becks-at-sunynassau.edu}
} URL: {http://www.sunynassau.edu/webpages/biology/becks.htm}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 08:17:48 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all-

I've just completed a great semester of teaching EM techniques. The
student projects that were required are quite interesting.
If you have a chance, please review the student's work at this URL:

http://xray.optics.rochester.edu/workgroups/cml/opt307/index.html

Thanks!
Brian

_________________________________________________
Brian McIntyre
Univ. of Rochester
The Institute of Optics
River Campus EMLab
585-275-3058/4875
585-244-4936 (fax)

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 08:36:45 2004

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Hi

Please help me. I'm really in trouble.
Just burned the second filament after 3 hours. Previously, I had about 200 h. Now the current is very unstable.
Before burning, is slowly going down and after that a quick increase up to 170 uA and bang.
We have a Jeol 1010 (1 year old).

Many thanks,
Luci
_________________________________________
Lucian Barbu-Tudoran
Electron Microscopy Center
Faculty of Biology & Geology
Babes-Bolyai University of Cluj-Napoca
5-7 Clinicilor Str., 3400 Cluj-Napoca, Romania
Tel/Fax: +40 264 598700
{http://hasdeu.ubbcluj.ro/emc/lucian_barbu_tudoran.htm} http://hasdeu.ubbcluj.ro/emc/lucian_barbu_tudoran.htm

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 08:43:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mcintyre-at-optics.rochester.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, May 3, 2004 at 08:10:50
---------------------------------------------------------------------------

Email: mcintyre-at-optics.rochester.edu
Name: Brian McIntyre

Organization: Univ.of Rochester

Title-Subject: [Microscopy] [Filtered] Review of Student Projects

Question: Hi all-

I've just concluded a great semester of teaching EM techniques to a mixed group of undergrads and grads. They've put together some interesting projects that are posted on the web here:

http://xray.optics.rochester.edu/workgroups/cml/opt307/index.html

Please take a look and provide feedback to them and me.

Thanks!
Brian

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 09:12:16 2004

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} Dear Listserver,
}
} I have recently processed Hela cells grown on covertslips by
} conventional chemical fixation( 2.5% formaldehyde plus 2.5% glutaraldehyde
} for 2h and postfixation in 1.5% Osmium in 0.1M sodium cacodylate buffer,
} dehydrated in a series of concentrations of ethanol over a period of 90
} minutes and then infiltrated in Epon-aradite). After sectioning, I stained
} the sections with 2% uranyl acetate in distill water for 10 min and lead
} citrate for 5 min. I could hardly visualize the membrane structrue,
} particularly nuclear membrane, plasma membrane, Golgi apparatus and ER
} membranes. However the other structures were well preserved. I am here
} asking for your advice and greatly appreciate any suggestions!
}
} Thank you very much in advance!
}
} Guofeng Zhang, Ph.D
} Division of Bioengineering & Physical Sciences
} National Institute of Health
} Bethesda, MD 20892
} Tel: 301-451-3856
} Email: zhangguo-at-mail.nih.gov
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 12:14:15 2004

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Hello,

I'm trying accquire EDS spectra of various posphors and am having
difficulty. There are peaks that do not seem to match any known elements,
and all of the peaks shift up and down in energy from one spectrum to the
next. I'm wondering if this is a common phenomenon with phosphors, or is my
system out to lunch? All ideas are welcome!

Diane Ciaburri

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 12:33:56 2004

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Guofeng

Having been around for what seems like forever, I really did not write
up some of the old literature as some of our students have suggested.
But there are old reports of just this problem. The conclusion was that
osmication does not adequately stabilize membranes against extraction
during ethanol dehydration. The reference is a bit fuzzy, but I believe
it was Dan Pease’s book ‘Histological Techniques for Electron
Microscopy’, 2nd edition, 1964. It was also never clear whether it was
the ethanol or the propylene oxide intermediate which was responsible
for membrane extraction. We have tested this out and confirmed that,
for whatever reason, in our hands we will see the loss of membranes you
describe if we use the procedures as you list.

There are two solutions. First, post-fixation in uranyl acetate.
Uranyl acetate will stabilize membranes. We wash 1x in buffer and 3x in
filtered water after the osmication step, and then fix in 2% UA. Our
monolayers and free suspensions are usually only fixed for a couple of
hours, but we do leave them in UA for up to several days without noting
any deleterious effect. This step usually improves stabilization of
membranes in our hands.

The second solution is to dehydrate in acetone. There are two reasons,
first is that acetone is not reported to extract membranes, and second,
you do not need an intermediate step such as propylene oxide, but go
directly into graded acetone:plastic for infiltration. This second
reason saves on costs, reduces turnaround, and is a little more
environmentally friendly. In fact, we have found that using acetone is,
by itself, sufficient to ensure good membrane stabilization.

Our normal procedure now is to use both UA en bloc postfixation followed
by acetone dehydration. Our results are usually very good, and we never
lose membranes.

Hope these ideas help.

Paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 13:07:05 2004

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On May 2, 2004, at 11:17 AM, Steve Beck wrote:

} Can anyone suggest an application (UNIX based ideally) that I might
} get started with? As a novice in this area I realize that the concept
} of 3-D imaging and stereographic projection are probably two entirely
} different principles. I would appreciate any references (articles,
} books, websites) that will help me to understand the concepts.
}
Dear Steve,
If you do not get sufficient info from this list, try the 3dem list:

} ADMINISTRIVIA
}
} To post to this list, send mail to
}
} 3dem-at-ucsd.edu
}
} To subscribe to this list, send mail to
}
} majordomo-at-3dem.ucsd.edu
}
} with the text
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} subscribe 3dem
}
} in the body of the message (not in the Subject:).
}
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}
} majordomo-at-3dem.ucsd.edu
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} with the text
}
} unsubscribe 3dem
}
} in the body of the message (not in the Subject:).

I also know that the group at the Wadsworth Center in Albany NY has
prepared stereo images from 3-D reconstructions, so you might want to
contact them.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 13:38:17 2004

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} } I have recently processed Hela cells grown on covertslips by
} } conventional chemical fixation( 2.5% formaldehyde plus 2.5% glutaraldehyde
} } for 2h and postfixation in 1.5% Osmium in 0.1M sodium cacodylate buffer,
} } dehydrated in a series of concentrations of ethanol over a period of 90
} } minutes and then infiltrated in Epon-aradite). After sectioning, I stained
} } the sections with 2% uranyl acetate in distill water for 10 min and lead
} } citrate for 5 min. I could hardly visualize the membrane structrue,
} } particularly nuclear membrane, plasma membrane, Golgi apparatus and ER
} } membranes. However the other structures were well preserved. I am here
} } asking for your advice and greatly appreciate any suggestions!

Try increasing the time in uranyl acetate to 25 or more minutes, and
decrease the time in lead citrate to 3 minutes. Unintuitively, sometimes
longer times in the lead citrate causes bleaching rather than staining!

On the other hand, I've also had success with 10 minutes in each, and with
5 minutes in lead followed by 10 minutes in UA followed by another 10
minutes in lead, and many other variations. Try several approaches and see
what works for you!

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 14:08:00 2004

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Dear Guofeng. I have worked on many cell culture preps. I normally use
microwave processing however for bench processing I would recommend that
you shorten all your processing steps. I would bench fix in glut and
osmium for 20 mins each at room temperature for example. I use 2%
glutaraldehyde on 0.1 M cacodylate buffer. I wash in 0.1M cacodylate
buffer with 0.3M sucrose added. I also add 0.3 M sucrose to the post fix.
The cells are very thin and not like a tissue chunk. Also, dehydration
times should be very short- 1-2 mins is sufficient. in your alcohol changes.
Cultured cells don't have much contrast so try using a reduced osmium fix
(2% osmium tetroxide in 0.1 M cacodylate buffer containing 0.8% potassium
ferricyanide). it gives really nice contrast to membranes and
cytoskeleton. Also try an en bloc UA step before the dehydration.
Your post staining sounds OK.
Good luck
JoAnn Buchanan
Dear Listserver,
}
} I have recently processed Hela cells grown on covertslips by
} conventional chemical fixation( 2.5% formaldehyde plus 2.5% glutaraldehyde
} for 2h and postfixation in 1.5% Osmium in 0.1M sodium cacodylate buffer,
} dehydrated in a series of concentrations of ethanol over a period of 90
} minutes and then infiltrated in Epon-aradite). After sectioning, I stained
} the sections with 2% uranyl acetate in distill water for 10 min and lead
} citrate for 5 min. I could hardly visualize the membrane structrue,
} particularly nuclear membrane, plasma membrane, Golgi apparatus and ER
} membranes. However the other structures were well preserved. I am here
} asking for your advice and greatly appreciate any suggestions!
}
} Thank you very much in advance!
}
} Guofeng Zhang, Ph.D
} Division of Bioengineering & Physical Sciences
} National Institute of Health
} Bethesda, MD 20892
} Tel: 301-451-3856
} Email: zhangguo-at-mail.nih.gov
}

Department of Molecular and Cellular Physiology
Stanford University School of Medicine
Stanford, CA 94305
650-723-5856

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 14:24:13 2004

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On May 3, 2004, at 10:16 AM, Diane.Ciaburri-at-gd-ais.com wrote:

} I'm trying accquire EDS spectra of various posphors and am having
} difficulty. There are peaks that do not seem to match any known
} elements,
} and all of the peaks shift up and down in energy from one spectrum to
} the
} next. I'm wondering if this is a common phenomenon with phosphors, or
} is my
} system out to lunch? All ideas are welcome!
}
Dear Diane,
I assume you're looking at inorganic phosphors, such as CdS, etc., in
which case there should be no problem. Just because it's a phosphor
does not change the interaction with beam electrons that produces
x-rays. There might be contaminants in the mix, but these would be
minor--not ~10%--so there could be some very small peaks, but
everything should match one or more known elements. Have you
calibrated the energy spectrum? The energies should not shift--the
only way that might happen is if the majority of the x-rays were
inelastically scattered. If you take multiple spectra from a single
area (assuming that there is not significant loss of material during
data collection) neither the energies nor the intensities should vary.
I suggest putting in a standard, such as Al evaporated onto a formvar
film on a Cu grid, and taking spectra from locations where both the Al
and Cu signals are strong. The spectra should be consistent, and you
should be able to check the energy calibration and see if the
resolution is OK. To see if the resolution meets spec, put in a grid
with Mn evaporated on formvar and measure the FWHM of the peak.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 15:03:34 2004

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Try changing your fixation protocols. I use the following fixatives
to help with membrane preservation:

"Yellow Fix for EM" (based on Ito, S and Karnovsky J. J Cell. Biol
Abstract 1968)
2.5% glut.
4.0% paraformaldehyde
0.02 % picric acid
in 0.1M sodium cacodylate buffer

(I use 20ml of 0.2M buffer, 10ml of 10% glut, 10 ml of 16% pfa and 2
ml of a saturated sol. of picric acid--I keep a jar of it in my hood,
with the crystals covered with water and draw off as I need it,
adding fresh water when I'm done so that it doesn't explode.)

For a secondary fix I use 1% osmium tetroxide and 1.5% potassium
ferricyanide (aqueous)made up my mixing stock solutions of 2% osmium
and 3% K-ferr 1:1.

Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 15:06:27 2004

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Cool! Well, maybe not for you.

We have an infrared chamber-scope that I have to instruct users to turn off
before they do any EDS. Otherwise, the flood of IR photons overwhelms the
EDS detector and runs it up to 100% dead time. Under less overwhelming
conditions, the photons are still detected and their energy adds on to the
real energy of the x-ray photons and peaks get shifted upscale. Its kind of
fun to watch the effect on our spectrum as we turn the light on and off and
the spectral peaks shift back and forth.

I had never thought about it, but the same effect should be expected when
working with cathodo-luminescent materials. And your phosphors are
definitely luminescent.

I recall that some EDS detectors have their windows coated (with Al, I
think) to avoid just this problem. I don't know if that is something that
can be done very well to an existing detector. I don't suppose you could
interpose another film in front of your detector; it would probably also
absorb your x-rays.

I wonder how others would suggest dealing with this.

Warren

At 12:16 PM 5/3/2004, you wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 15:30:18 2004

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Luci, the Microscopy Today journal, March/April 2003
issue has an article on "The Life and Death of a
Tungsten Hairpin Filament". In it there is described
the different failure modes for a hairpin filament
which may help you.

You should be able to access this article via the
following link:

http://www.microscopy-today.com/TableofContentsPDF.html

Stu Smalinskas, P.E.
Metallurgist
SKF
46815 Port Street
Plymouth, Michigan 48170

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Luci wrote:

Hi

Please help me. I'm really in trouble.
Just burned the second filament after 3 hours.
Previously, I had about 200 h. Now the current is very
unstable.
Before burning, is slowly going down and after that a
quick increase up to 170 uA and bang.
We have a Jeol 1010 (1 year old).

Many thanks,
Luci
_________________________________________
Lucian Barbu-Tudoran
Electron Microscopy Center
Faculty of Biology & Geology
Babes-Bolyai University of Cluj-Napoca
5-7 Clinicilor Str., 3400 Cluj-Napoca, Romania
Tel/Fax: +40 264 598700
{http://hasdeu.ubbcluj.ro/emc/lucian_barbu_tudoran.htm

__________________________________
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From MicroscopyL-request-at-ns.microscopy.com Mon May 3 16:24:54 2004

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We would guess the problem may be in your power supply. Your 200+ hours
indicates a good vacuum and clean system. Our customers average 200+ on
rebuilt filaments and slightly less on new filaments due to the special
process used on rebuilt filaments.

Based on your comments, I'd check with Jeol services.

John Arnott

Disclaimer: Ladd Research is a supplier of a wide variety of microscope
supplies and accessories, including new and rebuilt filaments.

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com

----- Original Message -----
} From: "Lucian Barbu (by way of Ask-A-Microscopist)"
{lbarbu-at-hasdeu.ubbcluj.ro}
To: {microscopy-at-ns.microscopy.com}
Sent: Monday, May 03, 2004 9:40 AM

Bill,

Yes, the system was just calibrated last Friday, and I double-checked it
again today which led me to think there must be something funny happening
with the samples. Here's the answer, thanks to a variety of helpful hints I
received. Apparently my detector is sensitive to visible light and the
whole spectrum was being shifted to higher energies by varying amounts
(depending on how much light I was generating). By switching from my thin
window to my berillium window, and blocking the visible light, things make
sense again.

Thanks, Bill and everyone else that responded. You guys are life savers!

Diane Ciaburri

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Monday, May 03, 2004 3:32 PM
To: microscopy-at-msa.microscopy.com

Dear Diane,
If you are using the modern thin-window EDS detectors sold nowadays, you should
know that they are very susceptible to light and that could easily be the source
of your strange signals. The old-style Be-window detectors were not
light-susceptible, so if you can find one you can test the elements above Ne.
For the elements below that, perhaps using a low accelerating voltage ( {5 kV)
will reduce the light emission from the phosphor enough to get a reading on a
thin-window detector.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {Diane.Ciaburri-at-gd-ais.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Monday, May 03, 2004 10:16 AM

Paul and Guofeng
I never though for staining in UA after osmication as a
"postfixation". It's hardly believe to me that UA has something to do with
"fixation". In my point of view UA stained positively nucleic acids and
don't interfere with membranes. When I need reduce the appearance of the
ribosomes in neurone's cytoplasm, I used to remove UA staining after
osmication step from procedure. In my hands, it absolutely does not affect
membranes (I did both: with and without that step). I used Spurr, not
Epon. I also did not see any effect of ethanol on membranes. I think, if
you are using it for 10-15 min each step, it should not affect membrane's
quality, otherwise nearly whole EM is pure artefact (most people still use
ethanol). The basic reason, not to use acetone for dehydratation is
because acetone is very strong denaturing agent (contrary to ethanol), so
acetone will definitely alternate the fine structure. For this reason,
people use acetone in freeze-substitution procedure at low temperature to
reduce denaturing effect of acetone. Returning back to original question,
I would suggest to check is OsO4 was good or not. If there is any
suspicious there, you need to use fresh solution/chemicals. After
osmication the tissue (even in monolayer) should turn brown. Sergey

At 12:36 PM 5/3/2004 -0500, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon May 3 18:28:33 2004

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Mary & Co.,

I think Diane's issue with phosphorous is visible fluorescence similar to the face of a CRT. After all, to get an image on a TV screen we shoot electrons at phosphorous coated screens and hence it fluoresces in visible light, and likely IR as well. Ideal to make the EDX detector do odd things. Chamberscopes, as Warren indicated, have the same effect.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
Sent: Monday, May 03, 2004 5:53 PM
To: Diane.Ciaburri-at-gd-ais.com
Cc: Microscopy

Dear Diane,
If you are using the modern thin-window EDS detectors sold nowadays, you should
know that they are very susceptible to light and that could easily be the source
of your strange signals. The old-style Be-window detectors were not
light-susceptible, so if you can find one you can test the elements above Ne.
For the elements below that, perhaps using a low accelerating voltage ( {5 kV)
will reduce the light emission from the phosphor enough to get a reading on a
thin-window detector.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {Diane.Ciaburri-at-gd-ais.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Monday, May 03, 2004 10:16 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donaldawbrey-at-hotmail.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, May 3, 2004 at 12:44:21
---------------------------------------------------------------------------

Email: donaldawbrey-at-hotmail.com
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] MListserver: EM scopes

Question: Dear MSA netters,

Our department is in the preliminary stages of aquiring a new electron microscope. The one in use is antiquated. I would like to have as many opinions of different scopes and their ancillary systems.

We are looking for a scope to be used for diagnostic services (such as kidney biopsies, tumors, and etc.).

Our requirements are: 120kv, flat bed camera scanner, subliminal printer, image software, dual digital/manual capabilities.

Thank you in advance for any opinions.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 21:47:58 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ecd10-at-psu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, May 3, 2004 at 14:10:00
---------------------------------------------------------------------------

Email: ecd10-at-psu.edu
Name: Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver:Postdoc opening at Penn State

Question: POST-DOCTORAL POSITION
in
Electron Microscopy of Nanostructured Electronic Materials
at
The Pennsylvania State University

A postdoctoral position is available in the area of nanostructured electronic materials beginning July 1, 2004. The research project focuses on understanding interface structure and chemistry in heterostructured thin films and nanowires. Aspects of the project will be conducted under the auspices of an NSF-NIRT program on semiconducting nanowires. Through a variety of electron imaging and spectroscopy techniques we aim to quantify atomic structure and chemistry of interfaces in heterostructured materials. Most of the research will be conducted on a JEOL 2010F Field Emission TEM/STEM outfitted with an EDAX energy dispersive x-ray spectrometer (EDS), Gatan Enfina electron energy loss spectrometer (EELS), high-angle annular dark field STEM detector, and acquisition hardware and software for spectrum imaging. The ideal candidate for this position will have experience in HRTEM, STEM, EDS and EELS. The salary will be commensurate with qualifications and experience.

Please forward questions or send applications to:

Professor Elizabeth Dickey
Department of Materials Science and Engineering
The Pennsylvania State University
223 Materials Research Building
University Park, PA 16802
USA

tel: (814) 865-9067
FAX: (814) 865-2326
email: ecd10-at-psu.edu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 03:20:46 2004

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Hi all !

does anyone know some manufacturers or distributors of coloďdal silica
also called "syton", for microsectionned dies polishing process ?

thanx in advance...

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 11:03:10 2004

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Dear Sylvain:

South Bay Technology offers 3 types of Colloidal Silica for cross
sectioning of semiconductor materials - as well as other applications.
The products we offer are:

CS1 - Non-crystallizing Colloidal Silica
CS2 - Syton
CS3 - Glanzox

All of these products are available through our local distributor in
France. All of our distrinbutor contact information can be found on our
website. As luck would have it, "Colloidal Silica" is also the featured
product on our website today. You can go to www.southbaytech.com and
find information on the colloidal silica products on the main page.
Alternatively, you can enter "colloidal silica" in the product search
box to bring up all references to our various colloidal silica products.

I hope this helps.

Best regards-

David

sylvain maury wrote:

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--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

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Toll-free in the USA: +1-800-728-2233
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From MicroscopyL-request-at-ns.microscopy.com Tue May 4 12:41:00 2004

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The clinical lab I used to work in had a Codonex
di-sub printer which we rarely used. Overall, our
imaging software (Gatan Micrograph ~2+years old) did
not jive with the printer too well - less resolution
with printed image. Not to say its a bad system. It
might have been because our imaging program needed
updating. Case in point, scanned images that were
'tweeked' in Adobe and printed with the Codonex came
out excellent.
Sara Goldston

by way of MicroscopyListserver
{donaldawbrey-at-hotmail.com} wrote:

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy
Society of America

Below is the result of your feedback form
(NJZFM-ultra-55). It was submitted by
(donaldawbrey-at-hotmail.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html
on Monday, May 3, 2004 at 12:44:21
---------------------------------------------------------------------------

Email: donaldawbrey-at-hotmail.com
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] MListserver: EM
scopes

Question: Dear MSA netters,

Our department is in the preliminary stages of
aquiring a new electron microscope. The one in use is
antiquated. I would like to have as many opinions of
different scopes and their ancillary systems.

We are looking for a scope to be used for diagnostic
services (such as kidney biopsies, tumors, and etc.).

Our requirements are: 120kv, flat bed camera scanner,
subliminal printer, image software, dual
digital/manual capabilities.

Thank you in advance for any opinions.

---------------------------------------------------------------------------

__________________________________
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Win a $20,000 Career Makeover at Yahoo! HotJobs
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From MicroscopyL-request-at-ns.microscopy.com Tue May 4 16:31:39 2004

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Dear Listserver,

Many thanks to all of your helpful comments and suggestions on membrane
visualization problems! I think I will get succeed in solving the problems
in near future after taking your advise.

Kind Regards!

Guofeng
}
} Guofeng Zhang, Ph.D
} Division of Bioengineering & Physical Sciences
} National Institute of Health
} Bethesda, MD 20892
} Tel: 301-451-3856
} Email: zhangguo-at-mail.nih.gov
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 17:14:38 2004

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Listers,
I have a researcher wanting to look at seed surface morphology. These
seeds are from dried herbarium sheets. I initially had him simply treat
the seeds with acetone to remove any waxes from the surface and then
O-T-O-T-O them. This was not adequate as we saw what I believe to be
fungal hyphae and spores plus a LOT of debris. Does anybody have a
"tried and true" (and easy!) method of preparing seeds? I was thinking
about doing acetolysis or 10% KOH, which I do with pollen routinely, but

wasn't sure how the seed surface would hold up. Also, I don't think the
person sonicated in acetone. Might that alone be adequate? TIA.

Bill

--
=============================================================
Bill Chissoe III
Electron Microscopist
University of Oklahoma
770 Van Vleet Oval
Norman, Ok. 73019
E-mail: wchiss-at-ou.edu Ph. (405)325-4391
=============================================================

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 20:01:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (cmeyer911-at-yahoo.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 4, 2004 at 19:31:16
---------------------------------------------------------------------------

Email: cmeyer911-at-yahoo.com
Name: Chris Meyer

Organization: Boeing

Title-Subject: [Microscopy] [Filtered] [TEM EELS Gatan 607]

Question: I have an old Gatan Model 607 EELS system that I have never run (I'm new to TEM). It used to be run by a TN-5500 system, that is soon to be replaced with a new EDS system. I do not want to lose EELS capability for future projects. A Gatan representative informed me the 607 system could be run with a Mac with an old operating system.

I'd like to talk (email) to any current or former 607 EELS users that would have ideas on how I could keep this capability for the future. Is my only option to keep the TN-5500 for this purpose alone? I'd appreciate it. Thanks.

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From MicroscopyL-request-at-ns.microscopy.com Wed May 5 02:58:16 2004

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look on the www.struers.com

best regards

chris

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 07:49:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jacqui.ross-at-auckland.ac.nz) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 4, 2004 at 23:18:40
---------------------------------------------------------------------------

Email: jacqui.ross-at-auckland.ac.nz
Name: Jacqui Ross

Organization: The University of Auckland

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: We are about to buy a new inverted fluorescence microscope, probably a Nikon.

Does anyone have any experience/feedback about the Nikon Digital Sight colour camera (DS-5Mc-U1)? We are intending to buy the new cooled one and I would appreciate hearing from anyone who has used one or seen one demonstrated recently.

Cheers,

Jacqui.

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From MicroscopyL-request-at-ns.microscopy.com Wed May 5 14:48:22 2004

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Listers,

Here is the TABLE OF CONTENTS for the MAY 2004 issue of MICROSCOPY TODAY.

New Subscriptions via http://www.microscopy-today.com only, please.
New subscriptions will close on Tuesday May 11th for this issue.

WE HAVE PURGED NON-MSA MEMBER, NON-NORTH AMERICAN, UNSUBSCRIBED INDIVIDUALS!
SEVERAL HUNDRED NON-QUALIFIED SUBSCRIBERS HAVE BEEN PURGED.

Scanning Wet Specimens
.Stephen W. Carmichael and Wilma L. Lingle, Mayo Clinic

Laboratory Design for High-Performance Electron Microscopy
.M.A. O'Keefe, et al., LBNL; C.J.D. Heatherington, et al., Oxford; B.
.Carragher, et al., Scripps; L.F. Allard, et al., ORNL

New CMEIAS Image Analysis Software for Computer-Assisted Microscopy of
Microorganisms and Their Ecology
.Frank B. Dazzo, Michigan State University

Making Slide Shows in Acrobat
.Jerry Sedgewick, University of Minnesota

Sub-Angstrom Resolution with a Mid-Voltage TEM
.M.A. O'Keefe, C.J.D. Hetherington, E. C. Nelson, LBNL, Berkeley

Viability and Versatility of the Yeast Cell
.Michelle J. Henry-Stanley & Carol L. Wells, Univ. of Minnesota

New Adhesion Mechanism in Giardia: Role of the Ventrolateral Flange in the
Attachment of Trophozoites to Rough and Porous Surfaces
.S.L. Erlandsen, U. Minnesota; A.P. Russo, & J.N. Turner, New York
.Wadsworth Center

Project VISUAL: Facilitating the Connection Between Art and Science
.L.M. Strzegowski & T.P. Russell, U. of Massachusetts, Amherst

Use and Disposal of Uranyl Acetate in the Electron Microscope Laboratory:
Glow in the Dark or Walk in the Park?
.Randy Tindall, University of Missouri

Confocal Microscopy for Diagnostic Cytology
.M.E. Boon, & L.P. Kok, U. Groningen, The Netherlands

Technical Note on the Preparation of Un-decalcified Trabecular Bone for
Examination by TEM
.Jeannette Taylor, Emory Univ. & Iwona Jasiuk, Georgia Inst. of Technology

The Low Voltage SEM Imaging Advantage: A Reminder
.Steven S. Hurban. Endicott Interconnect Technologies, Inc. NY

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:53:09 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (fremingt-at-fhcrc.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 5, 2004 at 11:24:55
---------------------------------------------------------------------------

Email: fremingt-at-fhcrc.org
Name: Franque Remington

Organization: Fred Hutchinson Cancer Research Center

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Many Thanks to all who offered suggestions and techniques for preserving conidia for SEM. They have been very helpful.

Franque Remington

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From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:53:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwareham-at-utah.gov) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 5, 2004 at 15:08:22
---------------------------------------------------------------------------

Email: bwareham-at-utah.gov
Name: Beverly Wareham

Organization: Utah Veterinary Diagnostic Lab

Title-Subject: [Microscopy] [Filtered] Fixation of animal lung tissue

Question: Hi all,
Does anyone have a protocol for fixing animal lung tissue (sheep) for EM and is willing to share it? I'd really appreciate it.

Thanks,
Beverly Wareham
Utah Veterinary Diagnostic Laboratory
435-797-1799
bwareham-at-utah.gov

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From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:54:19 2004

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Dear listers,

Sometimes you just gotta share the good news. After trying out my share
of handheld vacuum cleaners for small lab cleanup jobs and finding them
all to be pretty asthmatic, I finally hit paydirt. I found something
called the Euro Pro 700 watt hand vac down at the local Office Depot for
about $30, complete with small hose, attachments and shoulder strap.
Not only does it clean up the plastic fluff that builds up in
ultramicrotomy areas, it would probably suck up the whole microtome if
you turned your back. That's probably why it's also called "The Shark".

No financial interest, just a (finally) happy owner of a tiny vacuum
cleaner that works!

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:54:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ananthpb-at-rediffmail.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 5, 2004 at 16:07:20
---------------------------------------------------------------------------

Email: ananthpb-at-rediffmail.com
Name: Ananth Puthucode

Organization: Univ. North Texas

Title-Subject: [Microscopy] [Filtered] electropolisher

Question: Hi all,

I am looking for a used electropolisher for TEM sample preparation. Please let me know if anyone has got one and planning to sell it.

Thanks,
Ananth

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From MicroscopyL-request-at-ns.microscopy.com Thu May 6 03:53:57 2004

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hello microscopists !

I have a question for those who work in Failure Analysis of
semiconductors but anyone can answer...

I'm trying to define a methodology to use colloidal silica for polishing
process of microsectionned dies (Si, AsGA), for SEM observations. I'd
like to know the conditions that people commonly use for their sample
preparations with Syton.
Any suggestions are welcome...
Thanx in advance!

and thanx to David Henricks : i just received the documents about
colloidal silica and SEM sample preparation. But the paper about iridium
sputtering was not in the package. You must have forgotten it, but it
doesn't matter. thanx again...

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 07:28:23 2004

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-----

} hi !
}
} ask the company name "logitech" (a division from struers denmark)
} they are have a special equipment for polishing semiconductors !
} email info-at-logitech-us.com or www.logitech.uk.com
}
} best regards
}
} chris huebner
}
} Foundry Research Insitute, Kraków - Poland
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 08:38:24 2004

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Randy

I don't know if anyone else would wish to confirm my fears but I am concerned about the use of any basic vacuum cleaner for clearing up resin dust.

The problem as I see it is:
1. Vacuum cleaners do pump out small particles from their exhaust (unless they have some very fine submicron exhaust filter).
2. It's the fine stuff (below 2 or 3 microns) that remains airborne and worse still is the ideal size for inhalation. It is much more likely to penetrate deeper into the respiratory tract (hence the problem with certain sizes of dust such as asbestos).
3. Resins used for most biological purposes are not completely polymerised at 60 to 80 degrees. They are usually regarded as safe enough to handle but could well be hazardous if inhaled and retained in the lungs for long enough.

If you combine the above facts with, for instance, sawing or grinding resins (particularly epoxies like Spurr's) then you might actually be increasing your exposure to the most hazardous component of the resin dust. Generally I try to avoid sawing and only ever trim blocks with razor blades or glass knives because the pieces are big and even if you could inhale some I doubt they'd ever reach your lungs.

Some of this is assimilated information from years ago, so I can't give you a particular source or reference. I suspect that you could easily check if there is a problem by putting a 'sticky' stub near to the exhaust of your vacuum cleaner and see if it picks up much. I've never tried it because I just simply avoid fine dust now.

Malcolm

Malcolm Haswell
e.m. unit
University of Sunderland
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: "Tindall, Randy D." {TindallR-at-missouri.edu}

The International Metallographic Society is seeking a volunteer to serve as
the Local Chair for the 2005 International Metallographic Contest which will
be held in conjunction with the 38th Annual Convention of the IMS and the
Microscopy and Microanalysis 2005 meeting in Honolulu, Hawaii in July of
2005. Interested individuals from the Honolulu area should contact the
Contest Chair, Jeff Stewart, at jeff-at-metallography.com for additional
information. We would like to have the position filled within the next few
weeks.

Thanks,

Jeff Stewart
International Metallographic Contest Chair
Metallographic Laboratory Manager
Stern-Leach Co.
49 Pearl Street
Attleboro, MA 02703 USA
Phone: 508-222-7400 extension 1329
Fax: 508-699-4030
E-mail: jeff-at-metallography.com

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 08:43:47 2004

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Good points, Malcolm. I forgot to mention that this thing comes with a
HEPA filter. Anyway, most of our resin fluff comes from block trimming
with razor blades and glass knives.

Randy

-----Original Message-----
} From: Malcolm Haswell [mailto:malcolm.haswell-at-sunderland.ac.uk]
Sent: Thursday, May 06, 2004 8:42 AM
To: MSA microscopy listserver
Cc: Tindall, Randy D.

Micromavens,

I'm hoping to find someone with a Gatan model 626
cryostage/cryoholder who wishes to sell it or donate it to a
university. Cryostation is not necessary, we've got that. Anyone out
there?
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 10:12:47 2004

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One of faculty here will be processing lengths of rat femoral artery
for light microscopy and needs to keep track of the distal vs
proximal ends. She tried marking one end with India Ink, but it was
washed out sometime during the dehydration/xylene steps.
Any ideas?
Thanks,
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 10:49:32 2004

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Hi Beverly,

I was on a TEM project many years ago working with sheep and chicken
lungs. Jeff Weidner was the PI on the project. The problem in the
we had was to get the air out of the lungs before we could any of the
specimen prep procedures to work well. To many air bubbles and poor
infiltration.

We ended up use a standard EM procedure with each step done under low vacuum.

Mike

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
===================================================================================
Michael Dunlap
office (530) 752-0284
University of California lab (530) 752-5489
Chemical Engineering & Material Science Fax (530) 752-9554
110A Kemper Hall mrdunlap-at-ucdavis.edu
One Shields Ave.
http://www.chms.ucdavis.edu/
Davis CA, 95616
===================================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 11:43:58 2004

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On May 6, 2004, at 9:09 AM, Leona Cohen-Gould wrote:

} One of faculty here will be processing lengths of rat femoral artery
} for light microscopy and needs to keep track of the distal vs proximal
} ends. She tried marking one end with India Ink, but it was washed out
} sometime during the dehydration/xylene steps.
} Any ideas?
}
Dear Lee,
Could one end be cut straight across and the other cut at an angle? I
don't know how readily this could be done or whether it would be easy
to distinguish the ends, but if one cannot determine the shape of the
end, I'd wonder whether other morphology would be reliable.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 13:36:27 2004

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Hi Beverly,
We have the same experience as Mike with both lung, brain (and a few
others) and most plant tissues. Before microwaving, we used the
standard protocols (G, followed by Os, etc.) and did all steps in a low
vacuum. You can use an evaporator using only the rough pump (Good idea
to protect where the vials are set so resin doesn't get on evaporator
plate_, if you don't have another vac chamber such as a vacuum oven.
Now that we microwave most of our tissues, we use the cold plate and
vacuum chamber for hard to penetrate tissues on all steps. It is likely
that the alcohols don't need to be done in the MW however it is faster.

NOTE about pulling the vacuum. One needs to WATCH when pumping the
samples. We pump on the samples and wait for the bubbles to rise. Just
before they get too close to the top, we turn off the vacuum, let the
bubbles settle a bit and start again. Eventually no bubbles appear.
This of course is likely more crucial in the resin steps since resin all
over everything is not nice! After the bubbles have subsided and don't
appear in quantity, we let the vial sit in the vacuum chamber under
vacuum but with the pump off, for the desired time of the step.

When using a microwave with a vacuum chamber it is important to note
WHERE the gauge actually is since if it is directly off the pump, then
when it pulls down to 20mmHg that is only at the pump port, not the
chamber, so that must be taken into consideration. We usually use that
approximate vacuum for the vac chamber on the microwave for most
fixations that are done in the microwave. It is hoped, sincerely hoped,
that eventually the manufacturers will build in a vacuum chamber with a
cold plate in the microwave so it isn't quite so messy to set up.

Good luck,
Judy Murphy

Michael Dunlap wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi Beverly,
}
} I was on a TEM project many years ago working with sheep and chicken
} lungs. Jeff Weidner was the PI on the project. The problem in the
} we had was to get the air out of the lungs before we could any of the
} specimen prep procedures to work well. To many air bubbles and poor
} infiltration.
}
} We ended up use a standard EM procedure with each step done under low vacuum.
}
} Mike
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } Below is the result of your feedback form (NJZFM-ultra-55). It was
} } submitted by (bwareham-at-utah.gov) from
} } http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html
} } on Wednesday, May 5, 2004 at 15:08:22
} } ---------------------------------------------------------------------------
} }
} } Email: bwareham-at-utah.gov
} } Name: Beverly Wareham
} }
} } Organization: Utah Veterinary Diagnostic Lab
} }
} } Title-Subject: [Microscopy] [Filtered] Fixation of animal lung tissue
} }
} } Question: Hi all,
} } Does anyone have a protocol for fixing animal lung tissue (sheep)
} } for EM and is willing to share it? I'd really appreciate it.
} }
} } Thanks,
} } Beverly Wareham
} } Utah Veterinary Diagnostic Laboratory
} } 435-797-1799
} } bwareham-at-utah.gov
} }
} } ---------------------------------------------------------------------------
}
} --
} ===================================================================================
} Michael Dunlap
} office (530) 752-0284
} University of California lab (530) 752-5489
} Chemical Engineering & Material Science Fax (530) 752-9554
} 110A Kemper Hall mrdunlap-at-ucdavis.edu
} One Shields Ave.
} http://www.chms.ucdavis.edu/
} Davis CA, 95616
} ===================================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 14:26:10 2004

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Hi Leona:

When you use India Ink it needs to be fixed to the tissue's surface you are
labeling with a picric acid solution such as Bouin's fixative.

Make the ink mark with the opposite end of a swab and then switch to the
cotton tipped end of the swab. Dipp into the Bouin's and dab the area
marked with the India Ink. Blot slightly dry with a Kim Wipe and put back
into formalin. It will be permanently fixed in place and can be processed
and embedded in paraffin.

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 14:53:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (sbs38-at-email.byu.edu) from
http://www.msa.microscopy.org/Ask-A-Microscopist.html on Thursday,
May 6, 2004 at 10:14:58
---------------------------------------------------------------------------

Email: sbs38-at-email.byu.edu
Name: Briant Stringham

Organization: BYU

Education: Undergraduate College

Location: Provo, Utah, US

Question: I am collecting protocols for viewing HSV-1 through
negative staining, and I was hoping you could send what you feel is
the best protocol for viewing membrane and capsid integrity. Next, I
need to know the best stain and method for viewing empty or full
capsids.
Thank you for your reply

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From MicroscopyL-request-at-ns.microscopy.com Thu May 6 16:08:42 2004

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Hello MSA folks;

We here at the University of New Brunswick have a Jeol JXA-733
Superprobe that has served us faithfully for many years. Sadly we have
had a catastrophic failure of the oil-cooled objective lens/pole piece
assembly, and so require a replacement. If you have working one and
would be willing to part with it, please contact us.

Thanks for your time,

Steven Cogswell, P.Eng.
UNB Microscopy and Microanalysis Facility
Fredericton, New Brunswick Canada
Phone (506) 453-4887

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 18:32:09 2004

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You could try OsO4. Its guaranteed to darken on the
specimen and it won't wash out. The only concern is
how useful that end will be once its been treated with
Osmium. I know Osmium is used to fix fatty specimens
in order to give them more contrast. I would use a 1%
or maybe a 2% solution. It usually takes effect
within a few minutes, so you could maybe dip the
distal or promixal portion in the solution. Good
luck.
Sara Goldston
"Bentley, Karen" {Karen_Jensen-at-URMC.Rochester.edu}
wrote:

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Society of America

Hi Leona:

When you use India Ink it needs to be fixed to the
tissue's surface you are
labeling with a picric acid solution such as Bouin's
fixative.

Make the ink mark with the opposite end of a swab and
then switch to the
cotton tipped end of the swab. Dipp into the Bouin's
and dab the area
marked with the India Ink. Blot slightly dry with a
Kim Wipe and put back
into formalin. It will be permanently fixed in place
and can be processed
and embedded in paraffin.

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

__________________________________
Do you Yahoo!?
Win a $20,000 Career Makeover at Yahoo! HotJobs
http://hotjobs.sweepstakes.yahoo.com/careermakeover

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 21:04:00 2004

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Hi Listers
I am looking for contact information for American Laser. Are they
still out there? How can I contact them?
Thanx
David

____________________

David Elliott Ph.D.

Yale University School of Medicine
Campus Address: TAC S160
333 Cedar Street
PO Box 208022
New Haven, CT 06520-8022

Tel: (203) 785-7572
Fax: (203) 785-6815

From MicroscopyL-request-at-ns.microscopy.com Fri May 7 13:26:32 2004

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Dear listers

I recently received the parts to a Zeiss Axiotron microscope, which
is no longer supported by the manufacturer. Does anyone have a
manual or schematics for this unit--I hate to waste the box of very
high quality lenses that came with it, and our engineering department
is very interested in getting the unit assembled and working.

Anyone that can help me out with this, please contact me.

thanks in advance

Steve Barlow
--
Dr. Steven Barlow
EM Facility/Biology Dept.
San Diego State University
5500 Campanile Drive
San Diego CA 92182-4614
phone: (619) 594-4523
fax: (619) 594-5676
email: sbarlow-at-sunstroke.sdsu.edu
http://www.sci.sdsu.edu/emfacility

Chairman, Educational Outreach subcommittee
promoting microscopy instruction and increased access to microscopes
Microscopy Society of America
http://www.msa.microscopy.com/

From MicroscopyL-request-at-ns.microscopy.com Fri May 7 14:34:41 2004

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I'm hoping the microscopy community can help me. I had planned on taking a
course on imaging analysis and photomicrography at McCrone Research but it
was canceled (I was the only student.)

I have a real need to improve my imaging and image measurement skill. I
wish to do particle sizing on images captured via the SEM/TEM/light
microscope.

Does anyone know of short courses and such for the tyro? I would like take
one as soon as possible.

Thanks in advance!!!

Frank Karl
330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Fri May 7 18:15:57 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (e.gagnepain-at-wanadoo.fr) from
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7, 2004 at 10:04:31
---------------------------------------------------------------------------

Email: e.gagnepain-at-wanadoo.fr
Name: Gagnepain

Organization: ULP of Strasbourg

Education: Graduate College

Location: Strasbourg, France

Question: I have some samples of iron-aluminide (FeAL)and the
thickness is 2 millimeter. How to prepare thin layer of FeAl for an
observation with TEM (Transmission Electron Microscope) without
introduce defaults?

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Email: cryanez-at-criba.edu.ar
Name: Julia YaŇez

Organization: CONICET

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I need to stain a polymer sample with
RuO4, by oxidation of RuCl3 with
sodium hypochlorite.
I donĄt know the appropiate reactives concentrations.
Could you help me about this procedure?.
Thanks in advance

Julia Y·Ňez

Ing. MarĚa Julia Y·Ňez TE: 54-291-486-1666 int.: 362
Lab.Microscopia ElectrŰnica FAX: 54-291-486-1527
CRIBABB e-mail: cryanez-at-criba.edu.ar
Camino La Carrindanga Km 7
(8000) BahĚa Blanca

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I have never prepared specimens from this material, so I'm not
familiar with its properties.

Is it electrically conductive?

If so, to begin with I would spark errode with a trepanning tool to
get 3 mm dia. discs. Then mechanically grind and polish, preferably
with a dimple grinder, to ~100 um. Finally, electropolish, preferably
with a jet polisher.

Hirsch, Howie, Nicholson, Pashley and Whelan suggest, for Fe-Al
alloys acetic acid (133 cm3), water (7 cm3), chromic acid (25 g) with
a stainless steel cathode and rinses in acetic acid/methanol. Make
sure it remains cool ( {30 C). Voltage in the 25 V to 30 V range.

Possible problems:

1. Different phases may thin at different rates during
electropolishing - you'll need to change the polishing solution.

2. If it is very soft, the mechanical grinding and polishing may
create a deep damage layer - stop mechanical polishing sooner and use
electropolish earlier.

3. If there is stress in the material, thinning may cause a release
of stress and damage.

4. Safety officers

If you can't get electropolishing to work, ion milling should.
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail
will automatically be deleted.
:-)
PS - I'm an employee of JEOL UK.

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This humble amateur histologist always used "alcoholic Bouin"
("Duboscq-Brazil Fluid") combined with gentle vacuum applied the way
Judy Murphy describes it, to fix small pieces of rabbit lung...

Try google with "alcoholic bouin" as the search string.

"alcoholic Bouin" (aka:"Duboscq-Brazil Fluid")

Stock Alcoholic Bouin's Solution:
80% ETOH 750.0 ml
formaldehyde 300.0 ml
Picric acid 5.0 gm

Mix solution well, stable 1 year.

Working Solution:
Stock solution 70.0 ml 14.0 ml
Acetic acid 5.0 ml 1.0ml
Add the acetic acid right before use.

Y.

-----Original Message-----
} From: Judy Murphy [mailto:jmurphy-at-deltacollege.org]
Sent: donderdag 6 mei 2004 20:22
To: Michael Dunlap
Cc: Microscopy-at-msa.microscopy.com; bwareham-at-utah.gov

briant

the question really is what is the source of specimen? are you looking
for clinical isolates or at culture material. if culture material, has
it been purified in any way. these things may all affect the
preparation and ultimate quality.

the first issue you have to address is grids. you will need grids with
some form of plastic film, be it collodion, formvar or parlodian. if
you are not set up to make grids, they can be obtained from most EM
supply houses. for short term situations, if you are not going to need
a lot of grids and have no one trained in their preparation, buying them
will be best for your use. you may also wish to carbon coat the grids
to stabilize the film. again, carbon coated plastic coated grids may be
purchased. if cost is a problem, i could probably manage to liberate
50-100 grids.

carbon coated grids introduce several problems, mainly due to the fact
that they are quite hydrophobic. however, they do become more
hydrophilic over time. also, you can treat the grids by glow discharge
(within 2-3 weeks of use) or treat them with alcian blue. usually
clinical material has so much serum or fecal protein present that if you
leave the sample on the grid for several minutes you overcome all
problems of hydrophobicity. we view 2500-3000 clinical samples, and
over 4000 total negative stain preparations/ year. at the risk of being
labeled a reprobate and cretin, we usually do not carbon stabilize the
grids used to examine most samples. the added stability is not enough
benefit for clinical material. if it is a sample of importance we may
use carbon coated grids. if so, we use alcian blue, or old grids.
either way, with our concentration methods, hydrophobicity is not a
problem.

you may wish to consider pretreatment of the sample to stabilize the
virion. we either add glutaraldehyde to a concentration of 0.1%, or
formaldehyde to a concentration of 1-2%. this allows us to neutralize
infectivity, maintain antigenicity and reactivity for IEM, and
stabilizes structure against stresses which may arise during
preparation. the samples need to be vortexed very well immediately to
limit clumping which may be associated with fixative mediated
crosslinking of virions. because of the shorter chain size and mono
aldehyde nature, some argue that formaldehyde is less likely to result
in crosslinking, and is better than glutaraldehyde. personally, we have
never seen any difference between the two.

you do not mention mounting the sample on the grid. i assume you have
some method of preference. if not, please ask, we all have our
favourite methods and are more than willing to tell you them.

as far as staining, most viral electron microscopists have their own
preferences. that does not make any one method 'best', however. we use
several stains routinely, and do a panel 14 different negative stains
whenever we start a new project to confirm the best set of conditions.
that said, the two major staining methods use tungsten or uranyl salts.

the most common tungsten salt is 1.5 to 2% phosphotungstic acid (PTA).
to eqalize the different methods, i have adjusted the concentrations of
stains in my labs to maintain an equal amount of heavy metal atoms
available in the staining solution. therefore, we use 2.5mM PTA. this
works out to be approximately 1.6%. the pH is adjusted to 7.0. the
best method for adjusting pH with this stain is with NaOH. early
studies by Horne and his associates implicated the loss of membrane
integrity with pH adjustment by KOH. if you were working with paramyxo
or myxo, and wanted to release the nucleocapsid, this would be a good
method. for the greater part you do not wish to disrupt the membranes.
with most herpes preparations, you will already see a lot of naked
complete and empty nucleocapsids as it is. we also add 25 micrograms/ml
bacitracin as a surfactant. this helps with stain spreadability and
penetration. other small molecules are available for use. the most
common is probably BSA. again, the addition of fixative will also
stabilize the virions against loss of membranes due to stain
characteristics.

we use two different versions of uranyl stains, uranyl acetate(UA) and
uranyl sulfate (US). both of these must be used at low pH. in fact, if
you try to adjust the pH to around 4.0 you start to get problems keeping
material in solution - especially if your pH meter is not as accurate as
you think. as a rule, we use the material at pH of about 3.5. again,
most protocols call for 2% solutions. adjusting to molar concentrations
and maintaining equivalent heavy metal atoms, we use a 60mM solution.
this represents a 2.5% UA or 2.2% US stain. if you must work with
higher pH, it has been suggested that 1% UA can be adjusted to pH values
as high as 7.0 by the addition of 0.1% ammonium acetate and 0.5% EDTA
(disodium salt). i have not tried this, so i do not know how well it
works. rumour is that it is quite grainy and sublimates badly.

each stain system has its own properties. many feel particles degrade
in PTA but not in UA. PTA has a higher anhydrous density, so you see
more contrast, which could be bad or good. UA tends to be more granular
when imaging, while PTA is low granularity. here the issue is purely
what you think would 'look best'. UA/US tends to sublimate in the beam,
leading to a perceived column contamination problem, while PTA is very
stable, leading some to argue that the column is less contaminated by
vaporizing stain.

the best suggestion - try both PTA and a uranyl stain. i would also
refer you to a recent review: Hazelton, P.R. and Gelderblom, H.R. (2003)
The use of the electron microscope for rapid diagnosis of viral agents
in emergent situations. Emerging Infectious Diseases 9:294-303. it will
give some additional methods and general information. yes, i'm human,
it is one of my articles, but i think it's good, anyway.

hope these thoughts help. let me know if you want specific protocols.
we have them all in electronic file format, albeit WordPerfect files, so
they can be sent easily.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

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---------------------------------------------------------------------------

Email: hunny_pot-at-optusnet.com.au
Name: Linda

Organization: The University of Sydney

Education: Undergraduate College

Location: Australia

Question: Hello:

I am doing research paper on quanification of shrinkage due to fixation. There are some questions that I like answers to:

1. what are some of the methods used to measure shrinkage?

2. how the effects of foxation can be differentiated from other possible sources of shrinkage?

3. the practices and clincal signifance of quantifying shrinkage due to fixation.

I have been looking around, but I can't find my answers. Could you please help me? Thanks

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Hi

We are looking for a second hand Gatan 666 PEELS, to fit on VG HB5 STEM.
Perheps are there somme which are sleeping in cupboards ! It doesn't
matter if modifications are necessary. Preferently, for administrative
raions, we would prefer a europeen source, but all propositions are
welcome.

Answer directly to my collegue, at
Daniel.Spor-at-ipcms.u-strasbg.fr

Many Thanks.

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 08:04:46 2004

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Hi

What type of silver charged epoxy will be used to make embedding of powder
as standards for EDS microanalysis. If one looks at Epotek's catalog,
there are so much type of epoxys, with very different properties, shelf
live and price. So what is the best compromise. If someone has an advice.

Many thanks

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 08:53:24 2004

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Hi Linda:

A great deal of research was done on these questions in the late
1940's-1960's and you won't find it on the internet. For starters, get a
hold of "Principles of Biological Microtechnique" by John R. Baker,
published in 1958. He discusses various fixatives, their penetration
rates, how they do or do not promote shrinkage (in the fix or in
subsequent processing), etc. I will try to dig up some references to
specific papers later today.

Geoff

by way of Ask-A-Microscopist wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 09:43:36 2004

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"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Julia,

Prepare only the amount of stain that you will use at that moment. For 1
ml of RuO4 stain, use 0.02 g RuCl(subscript: 3 )(superscript: .) nH
(subscript: 2)O [14898-67-0] and 1 ml of NaOCl [7681-52-9].

I recommend that you purchase fresh hypochlorite every few months since the
concentration of hypochlorite in solution does diminish with time. I
discourage using bleach for the same reason, i.e. one is never sure how
long the bottle of bleach has been on the shelf. Keep the RuCl(subscript:
3) hydrate in a nitrogen desiccator when not in use.

The original reference on the use of the in-situ preparation of RuO4 is:
-- Montezinos, D., Well, B.G. and Burns, J.L., J. Polymer Sci.: Polym.
Lett. Ed., 1985, 23, 421.

Another important reference pertains to vapor-staining with RuO4 (using
RuO4 crystals, which are very difficult to find):
-- Sano, H., Usame, T. and Nakagawa, H., Polymer, 1986 27, 1497.

I hybridized the methods of Sano and Montezinos, i.e. using vapor staining
above the in-situ preparation of RuO4, and invariably get outstanding
results:
-- Brown, G. M. and Butler, J. H., Polymer, 1997, 38 (15), 3937.

Although the Montezinos and Sano papers are key, their practicality is
limited. Montezinos recommends staining in the solution using precursors
that are dirt cheap and readily available. Sano convinced me, however,
that solution staining is not a good practice because it produces severe
and uncontrolled oxidation of the outer surface of the sample. Sano's
vapor-staining method is beautiful but the solid RuO4 crystals he uses are
virtually impossible to find in the United States and are very expensive.
I simply combined the two methods and worked out staining durations. Refer
to the appendix of my paper for details including safe use, handling and
disposal as well as sample preparation from beginning to end and staining
durations for some polymer systems.

Happy staining,

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

cryanez-at-criba.edu.ar
(by way of To: microscopy-at-ns.microscopy.com
MicroscopyListserver) cc:
Subject: [Microscopy] viaWWW: stain a polymer

05/07/04 06:38 PM

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Email: cryanez-at-criba.edu.ar
Name: Julia YaŇez

Organization: CONICET

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I need to stain a polymer sample with
RuO4, by oxidation of RuCl3 with
sodium hypochlorite.
I donĄt know the appropiate reactives concentrations.
Could you help me about this procedure?.
Thanks in advance

Julia Y·Ňez

Ing. MarĚa Julia Y·Ňez TE: 54-291-486-1666 int.: 362
Lab.Microscopia ElectrŰnica FAX: 54-291-486-1527
CRIBABB e-mail: cryanez-at-criba.edu.ar
Camino La Carrindanga Km 7
(8000) BahĚa Blanca

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From MicroscopyL-request-at-ns.microscopy.com Mon May 10 09:45:04 2004

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You may be interested in a paper I published a few years ago in which
I measured the size distribution of cells in suspension after
different fixation conditions. Develop. Biol 23:36-61 (1970)

Joel

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} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (hunny_pot-at-optusnet.com.au) from
} http://www.msa.microscopy.com/Ask-A-Microscopist.html on Sunday, May
} 9, 2004 at 21:45:15
} ----------------------------------------------------------------------
} -----
}
} Email: hunny_pot-at-optusnet.com.au
} Name: Linda
}
} Organization: The University of Sydney
}
} Education: Undergraduate College
}
} Location: Australia
}
} Question: Hello:
}
} I am doing research paper on quanification of shrinkage due to
} fixation. There are some questions that I like answers to:
}
} 1. what are some of the methods used to measure shrinkage?
}
} 2. how the effects of foxation can be differentiated from other
} possible sources of shrinkage?
}
} 3. the practices and clincal signifance of quantifying shrinkage due
} to fixation.
}
} I have been looking around, but I can't find my answers. Could you
} please help me? Thanks
}
} ----------------------------------------------------------------------
} -----
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

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Jacques;

What is the material of interest? You need to say. Obviously it can't be silver but you may want to check to see if you have silver spectrally overlapping the material or element of interest. Is your concern primarily sample charging therefore you want a conductive epoxy?

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: Faerber Jacques [mailto:Jacques.Faerber-at-ipcms.u-strasbg.fr]
Sent: Monday, May 10, 2004 9:09 AM
To: Microscopy Society of America

Hi

What type of silver charged epoxy will be used to make embedding of powder
as standards for EDS microanalysis. If one looks at Epotek's catalog,
there are so much type of epoxys, with very different properties, shelf
live and price. So what is the best compromise. If someone has an advice.

Many thanks

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:06:37 2004

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"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Jacques,

I spent a considerable amount of time working on conductive embedding
media. See my abstract in the 2004 M&M Proceedings.

The problem with virtually all commercial electrically conductive embedding
media that I have seen is that they offer only macroscopic conductivity.
This means that expanses of unfilled, non-conducting and highly charging
epoxy will be found throughout the sample. We need microscopic
conductivity in which the embedding medium is highly conductive and does
not contain non-conductive domains of epoxy. For expoxy-embedding
applications, I recommend compounding (mixing) carbon black filler into the
resin of choice (without catalyst or accelerator) in a mortar and pestle.
Use equal parts by weight of the filler powder and epoxy. At the last
minute before embedding, mix the accelerator into the resin / carbon black
compound as quickly and thoroughly as possible. Embed the sample in this
thick paste.

If well mixed, the embedding medium will not charge at all. Also, since
only carbon and oxygen are present in any appreciable concentration, you
will not have problems with interference lines from metal filler particles,
i.e. silver, etc.

Have fun.

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

Faerber Jacques
{Jacques.Faerber-at-ipcms.u- To: Microscopy Society of America {Microscopy-at-MSA.Microscopy.Com}
strasbg.fr} cc:
Subject: [Microscopy] EDS standards embedding

05/10/04 08:08 AM

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Hi

What type of silver charged epoxy will be used to make embedding of powder
as standards for EDS microanalysis. If one looks at Epotek's catalog,
there are so much type of epoxys, with very different properties, shelf
live and price. So what is the best compromise. If someone has an advice.

Many thanks

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:12:59 2004

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Our standards from Tsousimis came prepared with regular epoxy and a coating
of carbon. We have used the same procedure for our homemade standards. Many
of the standard materials are not conductive anyway, so the conductivity
has to come from a coating. Of course a "conductive" epoxy should not hurt.

I presume you will be not be collecting spectra in variable pressure mode.
The scattering of the beam from the residual atmosphere would produce a
signal from the silver or nickel in your epoxy and would complicate things.

I also advise you to prepare the sample and standards the same. I thought I
was competent at EDS standards and realized fairly recently the difference
that can be caused by different thickness of C coatings (or lack thereof)
between standards and unknowns.

Warren Straszheim

At 08:08 AM 5/10/2004, you wrote:

} Hi
}
} What type of silver charged epoxy will be used to make embedding of powder
} as standards for EDS microanalysis. If one looks at Epotek's catalog,
} there are so much type of epoxys, with very different properties, shelf
} live and price. So what is the best compromise. If someone has an advice.
}
} Many thanks
}
} J. Faerber
} IPCMS-GSI
} (Institut de Physique et Chimie des Matériaux de Strasbourg
} Groupe Surface et Interfaces)
} 23, rue de Loess ; BP43
} 67034 Strasbourg CEDEX 2
} France
}
} Tel 00 33(0)3 88 10 71 01
} Fax 00 33(0)3 88 10 72 48
} E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

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I want to find a simple TEM protocol for negative staining of microsomal
preparations. Does anyone have suggestions?

Thank you,
Cheri Owen
Cheri Owen, PhD
Dept. Emergency Medicine
Wayne State University
Detroit, Mi 48201

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Ooh, one more question:

The Philips EM400 installations I know of all utilized a Haskris
chiller. We're looking to buy a new chiller and they are considerably
cheaper from Neslab. Would anyone recommend against going with Neslab
for any reason?

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:56:54 2004

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Hi folks,

Does anyone know of an archived discussion or a web site anywhere that
describes adapting a C-mount for a digital camera to the old Philips
EM400 TEM? Perhaps by custom machining a cover blank for the 35mm
camera mounting location?

We recently purchased a Pax-it 2.1 Mpixel digital camera to use with a
new inverted metallurgical LM, but after receiving the camera, funding
for the microscope didn't materialize, so we're thinking of using the
Pax-it on our EM400.

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 13:52:13 2004

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Eric -

The only thing I don't particularly care for in our (?8-year-old)
Neslab chiller is the fact that the water reservoir is pretty well sealed
up, like a miniature 45-gallon drum on its side, so you can't see what's
going on in there. The Haskris chillers always used to have a water tank
with a lid, making for much easier service and monitoring of water
condition. Other than that, both types are pretty well just pumps directly
driven by electric motors with some miscellaneous tubing and controls. Both
brands used to use the same pumps (made by Procon of Tennessee), and
probably still do.
Our Neslab has been pretty trouble-free; it's gone through one motor
so far and at least two pumps, but, as they say, your mileage may vary.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Eric Anderson [mailto:andersone1-at-southernct.edu]
Sent: Monday, May 10, 2004 1:03 PM
To: MSA listserver

Ooh, one more question:

The Philips EM400 installations I know of all utilized a Haskris
chiller. We're looking to buy a new chiller and they are considerably
cheaper from Neslab. Would anyone recommend against going with Neslab
for any reason?

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 15:32:29 2004

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We have been using a Neslab chiller since the beginning of time (I can't
find the original records). It runs without much complaint, most of the
time. We have replaced the motor (just an electric motor available from
Grainger's) once, replaced the pump once, and had the old pump rebuilt by
Procon once. We have replaced the shear pin ("nylon coupling")in the pump
head a number of times (maybe as much as once a year), and recharged the
compressor once in the last 6 years.

I've heard that the Haskris is a "better" chiller...but the Neslab seems to
do the job just fine. Their service support--by phone--is wonderful, and
they're in southern NH if you need to send something to them.

I highly recommend having a supply of shear pins available, and definitely
have them teach you how to change them if you never have done this
before--it's a little tricky the first time.

No interest in Neslab other than long experience as a user...

Deborah H. Gaynor, Ph.D.
Scanning Electron Microscopist
Analytical Services, Inc.
PO Box 515
Williston, VT 05495
802-878-5138 x21

-----Original Message-----
} From: Thomas, Frank [mailto:FThomas-at-nrcan.gc.ca]
Sent: Monday, May 10, 2004 2:58 PM
To: 'Eric Anderson'; MSA listserver

Eric -

The only thing I don't particularly care for in our (?8-year-old)
Neslab chiller is the fact that the water reservoir is pretty well sealed
up, like a miniature 45-gallon drum on its side, so you can't see what's
going on in there. The Haskris chillers always used to have a water tank
with a lid, making for much easier service and monitoring of water
condition. Other than that, both types are pretty well just pumps directly
driven by electric motors with some miscellaneous tubing and controls. Both
brands used to use the same pumps (made by Procon of Tennessee), and
probably still do.
Our Neslab has been pretty trouble-free; it's gone through one motor
so far and at least two pumps, but, as they say, your mileage may vary.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Eric Anderson [mailto:andersone1-at-southernct.edu]
Sent: Monday, May 10, 2004 1:03 PM
To: MSA listserver

Ooh, one more question:

The Philips EM400 installations I know of all utilized a Haskris
chiller. We're looking to buy a new chiller and they are considerably
cheaper from Neslab. Would anyone recommend against going with Neslab
for any reason?

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 17:03:35 2004

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Has anyone tried any of the anti-GFP antibodies on the market for
western blotting? Many seem to be cheaper than Clontech for the same
amount but we don't want to buy an untested antibody. Thanks- Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 18:18:11 2004

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What are you trying to look at with your EDS?
What kind of EDS is it?

The "normal" calibration of EDS is done at Al
K alpha (1.486KeV) and Cu K alpha (8.040KeV).
This sets resolution of the EDS according to these
two peaks. The other checks I do are done at C, O and F
and at N & O. And finally, FWMH at Mn.

For these measurements, I use X-Checker and X-Checker Extra.
For C, O and F, I use an Al stub with a Carbon sticky tab
with Teflon tape about 50% covering the stub and the other
50% split between sticky tab and bare Aluminum pin stub.
These readings do not calibrate the system. They produce
resolution figures for ability to resolve light elements.
You can do similar analysis for heavier elements with other
stub configurations.

The rationale for light element work is to see if the
EDS system, over time, drifts in the wrong direction.
Then I would know that something is going bad, either window
problems or EDS system problems. You will see this right
away at low Z.

If you are looking for ISO standards, I'm not sure how
that would work. Cu is Cu and Al is Al. The Cu and Al
peaks are used. If any foreign material was present, it
is simply ignored. The EDAX calibration routine only looks
at the Al and Cu peaks.

gary g.

At 06:08 AM 5/10/2004, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon May 10 18:27:40 2004

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I have been running my Haskris, on my EM410, virtually continuously,
since November 1982. I have replaced no parts. I have another Haskris
on my 1999 Hitachi S3500-N that has an intermittent algae problem, and
has also needed the starter capacitor on the motor replaced.

Rick A. Harris, exDirector
Microscopy and Imaging Facility
Section of Molecular and Cellular Biology
1241 Life Sciences Addition
University of California
Davis, CA
530 752 2914
http://microscopy.mcb.ucdavis.edu
raharris-at-ucdavis.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 11 02:06:04 2004

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Some precisions, as Peter has asked :

The question comes for a job on thin film of materials such Sr2TiMoO4 and
CoFe2O4 grown by laser ablation. The goal is to control the stochioametric
variation from the films, in comparaison with the target material, which
we have as a powder, or as sintered target. So I need to embed the powder,
or pieces of the sintered bulk, to make a polished surface of
it. I reed in a paper from Geller in the NIST bull. mentionned by someone
on the list about the use of silver charged epoxy. As I use some by the
way for fixing sample for spark machining, I was in question about what
kind could do the job for my standards.

As I have understand the electrical conductivity in such materials will be
done by tunneling effect between the silver grain, through the epoxy. So
it is not so macroscopic. I'll try the methode with carbon black. Seems to
be interesting and much cheaper than all the commercial silver epoxys. And
with carbon, the problem of siver L lignes signal will be avoid.

These standards are used as references for thin films analysis, using
Stratagem thin film software.

Some other suggestions ?
Many thanks.

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

On Mon, 10 May 2004, Tomic, Peter (Peter) wrote:

}
}
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} Jacques;
}
} What is the material of interest? You need to say. Obviously it can't be silver but you may want to check to see if you have silver spectrally overlapping the material or element of interest. Is your concern primarily sample charging therefore you want a conductive epoxy?
}
} Regards,
}
} Peter Tomic
} Agere Systems
}
} -----Original Message-----
} } From: Faerber Jacques [mailto:Jacques.Faerber-at-ipcms.u-strasbg.fr]
} Sent: Monday, May 10, 2004 9:09 AM
} To: Microscopy Society of America
} Subject: [Microscopy] EDS standards embedding
}
}
}
}
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}
} Hi
}
} What type of silver charged epoxy will be used to make embedding of powder
} as standards for EDS microanalysis. If one looks at Epotek's catalog,
} there are so much type of epoxys, with very different properties, shelf
} live and price. So what is the best compromise. If someone has an advice.
}
} Many thanks
}
} J. Faerber
} IPCMS-GSI
} (Institut de Physique et Chimie des Matériaux de Strasbourg
} Groupe Surface et Interfaces)
} 23, rue de Loess ; BP43
} 67034 Strasbourg CEDEX 2
} France
}
} Tel 00 33(0)3 88 10 71 01
} Fax 00 33(0)3 88 10 72 48
} E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 11 03:24:48 2004

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Rick

this may be drifting off topic a bit, but we used to have algae problems with our water cooler until I covered the translucent plastic hose with aluminium foil. There doesn't seem to have been a problem for over a year and there is little need to clean out the system these days.

I know that you can get black pressure hoses as an alternative but you can't buy them from your local supermarket for ~ 1 UK pound and fit them in a few minutes while the system is running.

Malcolm

Malcolm Haswell
e.m. unit
University of Sunderland
UK

e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: "Rick A. Harris" {raharris-at-ucdavis.edu}

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mivalmar-at-yahoo.es) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 11, 2004 at 15:10:15
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Email: mivalmar-at-yahoo.es
Name: Miguel V.Serrano

Organization: C.Haya Hospital

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I want to ask if someone has tryed to do an immunohistochemistry of PPAR alpha (peroxisome proliferator receptor alpha) in rat liver or another tissue ??. Thanks.

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From MicroscopyL-request-at-ns.microscopy.com Tue May 11 15:21:51 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donovanl-at-ufl.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 11, 2004 at 12:50:14
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Email: donovanl-at-ufl.edu
Name: Laura Donovan

Organization: University of Florida College of Veterinary Medicine

Title-Subject: [Microscopy] [Filtered] MListserver:Nikon Labophot 1x objective

Question: I am looking for a 1x objective for a Nikon Labophot, and having a difficult time.
Lab phone: (352)392-4700 ext. 3845
ask for Rose or Laura.

Thank you.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 00:36:05 2004

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I'm sorry that this is a bit of a deviation, but, knowing how diverse this list is, somebody
may be able to help:-

I have a Stanton-Redcroft Thermal Analyser, an STA-1600, the company in its last
years was acquired by Polymer Laboratories and then by Rheometrics, and I'm
interested in exploring the possibility of hooking analytical instruments, maybe NDIR or
even mass-spec, to the gas outlet line, to analyse the evolved gases (what was referred
to some time ago, so nicely, by Stanton-Redcroft as "hyphenated techniques").

Does anyone have such a setup?

Presumably one would use a heated PTFE interface tube, but the furnace internal
volume is fairly large, and not necessarily efficiently swept by the 50 ml/min or so of
purge gas, and what I'm wondering about is the time resolution of such EGA in this
instrument.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 04:52:33 2004

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Gary writes ...

} The "normal" calibration of EDS is done at Al
} K alpha (1.486KeV) and Cu K alpha (8.040KeV).
} ...

Out of curiosty, why would a calibration use these
2 peaks rather than CuK and CuL?? Understandably,
the L-line would be a convolution of the L-family,
but I would think the Al K line is in a more difficult
location relative to the slope in the continuum(???)
Is there any preference with respect to EDX window
type? (e.g., Be v UTW)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 05:04:38 2004

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Dear colleagues

We are looking for the RIGHT answers.
Addressing different institutions across the globe appear to be a very difficult.
We have been sent into circles for months without one clear cut answer.

Our EM technician has a HND in Environmental Science. He has been in the EM Unit for just over
a year and is slowly getting the hang of things. We would like to promote him up the ranks.
He has got the right aptitude, has matured and is responsible. Nice to find people like that still.

For him to be promotable, the University require at least a first degree (Senior Technician)
and Masters (Chief Technician). Without going through the rest of the gory details, he need further study. It is the policy of the University of Botswana to send citizens abroad rather than to study locally to enrich the nation academically.

The ranking of preference is 1) South Africa, 2) Australia, 3) USA, 4) UK.

He would prefer to do a EM focused masters. If he can do a pure Electron Microscopy Masters through course and lab work the better. The preference will be in the field of Material Science if he can not do a masters in "electron microscopy".

1) For him to be send by the University for a first degree and a masters consecutively, he must find at least partial sponsorship/bursary.
2) Who must he contact. (Please one name only in your institution, not a string of people!)
3) Can he get Credit for his current qualification?
4) Academic year start, requirements, and duration of study.

We are keeping our fingers crossed.
Thanks

Since my UB mail address is not reliable please send
a copy of all urgent mail to coetzeesh-at-yahoo.co.uk

Mr S. H. Coetzee
Electron Microscope Unit
University of Botswana
Private Bag 0022
Gaborone
Botswana

Phone : +267 355 2462/5222
Mobile : +267 714 55701 (Now active)
Fax : +267 318 5097
e-mail : coetzees-at-mopipi.ub.bw

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 06:52:59 2004

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Hello Ritchie,

FWIW, we have a Leybold quadrapole RGA which we often connect to our vacuum
furnace to monitor evolved gasses. Since the RGA operates at much higher
vacuum than the furnace, the interface is made using conflat flanged s-steel
fittings and a quality leak valve.

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Wednesday, May 12, 2004 1:45 AM
To: Microscopy-at-sparc5.microscopy.com

I'm sorry that this is a bit of a deviation, but, knowing how diverse this
list is, somebody
may be able to help:-

I have a Stanton-Redcroft Thermal Analyser, an STA-1600, the company in its
last
years was acquired by Polymer Laboratories and then by Rheometrics, and I'm
interested in exploring the possibility of hooking analytical instruments,
maybe NDIR or
even mass-spec, to the gas outlet line, to analyse the evolved gases (what
was referred
to some time ago, so nicely, by Stanton-Redcroft as "hyphenated
techniques").

Does anyone have such a setup?

Presumably one would use a heated PTFE interface tube, but the furnace
internal
volume is fairly large, and not necessarily efficiently swept by the 50
ml/min or so of
purge gas, and what I'm wondering about is the time resolution of such EGA
in this
instrument.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext
87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 07:42:46 2004

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shAf,
I've thought that for a long time but have yet to find a software-based
calibration that can use the 2 Cu peaks. Maybe the vendors can speak to
this.

As to Gary's question of why one needs standards, I have a hunch
they're not looking for EDS calibration standards (a piece of Cu tape on
an Al stub works just fine) but quantitative analysis standards for high
quality quant work. Despite the software advances in standardless
analysis, everyone I've talked to who really knows x-ray says that
standardless quant just doesn't have the accuracy or precision of
standards-based analysis.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

michael shaffer wrote:

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From MicroscopyL-request-at-ns.microscopy.com Wed May 12 08:48:21 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sp-bf-at-physik.upb.de) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 12, 2004 at 05:24:26
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Email: sp-bf-at-physik.upb.de
Name: Bettina Friedel

Organization: University of Paderborn

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi all!

Our physics group got a Hitachi H-600 a few years ago from biology group. We repaired it and there was no problem. But now the wire from the linkage of the specimen chamber has broken. It jumped out from the guide rolls and now we cannot move the specimen in one direction. "Nissei Sanyo Europe",the Hitachi Service Center here, demands 3500Ä for repair of this silly wire.
I hope anyone can help me!!! Is there a plan (blueprint?) how to thread the wire through the rolls, so that we could repair it ourself, not perfect but in this way, that moving of the specimen would be possible?

Bettina Friedel

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From MicroscopyL-request-at-ns.microscopy.com Wed May 12 09:33:30 2004

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I am trying to label the GFP in yeast on either Lowicryl sections or Tokuyashu cryosections. So far, we have had rather poor labeling/high background. I would appreciate any recommendations on a particular commercially available antibody and the fixation protocol.

Also, we would need to label a biotin-tagged protein. We were trying Streptavidin - gold, but to little success. Is there a good anti-biotin antibody (or, even better, anti-biotin/gold conjugate) people have used
for this purpose before?

Any recommendations would be highly appreciated.

Michael Jarnik,
EM Facility
Fox Chase Cancer Center
Philadelphia, PA

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 10:50:57 2004

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Just guessing, but I would suppose the energy calibration is a rather
simplistic algorithm. I am pretty sure that is much easier to work with a
symmetric K peak and pick off the centroid than it is to deconvolute the L
peaks to find the energy of the alpha line.

Presumably the effect of the background slope and curvature is negligible
compared to the peak intensity if all they have to do is get a peak energy.

Warren

At 04:57 AM 5/12/2004, "michael shaffer" wrote:
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From MicroscopyL-request-at-ns.microscopy.com Wed May 12 12:36:06 2004

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michael

i', sorry, but your second question is not clear to me. are you simply
trying to label your protein with gold, or is this a detection step
where you have already used the antibody to react with its antigen and
now want to see if where the antigen is? also, do you have any antibody
which is not tagged with biotin and that you could use for tagging with
either nanogold or directly onto larger gold labels? finally, could you
do an indirect reaction using gold tagged antibody to the host species
antibody you are using, eg, say the biotin-antibody is an IgG species,
raised in mouse, could you come back with colloidal gold:anti mouse IgG?

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-392

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 12:38:32 2004

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On May 12, 2004, at 2:57 AM, michael shaffer wrote:

} Out of curiosty, why would a calibration use these
} 2 peaks rather than CuK and CuL?? Understandably,
} the L-line would be a convolution of the L-family,
} but I would think the Al K line is in a more difficult
} location relative to the slope in the continuum(???)
} Is there any preference with respect to EDX window
} type? (e.g., Be v UTW)
}
} I've thought that for a long time but have yet to find a
} software-based calibration that can use the 2 Cu peaks. Maybe the
} vendors can speak to this.

Dear Mike and Ken,
Since the Al k-line is at 1.4 keV and the Cu l-line(s) is at ~1 keV,
the Al is more readily separated from the continuum. I don't know of a
difference between Be and UTW calibrations, since it is the response of
the crystal that is being measured, but, perhaps there is an advantage
to using a lower-energy line with the UTW.
The TN2000 had software that could use any two lines. One simply
entered the energies and ran the calibration routine. I guess someone
must have "improved" the system by entering the line energies for us.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 12:54:20 2004

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Sorry, I would try to make it clearer. We need to localize a viral
protein which has been biotin-tagged and expressed in cell culture. I
expected it should be no problem to label it with Streptavidin
conjugate, but it is not that easy, it seems (even according to some
other people). So, as we do not have a good antibody to the viral
protein, I am considering an indirect labeling with anti-biotin
antibody and a secondary conjugate. There are tons of commercially
available anti-biotin antibodies, but certainly not all of them will
work with EM protocols - so I was interested whether somebody has
experience with some of these.

Thanks,

Michael

paul r hazelton wrote:

} michael
}
} i', sorry, but your second question is not clear to me. are you simply
} trying to label your protein with gold, or is this a detection step
} where you have already used the antibody to react with its antigen and
} now want to see if where the antigen is? also, do you have any antibody
} which is not tagged with biotin and that you could use for tagging with
} either nanogold or directly onto larger gold labels? finally, could you
} do an indirect reaction using gold tagged antibody to the host species
} antibody you are using, eg, say the biotin-antibody is an IgG species,
} raised in mouse, could you come back with colloidal gold:anti mouse IgG?
}
} paul
}
} Paul R. Hazelton, PhD
} Electron Microscope Unit
} University of Manitoba
} Department of Medical Microbiology
} 531 Basic Medical Sciences Building
} 730 William Avenue
} Winnipeg, Manitoba, Canada, R3E 0W3
} e-mail: paul_hazelton-at-umanitoba.ca
} Phone:204-789-3313
} Pager:204-931-954
} Cell:204-781-1502
} Fax:204-789-392
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:22:55 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rpowell-at-nanoprobes.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 12, 2004 at 12:22:51
---------------------------------------------------------------------------

Email: rpowell-at-nanoprobes.com
Name: Rick Powell

Organization: Nanoprobes, Incorporated

Title-Subject: [Microscopy] Anti-GFP and anti-biotin Abs for TEM (vendor reply)

Question: Hello Michael:

[Vendor reply...] We (Nanoprobes, Inc,) make an anti-biotin-IgG gold conjugate using our 1.4 nm Nanogold particle; we also offer streptavidin-Nanogold. You don't say why the streptavidin-gold didn't work - if you could let us have some details, we may have some suggestions.

Hope this is useful,

Rick Powell
Nanoprobes, Inc.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:24:42 2004

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In a discussion I had with a service rep for EDAX Inc., the calibration is nothing more than setting the A/D [Analog to digital] converter's scale and offset. It doesn't change anything with respect to the detector itself.

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]
Sent: Wednesday, May 12, 2004 11:57 AM
To: Microscopy-at-msa.microscopy.com

Just guessing, but I would suppose the energy calibration is a rather
simplistic algorithm. I am pretty sure that is much easier to work with a
symmetric K peak and pick off the centroid than it is to deconvolute the L
peaks to find the energy of the alpha line.

Presumably the effect of the background slope and curvature is negligible
compared to the peak intensity if all they have to do is get a peak energy.

Warren

At 04:57 AM 5/12/2004, "michael shaffer" wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:26:36 2004

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Hi Michael,

I've had great results on cryo-sections with a rabbit anti-GFP antibody
from
Molecular Probes: cat# 11122
Works well at dilutions ranging from 1:50-1:200.
Low background.
Hope it works for you.
Best

Marc

On Wednesday, May 12, 2004, at 10:39 AM, Michal Jarnik wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
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} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
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}
} I am trying to label the GFP in yeast on either Lowicryl sections or
} Tokuyashu cryosections. So far, we have had rather poor labeling/high
} background. I would appreciate any recommendations on a particular
} commercially available antibody and the fixation protocol.
}
} Also, we would need to label a biotin-tagged protein. We were trying
} Streptavidin - gold, but to little success. Is there a good
} anti-biotin antibody (or, even better, anti-biotin/gold conjugate)
} people have used for this purpose before?
} Any recommendations would be highly appreciated.
} Michael Jarnik,
} EM Facility
} Fox Chase Cancer Center
} Philadelphia, PA
}
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:32:23 2004

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Fellow Microscopists,

The Microscopy Lab in our Research Center has 3 SEM's, 1 TEM and 1 EMPA
(with a second due in November) in addition to 4 XRD instruments. Our
main function has been as a problem solving facility to our researchers as
well as our field service engineers. Data produced by our lab is usually
issued as reports with images, spectra and graphs as attachments.
Management has directed us to implement a LIMS by the end of the year.
Their requirements include the ability of the researchers and field service
engineers to log samples in from their locations and the tracking of the
sample from the arrival in our lab to the issuance of data. It must also
be able to archive the data as well. For us this means literally hundreds
of images, spectra and reports each month that must be categorized and
saved. The researchers and engineers must also be able to access the data
from their location. This will probably mean a web based system since our
facilities cover the globe.

Has anyone out there been faced with a similar request? Our main hurdle is
convincing management that ours is not a "sample in - number out" type of
lab, and that most LIMS packages out there are designed for that type of
simple operation. If you have implemented such a system, was it an off the
shelf package, a custom designed package or a combination? If you want to
respond to me directly that would be fine. I am not interested in "system
bashing" just some helpful suggestions on how to make management happy
without losing my sanity.

Sharon Goresh
Chemist
sharon.goresh-at-engelhard.com

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 15:04:11 2004

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we like the bethyl labs mouse anti-biotin then follow that with goat
anti-mouse conjugated to gold. it is much better than streptavidin
gold. i am looking for a gfp ab so let me know what works.

At 10:39 AM 5/12/2004 -0400, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 15:26:13 2004

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The Moran Scientific EDS software can use the Cu L and K peaks (or any others the
user chooses) for the peak position calibration. I do this.

It would be a bit more correct not to use L peaks, because, as Shaf said, it's an
unresolved group of lines, so the resolution that gets calculated at the low energy end
isn't quite correct, but unless you're using virtual standards, that doesn't matter.

But hey, even the Al K peak is the Ka1 plus the Ka2 plus the Kb anyway, on an EDS.

cheers

rtch

Date sent: Wed, 12 May 2004 08:48:26 -0400
} From: qualityimages {qualityimages-at-netrax.net}
To: michael shaffer {michael-at-shaffer.net} ,
Microscopy {Microscopy-at-Sparc5.Microscopy.Com}

Dear Michael,
I just checked, and my Quartz XOne system can use any two peaks, including Cu Ka
and Cu La, to calibrate the system. The tradition may be to use Al Ka and Cu La
because those two elements are easy to find in most EM labs and the old
Be-window detectors did not always see Cu La well. Of course, the accuracy of
your calibration will depend on the separation of your peaks and their accurate
location. Ka peaks are sharper than La peaks, so it may improve your calibration
accuracy to use two Ka peaks.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 12, 2004 2:57 AM

Michael,

In response to your question, most, if not all, EDX manufacturers today
including RÖNTEC find it necessary to use only one specified energy line
plus the zero peak. This is because linearity is so high, that a 3-point
calibration (two specified spectral lines + zero peak) for almost all cases
is not beneficial.

Martin Rohde
RÖNTEC GmbH
RÖNTEC USA, Inc.
www.rontec.com

} On May 12, 2004, at 2:57 AM, michael shaffer wrote:

} Out of curiosty, why would a calibration use these
} 2 peaks rather than CuK and CuL?? Understandably,
} the L-line would be a convolution of the L-family,
} but I would think the Al K line is in a more difficult
} location relative to the slope in the continuum(???)
} Is there any preference with respect to EDX window
} type? (e.g., Be v UTW)
} }
} I've thought that for a long time but have yet to find a
} software-based calibration that can use the 2 Cu peaks. Maybe the
} vendors can speak to this.

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 17:04:32 2004

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Hi Michael,

It's me again.
Actually I have used an anti-biotin that
worked well for immuno-EM.
It's from Rockland, cat # 200-4198.
It's a rabbit antibody, IgG fraction.

I too had problems using streptavidin-gold.
The reason for this, I think, is a lack of stability of
the conjugate. Don't forget that when you purchase
a gold conjugate, it might have sat for months on
a refrigerator shelve and the proteins have either
been degraded or fallen off the gold particles!

In my experience, good sources for antibodies
that work at the EM level are Cappel (bought a
a few years back by ICN - now called MP
Biomedicals), Rockland (to a lesser extent),
and Molecular Probes. I only use protein A
gold for my labelings, and I certainly avoid
gold conjugates from Ted Pella that have not
worked for me even once in the last 5 years!
Good luck

Marc

On Wednesday, May 12, 2004, at 01:59 PM, Michal Jarnik wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Sorry, I would try to make it clearer. We need to localize a viral
} protein which has been biotin-tagged and expressed in cell culture. I
} expected it should be no problem to label it with Streptavidin
} conjugate, but it is not that easy, it seems (even according to some
} other people). So, as we do not have a good antibody to the viral
} protein, I am considering an indirect labeling with anti-biotin
} antibody and a secondary conjugate. There are tons of commercially
} available anti-biotin antibodies, but certainly not all of them will
} work with EM protocols - so I was interested whether somebody has
} experience with some of these.
}
} Thanks,
}
} Michael
}
} paul r hazelton wrote:
}
} } michael
} }
} } i', sorry, but your second question is not clear to me. are you
} } simply
} } trying to label your protein with gold, or is this a detection step
} } where you have already used the antibody to react with its antigen and
} } now want to see if where the antigen is? also, do you have any
} } antibody
} } which is not tagged with biotin and that you could use for tagging
} } with
} } either nanogold or directly onto larger gold labels? finally, could
} } you
} } do an indirect reaction using gold tagged antibody to the host species
} } antibody you are using, eg, say the biotin-antibody is an IgG species,
} } raised in mouse, could you come back with colloidal gold:anti mouse
} } IgG?
} }
} } paul
} }
} } Paul R. Hazelton, PhD
} } Electron Microscope Unit
} } University of Manitoba
} } Department of Medical Microbiology
} } 531 Basic Medical Sciences Building
} } 730 William Avenue
} } Winnipeg, Manitoba, Canada, R3E 0W3
} } e-mail: paul_hazelton-at-umanitoba.ca
} } Phone:204-789-3313
} } Pager:204-931-954
} } Cell:204-781-1502
} } Fax:204-789-392
} }
} }
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 17:44:13 2004

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I believe the real object of this is to find two peaks separated far enough in energy to allow the A/D converter to calibrate over a broad range. The broader the less the error. From an electronic point of view, it doesn't matter which peaks are used, just that they have significant separation. The electronics doesn't know the difference. It goes from peak height to a position in energy which corresponds to a voltage which gates a clock. I'm babbling, only electrical engineers worry about these things.

Any EDX vendors care to comment?

Peter

-----Original Message-----
} From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
Sent: Wednesday, May 12, 2004 4:31 PM
To: michael shaffer
Cc: Microscopy

Dear Michael,
I just checked, and my Quartz XOne system can use any two peaks, including Cu Ka
and Cu La, to calibrate the system. The tradition may be to use Al Ka and Cu La
because those two elements are easy to find in most EM labs and the old
Be-window detectors did not always see Cu La well. Of course, the accuracy of
your calibration will depend on the separation of your peaks and their accurate
location. Ka peaks are sharper than La peaks, so it may improve your calibration
accuracy to use two Ka peaks.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 12, 2004 2:57 AM

Dear Peter,
Your age is showing, the electronics are all purely digital, now. No A/D
converter needed. The only reason to use two Ka peaks instead of a Ka and an La
peak are that the Ka peaks are sharper and so the peak centroid is more
precisely located. The software calibration sets the zero point and the
amplifier gain to a fraction of a channel. With the newer, higher-resolution
detectors, more quant precision and lower detection limit is possible, but the
calibration is more critical, since a tiny shift of the peak throws off all the
quant calculations. I find my self calibrating every month where I used to do it
once a year with the old A/D system, but my results are much better.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "Tomic, Peter (Peter)" {ptomic-at-agere.com}
To: "Mary Mager" {mager-at-interchange.ubc.ca} ; "michael shaffer"
{michael-at-shaffer.net}
Cc: "Microscopy" {microscopy-at-MSA.microscopy.com}
Sent: Wednesday, May 12, 2004 3:49 PM

Dear Michael,
I just checked, and my Quartz XOne system can use any two peaks, including Cu Ka
and Cu La, to calibrate the system. The tradition may be to use Al Ka and Cu La
because those two elements are easy to find in most EM labs and the old
Be-window detectors did not always see Cu La well. Of course, the accuracy of
your calibration will depend on the separation of your peaks and their accurate
location. Ka peaks are sharper than La peaks, so it may improve your calibration
accuracy to use two Ka peaks.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 12, 2004 2:57 AM

} I find my self calibrating every month where I used to do it once a
} year with the old A/D system, but my results are much better.

Once a month!

Once a year!

I do it once or twice a day.

But that's Virgoans for you. We worry a lot.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 20:07:12 2004

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Hi Bettina,
I have the user's manual for the Hitachi H-600.
I will email you the diagrams.
I remember my boss trying to fix this problem and it almost drove him crazy.

Good luck!

John Brealey
Medical Scientist
Electron Microscopy Unit
The Queen Elizabeth Hospital
IMVS - TQEH Pathology
Woodville, 5011
South Australia
(08) 82226612

Bettina Friedel wrote:

Email: sp-bf-at-physik.upb.de
Name: Bettina Friedel

Organization: University of Paderborn

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi all!

Our physics group got a Hitachi H-600 a few years ago from biology group. We
repaired it and there was no problem. But now the wire from the linkage of
the specimen chamber has broken. It jumped out from the guide rolls and now
we cannot move the specimen in one direction. "Nissei Sanyo Europe",the
Hitachi Service Center here, demands 3500Ä for repair of this silly wire.
I hope anyone can help me!!! Is there a plan (blueprint?) how to thread the
wire through the rolls, so that we could repair it ourself, not perfect but
in this way, that moving of the specimen would be possible?

Bettina Friedel

____________________________

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 22:08:20 2004

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That is nice, but I would like more justification about
why only one point is adequate. I do not buy into this
hypothesis.

EDAX uses Al and Cu peaks. I think that this works very well.
And, it uncovers subtle problems that otherwise would go
un-noticed. I cannot see how a one point calibration
is a calibration at all. Please explain this to me.

The two disparate Al-Cu peaks makes a lot of sense for
calibrating an EDS. In addition to this, I do C, O, F
and Al measurements with one stub. This is a separate
"standard." When the results shift, if they do, I am
concerned. Lately, they have shifted. And I am concerned.
EDAX is on the job. Cool.

The point is to establish a set of standards and
use them frequently. When the results change, contact
the manufacturer. They will not know your situation
unless you tell them.

gary g.

At 02:52 PM 5/12/2004, you wrote:
} Michael,
}
} In response to your question, most, if not all, EDX manufacturers today
} including RÖNTEC find it necessary to use only one specified energy line
} plus the zero peak. This is because linearity is so high, that a 3-point
} calibration (two specified spectral lines + zero peak) for almost all cases
} is not beneficial.
}
} Martin Rohde
} RÖNTEC GmbH
} RÖNTEC USA, Inc.
} www.rontec.com
}
} } On May 12, 2004, at 2:57 AM, michael shaffer wrote:
}
} } Out of curiosty, why would a calibration use these
} } 2 peaks rather than CuK and CuL?? Understandably,
} } the L-line would be a convolution of the L-family,
} } but I would think the Al K line is in a more difficult
} } location relative to the slope in the continuum(???)
} } Is there any preference with respect to EDX window
} } type? (e.g., Be v UTW)
} } }
} } I've thought that for a long time but have yet to find a
} } software-based calibration that can use the 2 Cu peaks. Maybe the
} } vendors can speak to this.

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 02:22:32 2004

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Intersting !

The topic shifted a bit but with interesting points !

About that calibration questions, my few (Euro) cents :

No ADC ? Of coarse, an ADC is still necessary, but just after the
(still analogic) preamp, and no more after the hole ( former analogic)
counting unit.

Two points or more for energy calibration ? First point, the zero.
I suppose that all today sold systems, like that we have, have a dynamic
zero measurement, done on the noise peak. So nothing to do with the zero,
it is continously corrected. I suppose too that the energie range of the
(numerical) MCA is linear. So one (measured) peak in the midlle of the
range, that is between 6 and 12 keV will be good, as said a k line will be
sharper. Fe, Co or Cu... On our first Tracor NS 880, it was the first job
every morning, to play with the the gain and offset trimpot, on two lines.
With 150 eV resolution and a Be window, Al K was better tha Cu L (+ Cu K
for high energy). A good way to put your nerves in condition to welcome
your boss with a smile, when he came with a stupid question !

How often is it necessary to calibrate it ? Depends of the
stability of the system and of the accuracy wanted. But realy, the need of
a new calibration will be easily seen when one look the currently acquired
spectra. Particulary when one work with the same family of coumpound. A
shift in energy, whith a good statistic, if not been quantified, can be
well detected with the eyes ! It's too with the eyes on the spectrum, that
one can apreciated the real presence of a trace element, even when the
soft say that you have 0.000005 % of element Xy (without overlapping, of
coarse) !

And the embeding of my standards ? Nothing more to suggest ? My tests with
the epoxy I have show that it is not fluid enough. So, much bulbes...

Jacques

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 02:36:03 2004

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Resisted the urge to jump in before now, but can't any longer.

Your reasons for use of two K peaks is good, might I also add that K peaks
will also offer better statistics as their count rates will be higher, thus
distinguishing them better from noise and background. Most software these
days allows the use of any two peaks. The choice of calibration peaks
should be made on the materials you normally analyze. There can be
non-linearities in the detector, pre-amplifier and amplifier responses that
could be a problem if you choose peaks that are too widely separated.
Aluminum and copper are commonly used because they fall within the range
of elements commonly analyzed. If, on the other hand, you commonly are
analyzing lanthanide's or actinides, you might want to choose peaks of
higher atomic number.

Problem is that we still have to render the avalanche pulse output from a
silicon detector, that merges millions of electron transfers into a single
pulse who's voltage peak represents energy of the x-ray photon causing it,
to a digital format. That pretty much is the definition of an analog to
digital converter. This function is not abandoned in current designs, only
performed earlier in the electronics. There is still an A/D converter in
the signal chain, it is just faster and controlled by a DSP.

Modern designs, because of increased time resolution of processors and A/D
converters, use digital signal processors (DSP) to provide many of the
functions that were previously done with dedicated electronics. This
trade-off has its own set of problems. Firmware is now responsible for the
identification of peaks, dead time and pulse pile-up and there may be cases
where that firmware could use a little tuning. This trend has resulted in
manufacturer's claims of greater counting rates and resolution but also
results in greater uncertainties as manufacturers strive to meet those
claims. If you are finding that you have to calibrate your EDS system more
frequently that is probably because of those uncertainties.

The recent trend has been to blame the inadequacies of EDS analyses on the
interpretation of the signals from the detectors rather than those signals
themself. In truth, we seem to have, for the moment, stretched the limit
of detector technology and perhaps over-stretched the detection of those
signals. The need for more frequent calibration may well be because the
state of the art in pulse measurement has exceeded the state of the art in
detector technology.

This thread has bifurcated into one that addresses the basic energy
calibration of the detector and electronics and one that addresses the
similar matrix calibrations required for good quantitative analysis. In
regards to that, let me say that these are two very different, yet
interrelated, areas. These are some of the most accurate measurements made
in common laboratory settings and deserve some common understanding. In
one case, we are calibrating our instrumentation to simplistic physical
properties we understand. In the other, we are accommodating our
instruments to complex interactions that we can't completely explain.

EDS calibration involves finding two reliable points that we can use to
establish a linear correction to the corresponding digital values that are
delivered to the computer doing the analysis. While the underlying
assumption is that this is a linear relationship, that's not necessarily
so. That assumption is generally made in the software that then uses this
data to produce results that claim to be quantitative using either
standards based or standardless algorithms.

Similar matrix calibration involves the use of well characterized standards
that are of a range of composition similar to that expected in the unknown
sample to provide a refinement of the simplistic linear corrections
mentioned above. These standards and corrections allow us to improve our
quantitative estimations by narrowing the range of linear corrections used.
In reality, the interelement interactions in any particular sample can not
be completely derived from the actions of their individual components at
the present time.

This is still an empirical science, like it or not. As such, we have to
continually accommodate our instrumentation to the task rather than to an
ideal. Those accommodations will continue to be a problem and a limitation
to the results we derive.

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174

phone (630) 513-7093 fax (630) 513-7092 http://www.sem.com

On Wednesday, May 12, 2004 6:09 PM, Mary Mager
[SMTP:mager-at-interchange.ubc.ca] wrote:
}
}
}
------------------------------------------------------------------------
------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
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-------
}
} Dear Peter,
} Your age is showing, the electronics are all purely digital, now. No A/D
} converter needed. The only reason to use two Ka peaks instead of a Ka and
an La
} peak are that the Ka peaks are sharper and so the peak centroid is more
} precisely located. The software calibration sets the zero point and the
} amplifier gain to a fraction of a channel. With the newer,
higher-resolution
} detectors, more quant precision and lower detection limit is possible,
but the
} calibration is more critical, since a tiny shift of the peak throws off
all the
} quant calculations. I find my self calibrating every month where I used
to do it
} once a year with the old A/D system, but my results are much better.
} Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on
occasion.
} Regards,
} Mary Mager
} Electron Microscopist
} Department of Materials Engineering
} University of British Columbia
} 6350 Stores Road
} Vancouver, B.C. V6T 1Z4
} CANADA
} tel: 604-822-5648
} e-mail: mager-at-interchange.ubc.ca
}
} ----- Original Message -----
} } From: "Tomic, Peter (Peter)" {ptomic-at-agere.com}
} To: "Mary Mager" {mager-at-interchange.ubc.ca} ; "michael shaffer"
} {michael-at-shaffer.net}
} Cc: "Microscopy" {microscopy-at-MSA.microscopy.com}
} Sent: Wednesday, May 12, 2004 3:49 PM
} Subject: [Microscopy] RE: Re: RE: Re: EDS standards embedding
}
}
} I believe the real object of this is to find two peaks separated far
enough in
} energy to allow the A/D converter to calibrate over a broad range. The
broader
} the less the error. From an electronic point of view, it doesn't matter
which
} peaks are used, just that they have significant separation. The
electronics
} doesn't know the difference. It goes from peak height to a position in
energy
} which corresponds to a voltage which gates a clock. I'm babbling, only
} electrical engineers worry about these things.
}
} Any EDX vendors care to comment?
}
} Peter
}
} -----Original Message-----
} } From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
} Sent: Wednesday, May 12, 2004 4:31 PM
} To: michael shaffer
} Cc: Microscopy
} Subject: [Microscopy] Re: RE: Re: EDS standards embedding
}
}
}
}
}
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} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
} Dear Michael,
} I just checked, and my Quartz XOne system can use any two peaks,
including Cu Ka
} and Cu La, to calibrate the system. The tradition may be to use Al Ka and
Cu La
} because those two elements are easy to find in most EM labs and the old
} Be-window detectors did not always see Cu La well. Of course, the
accuracy of
} your calibration will depend on the separation of your peaks and their
accurate
} location. Ka peaks are sharper than La peaks, so it may improve your
calibration
} accuracy to use two Ka peaks.
} Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on
occasion.
} Regards,
} Mary Mager
} Electron Microscopist
} Department of Materials Engineering
} University of British Columbia
} 6350 Stores Road
} Vancouver, B.C. V6T 1Z4
} CANADA
} tel: 604-822-5648
} e-mail: mager-at-interchange.ubc.ca
}
} ----- Original Message -----
} } From: "michael shaffer" {michael-at-shaffer.net}
} To: "Gary Gaugler" {gary-at-gaugler.com}
} Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
} Sent: Wednesday, May 12, 2004 2:57 AM
} Subject: [Microscopy] RE: Re: EDS standards embedding
}
}
} }
} }
} }
------------------------------------------------------------------------
------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
------------------------------------------------------------------------
------
} -
} }
} } Gary writes ...
} }
} } } The "normal" calibration of EDS is done at Al
} } } K alpha (1.486KeV) and Cu K alpha (8.040KeV).
} } } ...
} }
} } Out of curiosty, why would a calibration use these
} } 2 peaks rather than CuK and CuL?? Understandably,
} } the L-line would be a convolution of the L-family,
} } but I would think the Al K line is in a more difficult
} } location relative to the slope in the continuum(???)
} } Is there any preference with respect to EDX window
} } type? (e.g., Be v UTW)
} }
} } cheerios ... shAf :o)
} } Avalon Peninsula, Newfoundland
} } www.micro-investigations.com (in progress)
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 02:47:11 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

Most of us at some moment have to deal with the capture and storage of
image sequences, either as part of a video-experiment or when doing a
video time-lapse. Until 3 years ago, I did my video-microscopy on a
Silicon Graphics based system. The nice features of SGI were that we
could do multiple videostreams in parallel, which allowed us to do
multiposition time-lapse experiments.

However, three years ago I changed to another Unix-platform (Linux) and
to my unpleasant surprise, it was not so trivial anymore to keep
multiple video-streams in the air during an experiment and there were
some other caveats too.

In the end I decided that the only thing I needed was a simple way to
concatenate individual frames into a filestream, as for me the most
important issue is to put the frames where I can find them afterwards
for analysis, not so much for looking a them over anetwork at high
speed. The format should be simple, no overhead and frame-oriented, so
even mixing frames of different types should be possible. Another thing
I wanted to have, was that it should be possble to store 3D-frame
movie-sequences. Lossy compression schemes are not so beneficial for
image anlsysis aftwerwards, as they manipulate the frame content which
causes artefacts in the analysis.

The drawback of this frame-oriented approach is that some lossy
compression techniques, which require multiple frame comparison, are not
possible.

I would like to know if there are other people, doing video microscopy
who are also interested in this approach, maybe we could create a simple
software-library (ANSI C) which we can link with software we use, so we
can have a video-system designed and optimized for video-microscopy
(analysis oriented instead of visualization-oriented) ?

Regards,

Peter Van Osta

Director Imaging
MAIA SCIENTIFIC (formerly Union Biometrica NV)
Cipalstraat 3
B-2440 Geel
Belgium
Tel.: +32-(0)14 570 620
Fax.: +32-(0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 03:08:48 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Sharon,
it is possible to spend a lot of money on these systems. However, I
have yet to find one which offers significantly more than can be done with
MSExcel spreadsheets.

MSExcel spreadsheets on a server can be used in a 'shared' format, where
many people can open the same file without that irritating 'This file is
being used by...' error. In the system we have here, the files can only be
written to by a member of the analysis group, but read by anyone. People
have to come here to give us a sample anyway, so this is not a problem.
Each sample gets a line in the spreadsheet with the usual fields (date,
name, analysis needed etc.). When someone is working on a job, they put
their initials in the box for that analysis type; when the job is done, a
date goes in the box instead. The spreadsheet is updated every time someone
saves it. Each column has an 'Autofilter' at the top which means they can
be searched for any of the fields.
This 'master' spreadsheet contains hyperlinks to the electronic log books
for each microscope or technique (also shared MSExcel spreadsheets). These
are updated as the analysis happens, and here each image has a line giving
sample, analysis details, operator, customer, etc.. Each line in these
'technique' spreadsheets has a hyperlink to the data file. Again, each
column has an 'Autofilter' at the top which means they can be searched for
any of the fields.

As a user, it is easy to operate (that 'fill down' feature of Excel allows
you to copy the provious line and change one box without having to make 10
entries for each image). The only discipline needed is to keep saving the
files frequently (autosaving doesn't work, if two computers try to save at
the same time they can lock up). Our customers seem to be happy too - they
know the status of their job and can find the data without having to hassle
us. We rely on the standard software on each user's PC to be able to open
the images.

I'm not sure how this could be implemented on a web-based system, but for a
server it works very well. We keep track of about 4000 samples a year - and
all the data files they generate - with this system, and it usually only
takes a few minutes to find old data even from a vague description. I have
yet another spreadsheet which allows me to count how many jobs have been
done, are left to do, etc., for each analysis type. The nice thing about
spreadsheets is that they are totally 'customizable', so you only keep track
of what you think is important.

I'd be happy to send you an example of the files if you like. As a 'free'
solution it is hard to beat!

Cheers

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com
All incoming mail is filtered for spam. If you do not receive a reply from
me, do not assume I have received your mail.

-----Original Message-----
} From: Sharon_Goresh-at-engelhard.com [mailto:Sharon_Goresh-at-engelhard.com]
Sent: 12 May 2004 19:20
To: Microscopy-at-MSA.Microscopy.Com

Fellow Microscopists,

The Microscopy Lab in our Research Center has 3 SEM's, 1 TEM and 1 EMPA
(with a second due in November) in addition to 4 XRD instruments. Our
main function has been as a problem solving facility to our researchers as
well as our field service engineers. Data produced by our lab is usually
issued as reports with images, spectra and graphs as attachments.
Management has directed us to implement a LIMS by the end of the year.
Their requirements include the ability of the researchers and field service
engineers to log samples in from their locations and the tracking of the
sample from the arrival in our lab to the issuance of data. It must also
be able to archive the data as well. For us this means literally hundreds
of images, spectra and reports each month that must be categorized and
saved. The researchers and engineers must also be able to access the data
from their location. This will probably mean a web based system since our
facilities cover the globe.

Has anyone out there been faced with a similar request? Our main hurdle is
convincing management that ours is not a "sample in - number out" type of
lab, and that most LIMS packages out there are designed for that type of
simple operation. If you have implemented such a system, was it an off the
shelf package, a custom designed package or a combination? If you want to
respond to me directly that would be fine. I am not interested in "system
bashing" just some helpful suggestions on how to make management happy
without losing my sanity.

Sharon Goresh
Chemist
sharon.goresh-at-engelhard.com

=======================================================================
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information contained in it may be confidential and/or protected by
law. If you are not the intended recipient of this message, you must
not make any use of this information, or copy or show it to any
person. Please contact us immediately to tell us that you have
received this e-mail, and return the original to us. Any use,
forwarding, printing or copying of this message is strictly prohibited.
No part of this message can be considered a request for goods or
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=======================================================================
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From MicroscopyL-request-at-ns.microscopy.com Thu May 13 05:16:19 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Michael,

A two-step detection method is indeed a good option to visualize your
biotinylated viral protein. Compared to the 2-step method the advantage
of a 1-step immunodetection method, as you initially suggested, will be
improved resolution. Your labeling density decreases however. As you
know labeling density is inversely related to the gold particle size.

Improved resolution combined with high sensitivity can be obtained when
using gold conjugates prepared with Ultra-Small gold particles. For
your application we would recommend Goat anti Biotin Ultra-Small. See
e.g. Müller-Höcker et al., (1998), Histochem. and Cell Biol. 109(2),
119-125.

When the protein of interest is located on the outside of the virus, in
other words the biotin is accessible for the antibodies, another option
may be the use of a pre-embedding labeling procedure. The use of
Ultra-Small gold conjugates is a prerequisite to successfully combine
appropriate labeling densities with a decent morphology. See e.g.
Decossas et al, (2003) J. of Comp. Neurology 462(3), 302-314 for
details on this technique.

Hope this is of help
Kind regards,
Peter

------------------------------------------
Michael Jarnik wrote:

Sorry, I would try to make it clearer. We need to localize a viral
protein which has been biotin-tagged and expressed in cell culture. I
expected it should be no problem to label it with Streptavidin
conjugate, but it is not that easy, it seems (even according to some
other people). So, as we do not have a good antibody to the viral
protein, I am considering an indirect labeling with anti-biotin
antibody and a secondary conjugate. There are tons of commercially
available anti-biotin antibodies, but certainly not all of them will
work with EM protocols - so I was interested whether somebody has
experience with some of these.

Thanks,

Michael

-----------
Peter van de Plas
Aurion
Costerweg 5
6702 AA Wageningen
The Netherlands
Phone: +31 317 497676
Fax: +31 317 415955

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 06:55:04 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Michael,

A two-step detection method is indeed a good option to visualize your
biotinylated viral protein. Compared to the 2-step method the advantage
of a 1-step immunodetection method, as you initially suggested, will be
improved resolution. Your labeling density decreases however. As you
know labeling density is inversely related to the gold particle size.

Improved resolution combined with high sensitivity can be obtained when
using gold conjugates prepared with Ultra-Small gold particles. For
your application we would recommend Goat anti Biotin Ultra-Small. See
e.g. Müller-Höcker et al., (1998), Histochem. and Cell Biol. 109(2),
119-125.

When the protein of interest is located on the outside of the virus, in
other words the biotin is accessible for the antibodies, another option
may be the use of a pre-embedding labeling procedure. The use of
Ultra-Small gold conjugates is a prerequisite to successfully combine
appropriate labeling densities with a decent morphology. See e.g.
Decossas et al, (2003) J. of Comp. Neurology 462(3), 302-314 for
details on this technique.

Hope this is of help
Kind regards,
Peter

------------------------------------------
Michael Jarnik wrote:

Sorry, I would try to make it clearer. We need to localize a viral
protein which has been biotin-tagged and expressed in cell culture. I
expected it should be no problem to label it with Streptavidin
conjugate, but it is not that easy, it seems (even according to some
other people). So, as we do not have a good antibody to the viral
protein, I am considering an indirect labeling with anti-biotin
antibody and a secondary conjugate. There are tons of commercially
available anti-biotin antibodies, but certainly not all of them will
work with EM protocols - so I was interested whether somebody has
experience with some of these.

Thanks,

Michael

-----------
Peter van de Plas
Aurion
Costerweg 5
6702 AA Wageningen
The Netherlands
Phone: +31 317 497676
Fax: +31 317 415955

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 09:29:14 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rosscac-at-aol.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, May 13, 2004 at 07:52:40
---------------------------------------------------------------------------

Email: rosscac-at-aol.com
Name: Connie Cummings

Title-Subject: [Microscopy] [Filtered] Print processors

Question: I am interested in purchasing a print processor and was
wondering if anyone out there is using or has used either a Fujimoto
Roller Transport print processor CP51 or a JOBO printlab 3504 print
processor. I was looking for some feedback on these units on there
durablility and functionalitiy or any other tidbits! You can respond
back via email to me at rosscac-at-aol.com or at
connie.a.cummings-at-gsk.com.
Thanks in advance.
Connie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:01:17 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi fellow microscopists,

A post doc is trying to detect GFP being expressed in plant leaves. She is
fixing leaves in formaldehyde and doing a standard paraffin embedding. Her
question is if GFP going to survive xylene treatments for paraffin
infiltration. She plans to section the paraffin embedded blocks and look
for GFP using fluorescence microscopy.

If anyone has an answer please reply back to me.

Thanks in advance.

Soumitra

*************************************************************
Soumitra Ghoshroy
College Associate Professor, Biology
Director, Electron Microscopy Lab
Box 3EML
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office), 646-3283 (lab)
Fax: 505-646-3282
e-mail:sghoshro-at-nmsu.edu
http://www.cs.nmsu.edu/~biology/Faculty%20&%20Staff/Ghoshroy/Ghoshroy.htm
http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:16:44 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

hi all!

a simple question :

Does anyone have ever used graphite for sputtering or coating a SEM
sample ?

maybe a question from a dummy boy :-) , doesn't it?

thanx for answers...

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:35:04 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi all,
Lazy me recommended pre-coated SuperFrostPlus slides to Anne Dunn a
post-doc working on antlions but the gut goo doesn't always survive her
processing protocol (see her message below).

So the question is - What is the preferred slide coating method?
Gelatin vs poly-L-lysine...or something else?

advice and recipes would be greatly appreciated.
thanks,
Beth

} Hi Beth,
}
} I am finding that when I use the superfrost plus slides for
} my cryosections that often if there is material inside the
} gut that it will wash away as I am fixing and dehydrating
} my sections before hybridization (and I am not seeing any
} bacteria in the gut area after hybridization). I have no idea
} whether it is just something that is going to happen with
} a fluid-feeding insect, or if it is the superfrost slides not
} being sticky enough. I don't seem to be having a
} problem with the tissue itself sticking.
}
} I was looking up ways to coat slides and found there is
} the gelatin method and the poly-L-lysine method.
} Unfortunately I am not finding any info that tells me if one
} is better than the other. Do you have an opinion? I was
} wondering if it is a case of one coating being better for
} certain applications than another?
}
} I was going to go ahead and dissect out a gut or two, fix
} and hybridize them, trying to see if I can find any
} bacteria-like objects in the gut smooshate...to let me
} know if the loss of the material in the gut is an issue or
} not, but wanted to start thinking/plotting if I need to coat
} some slides.

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:52:50 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I'm looking for a shield to exclude air movement around the stage of my
Ultracut. I remember years ago having one for my Reichert OM-U3 but I
don't believe I got one for my Ultracut a few years ago. I've checked a
couple of the vendors and found nothing. I could find nothing at the
Leica site either. Does anyone have a source for these or will I have
to make my own?

Rick A. Harris, exDirector
Microscopy and Imaging Facility
Section of Molecular and Cellular Biology
1241 Life Sciences Addition
University of California
Davis, CA
530 752 2914
http://microscopy.mcb.ucdavis.edu
raharris-at-ucdavis.edu

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 11:41:29 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello Sharon,

Richard is of course right -- you can spend a fortune on LIMS systems and
for most users it may be overkill. On the other hand, the Excel sheets that
Richard mentions may be too limited.

A third option, somewhat in the middle, could be to use software that
supports or can read the images and other data from your software and keep
track of those in an archive or database. That way you can search for
keyfields, you deal with the same software for all applications, and you can
distribute the images easily. Our software analySIS includes such a
database. We also have a web frontend for this database so you can deal with
the global issues you mentioned.

Please take a look at our website or contact me directly if you wolud like
to get more information.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Richard Beanland [mailto:richard.beanland-at-bookham.com]
Sent: Thursday, May 13, 2004 02:14
To: 'Sharon_Goresh-at-engelhard.com'
Cc: 'Microscopy-at-MSA.Microscopy.Com'

Sharon,
it is possible to spend a lot of money on these systems. However, I
have yet to find one which offers significantly more than can be done with
MSExcel spreadsheets.

MSExcel spreadsheets on a server can be used in a 'shared' format, where
many people can open the same file without that irritating 'This file is
being used by...' error. In the system we have here, the files can only be
written to by a member of the analysis group, but read by anyone. People
have to come here to give us a sample anyway, so this is not a problem.
Each sample gets a line in the spreadsheet with the usual fields (date,
name, analysis needed etc.). When someone is working on a job, they put
their initials in the box for that analysis type; when the job is done, a
date goes in the box instead. The spreadsheet is updated every time someone
saves it. Each column has an 'Autofilter' at the top which means they can
be searched for any of the fields.
This 'master' spreadsheet contains hyperlinks to the electronic log books
for each microscope or technique (also shared MSExcel spreadsheets). These
are updated as the analysis happens, and here each image has a line giving
sample, analysis details, operator, customer, etc.. Each line in these
'technique' spreadsheets has a hyperlink to the data file. Again, each
column has an 'Autofilter' at the top which means they can be searched for
any of the fields.

As a user, it is easy to operate (that 'fill down' feature of Excel allows
you to copy the provious line and change one box without having to make 10
entries for each image). The only discipline needed is to keep saving the
files frequently (autosaving doesn't work, if two computers try to save at
the same time they can lock up). Our customers seem to be happy too - they
know the status of their job and can find the data without having to hassle
us. We rely on the standard software on each user's PC to be able to open
the images.

I'm not sure how this could be implemented on a web-based system, but for a
server it works very well. We keep track of about 4000 samples a year - and
all the data files they generate - with this system, and it usually only
takes a few minutes to find old data even from a vague description. I have
yet another spreadsheet which allows me to count how many jobs have been
done, are left to do, etc., for each analysis type. The nice thing about
spreadsheets is that they are totally 'customizable', so you only keep track
of what you think is important.

I'd be happy to send you an example of the files if you like. As a 'free'
solution it is hard to beat!

Cheers

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com
All incoming mail is filtered for spam. If you do not receive a reply from
me, do not assume I have received your mail.

-----Original Message-----
} From: Sharon_Goresh-at-engelhard.com [mailto:Sharon_Goresh-at-engelhard.com]
Sent: 12 May 2004 19:20
To: Microscopy-at-MSA.Microscopy.Com

Fellow Microscopists,

The Microscopy Lab in our Research Center has 3 SEM's, 1 TEM and 1 EMPA
(with a second due in November) in addition to 4 XRD instruments. Our
main function has been as a problem solving facility to our researchers as
well as our field service engineers. Data produced by our lab is usually
issued as reports with images, spectra and graphs as attachments.
Management has directed us to implement a LIMS by the end of the year.
Their requirements include the ability of the researchers and field service
engineers to log samples in from their locations and the tracking of the
sample from the arrival in our lab to the issuance of data. It must also
be able to archive the data as well. For us this means literally hundreds
of images, spectra and reports each month that must be categorized and
saved. The researchers and engineers must also be able to access the data
from their location. This will probably mean a web based system since our
facilities cover the globe.

Has anyone out there been faced with a similar request? Our main hurdle is
convincing management that ours is not a "sample in - number out" type of
lab, and that most LIMS packages out there are designed for that type of
simple operation. If you have implemented such a system, was it an off the
shelf package, a custom designed package or a combination? If you want to
respond to me directly that would be fine. I am not interested in "system
bashing" just some helpful suggestions on how to make management happy
without losing my sanity.

Sharon Goresh
Chemist
sharon.goresh-at-engelhard.com

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From MicroscopyL-request-at-ns.microscopy.com Thu May 13 12:27:22 2004

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Hi Beth,

We use silane to coat our slides, it is the standard for the histology labs in the pathology dept.

Silane = 3-aminopropyl-triethoxy-silane

Protocol:

Silane 20 ml
Actenoe 2000 ml

Dip precleaned slides in Silane solution for 2 minutes
Drain and wash in distilled water 2 times
Drain and dry at 60 degrees C for 1 hour
Store away from light and moisture.

Our sildes last for many months (6+), we make huge batches at a time.

I hope this helps you out of your sticky situation!

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax

} } } Beth Richardson {beth-at-plantbio.uga.edu} 05/13/04 11:38AM } } }

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi all,
Lazy me recommended pre-coated SuperFrostPlus slides to Anne Dunn a
post-doc working on antlions but the gut goo doesn't always survive her
processing protocol (see her message below).

So the question is - What is the preferred slide coating method?
Gelatin vs poly-L-lysine...or something else?

advice and recipes would be greatly appreciated.
thanks,
Beth

} Hi Beth,
}
} I am finding that when I use the superfrost plus slides for
} my cryosections that often if there is material inside the
} gut that it will wash away as I am fixing and dehydrating
} my sections before hybridization (and I am not seeing any
} bacteria in the gut area after hybridization). I have no idea
} whether it is just something that is going to happen with
} a fluid-feeding insect, or if it is the superfrost slides not
} being sticky enough. I don't seem to be having a
} problem with the tissue itself sticking.
}
} I was looking up ways to coat slides and found there is
} the gelatin method and the poly-L-lysine method.
} Unfortunately I am not finding any info that tells me if one
} is better than the other. Do you have an opinion? I was
} wondering if it is a case of one coating being better for
} certain applications than another?
}
} I was going to go ahead and dissect out a gut or two, fix
} and hybridize them, trying to see if I can find any
} bacteria-like objects in the gut smooshate...to let me
} know if the loss of the material in the gut is an issue or
} not, but wanted to start thinking/plotting if I need to coat
} some slides.

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 13:19:34 2004

Contents Retrieved from Microscopy Listserver Archives
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I am going to buy scanner for TEM negatives and considering two models:
Microtek ArtixScan 1800f and Epson Expression 1680 Pro. Any advise and
comments are very welcome.

Thank you in advance,

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 13:39:06 2004

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Hello,

I am looking for a replacement glass spacer for a Polaron E5100 series
II 'Cool' Sputter Coater. The external diameter etched on metal collar
base is 165.1 m/m. The internal diameter of the metal collar is 5.75".
The height of the glass spacer is 3 and 3/16". I have been working with
EBS to locate a replacement collar but would like to know if there are
any other sources I could contact.

Thank you in advance for your help

aruna

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 15:30:40 2004

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Dear Sylvain,
I use graphite, evaporated in a high-vacuum evaporator, to make SEM samples
conductive when I want to do EDS analysis. I use gold/palladium for SEM imaging
without analysis, but carbon coating to minimize any interference of the coating
with the EDS analysis.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "sylvain maury" {sylvain.maury-at-thalesgroup.com}
To: "Microscopy community" {microscopy-at-msa.microscopy.com}
Sent: Thursday, May 13, 2004 8:22 AM

} I'm looking for a shield to exclude air movement around the stage of my
} Ultracut. I remember years ago having one for my Reichert OM-U3 but I
} don't believe I got one for my Ultracut a few years ago. I've checked a
} couple of the vendors and found nothing. I could find nothing at the
} Leica site either. Does anyone have a source for these or will I have
} to make my own?
}
} Rick A. Harris, exDirector
} Microscopy and Imaging Facility
} Section of Molecular and Cellular Biology
} 1241 Life Sciences Addition
} University of California
} Davis, CA
} 530 752 2914
} http://microscopy.mcb.ucdavis.edu
} raharris-at-ucdavis.edu

Rick -

Make a hole in the bottom of a plastic veggie bag from your
supermarket & rubber-band it around the binocular objective. Ugly,
but it works better than a rigid plastic box.

Caroline
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 16:09:34 2004

Contents Retrieved from Microscopy Listserver Archives
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Short and sweet: about a year ago we bought a Microtek ArtixScan 2500f (firewire); a little different from the 1800f but I don't know how much. Anyway, we like it. Great dynamic range and reasonable software (we scan into a G4 Mac running OSX).

cheers, John

********
John S. Vetrano
Sr. Research Scientist
Materials Structure and Performance Group
Pacific Northwest National Laboratory
MSIN P8-16
P.O. Box 999
Richland, WA 99352
Phone: (509)372-0724 Fax: (509)376-6308
Email: mailto:john.vetrano-at-pnl.gov

} ----------
} From: Dusevich, Vladimir
} Sent: Thursday, May 13, 2004 11:25 AM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy]
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I am going to buy scanner for TEM negatives and considering two models:
} Microtek ArtixScan 1800f and Epson Expression 1680 Pro. Any advise and
} comments are very welcome.
}
} Thank you in advance,
}
} Vladimir
}
} Vladimir M. Dusevich, Ph.D.
} Electron Microscope Lab Manager
} 3127 School of Dentistry
} 650 E. 25th Street
} Kansas City, MO 64108-2784
}
} Phone: (816) 235-2072
} Fax: (816) 235-5524
} Web: http://www.umkc.edu/dentistry/microscopy
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 16:33:19 2004

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Hi,
I would like to have an evaluation of the Denton Desk III TSC sputter
coater from those who are using or have used this instrument for preparation
of samples for FESEM imaging. Please direct your response to me rather than
to the list.

Many thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 18:42:36 2004

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I don't use C. I use Au/Pd and Pt. C is
too messy.

Depending on what you are looking at, either
image- or EDS/WDS-wise, your options may vary.
For EDS, I just ignore the small Au/Pd peaks.
The coating is only 40-60A and is typically
only seen as piled up Au with Al, Si and W.
With my specimens, Pd is by itself.

I suppose that if you were looking at P or Zr
specimens, Au/Pd or Pt would be a problem. Perhaps
the ultimate coating is Os. Someday, I would love
to try one of these coaters. It ought to be
great for EBSD.

But let us know what type of work you are trying
to do. That may make a big difference in coating
strategies.

gary g.

At 08:22 AM 5/13/2004, you wrote:

} hi all!
}
} a simple question :
}
} Does anyone have ever used graphite for sputtering or coating a SEM
} sample ?
}
} maybe a question from a dummy boy :-) , doesn't it?
}
} thanx for answers...
}
} Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 20:43:29 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I don't use C. I use Au/Pd and Pt. C is
too messy.

Depending on what you are looking at, either
image- or EDS/WDS-wise, your options may vary.
For EDS, I just ignore the small Au/Pd peaks.
The coating is only 40-60A and is typically
only seen as piled up Au with Al, Si and W.
With my specimens, Pd is by itself.

I suppose that if you were looking at P or Zr
specimens, Au/Pd or Pt would be a problem. Perhaps
the ultimate coating is Os. Someday, I would love
to try one of these coaters. It ought to be
great for EBSD.

But let us know what type of work you are trying
to do. That may make a big difference in coating
strategies.

gary g.

At 08:22 AM 5/13/2004, you wrote:

} hi all!
}
} a simple question :
}
} Does anyone have ever used graphite for sputtering or coating a SEM
} sample ?
}
} maybe a question from a dummy boy :-) , doesn't it?
}
} thanx for answers...
}
} Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 08:16:15 2004

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I have an earlier model of the Epson (the 1600 Pro) and I"ve been
happy with it.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 09:44:02 2004

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Someone recently posed the same question on ListServer. We have an Epson
Perfection 3200 Photo and love it. There is no holder for the standard 3 1/4 X
4 negatives, but I just put them directly on the glass and they come out fine.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Dusevich, Vladimir [mailto:DusevichV-at-umkc.edu]
Sent: Thursday, May 13, 2004 2:26 PM
To: microscopy-at-msa.microscopy.com

I am going to buy scanner for TEM negatives and considering two models:
Microtek ArtixScan 1800f and Epson Expression 1680 Pro. Any advise and
comments are very welcome.

Thank you in advance,

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 15:04:09 2004

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Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 16:30:39 2004

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What is the cross sectional construction like?
Is the die passivated? If it is, use MIL-STD-883 for
GLIT. If there is metal underneath the passivation,
and the passivation has voids, GLIT will show it
up big time. GLIT is glassivation layer integrity test.

gary g.

At 01:10 PM 5/14/2004, you wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Fri May 14 17:47:07 2004

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Dear Pavel: my first thought is, don't coat the device. Find an
accelerating voltage/tilt angle combination that will prevent of
minimize charging. Next thought, coat with something besides gold. But
I've done a lot of cracked devices and have never had any problems
telling the cracks from the original surface. Unless they are huge
cracks, the gold won't get in them to confuse the issue. Are these
surface cracks or cracks going down into the surface?

AtcSEM wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Sat May 15 00:47:25 2004

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------------------------------------------------------------------------
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------------------------
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LAMBS, Department of Physics, University of Genoa, June 14-16, 2004.

The use and application of fluorescence techniques is increasing daily
both in the academia and in industry. The Principles of Fluorescence
Techniques course will outline the basic concepts of fluorescence
techniques and the successful utilization of the currently available
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The course is designed for students who utilize fluorescence
instrumentation and techniques, as well as for researchers
and industrial scientists who intend to deepen their knowledge of
fluorescence techniques. The theoretical lectures delivered by key
scientists in the field are complemented by the direct utilization of
steady state and lifetime fluorescence instrumentation provided by
leading companies.

It is recommended that participants have at least a bachelor's degree
in the life science, physical sciences or engineering before attending
this course. Topics addressed in this course include:

Basic Definitions and Principles of Fluorescence
Fluorescence Polarization
Time- resolved Fluorescence
Instrumentation

Data Manipulation and Data Analysis
Fiber Optic Sensors
Confocal Fluorescence Microscopy
Lifetime Imaging
Fluorescence Correlation Spectroscopy
Multiphoton excitation microscopy and spectroscopy
Quantum dots

The Principles of Fluorescence Techniques course will be held at:

Laboratory for Advanced Microscopy, Bioimaging and Spectroscopy
Diaspro lab, Research Center MICROSCOBIO
Department of Physics, University of Genoa
via Dodecaneso, 33
16146 Genova, Italy

Details: www.lambs.it; diaspro-at-fisica.unige.it

The number of participants to the Principles of Fluorescence Techniques
Course

is limited to 40 people. PLEASE RESERVE YOUR PARTICIPATION AS SOON AS
POSSIBLE SENDING AN E-MAIL TO: coordinator-at-fluorescence-foundation.org.

Details : www.fluorescence-foundation.org
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---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 16 13:24:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (zr zrzhang_xrli-at-ybb.ne.jp) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, May 15, 2004 at 21:16:24
---------------------------------------------------------------------------

Email: zr zrzhang_xrli-at-ybb.ne.jp
Name: Zheng-Rong Zhang

Organization: Yokohama National University

Education: Graduate College

Location: Yokohama, Japan

Question: Dear Microscopist,

I need to prepare TEM samples from Ag and Ag-Pd(10pct) alloy sheets. May you suggest me any electrolytes for twin-jet electropolishing and the corresponding conditions? No toxic chemicals would be used.

Thank you in advance!

With best regards

Zheng-Rong Zhang

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 16 13:44:10 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jtrynak-at-SciGenium.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 12, 2004 at 18:22:09
---------------------------------------------------------------------------

Email: jtrynak-at-SciGenium.com
Name: JT Rynak

Organization: SciGenium

Title-Subject: [Microscopy] [Filtered] Opening - New England Regional - Imaging Sales

Question: New England Regional - Imaging Sales

5+ years experience selling imaging / visualization capital equipment into Research Market space. Ideal person will have a rolodex of PI and Lead Vivo research scientists. BS/MS is Biology or Zoology

If you have any further questions feel free to contact me at 617-661-1067 or via email at jtrynak-at-scigenium.com

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 16 18:53:06 2004

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Pavel;

Having looked at more fractures in silicon and GaAs devices than I care to remember, it's not generally a problem finding them and as often with optical means as with EM.

If you would kindly provide the list with more specifics about your samples and the nature of these "cracks?" That is, are they along crystal planes or fractures that travel at random angles with respect to the surface? Fractures, or cleaves perpendicular to the die surface, are difficult to detect with EM but apparent with visible light microscopy. How separated are both sides of the crack and why do you need to see into them? Sounds like you only need to identify whether they exist or not. How long are the cracks?

I have plenty of EM's I'd be happy to send you images of samples that have fractured for various reasons, and there are multiple root causes of this failure mechanism. I'm sure if you provide a little more detail you'll get plenty of good suggestions on how to image your samples.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Friday, May 14, 2004 4:10 PM
To: MicroscopyListServer (MicroscopyListServer)

Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Sun May 16 19:26:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Any course that will promote even the correct spelling of
fluorescence has to be a good thing.

Maybe someone will run one on how to spell 'JEOL' someday.

:)

cheers

rtch

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 00:12:47 2004

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Hello listers,

We are in the process of justifying, to the University, a proposal to
purchase an ESEM. In prepapring the business case I am including the
ten year financials for both FEG and Tungtsen filament machines. Given
that we have to break even in that time, including covering our
depreciation, the Tungsten instrument is easier to justify in a purely
financial sense.

From a scientific and operational viewpoint, though, I was hoping some
of you could provide opinions on the relative merits of Tungsten or FEG.
Our current conventional SEM is a Philips XL-30 S-FEG so we already know
of the costs associated with the emitter.

The range of samples we will be required to put in our ESEM will be
anything you oculd possibly imagine from the Faculties of Engineering,
Science and Medicine. Samples will inlcude food materials (big dairy
industry in New Zealand), polymers, conducting polymers, mammalian
tissue, bacteria, fruit and veg, fish and chips, superconductors,
ceramic coatings and bees knees. We will definitely need a hot-stage.

If you would like to contact me off list with your opinions please feel
free.

Kind regards
Bryony James
Research Centre for Surface and Materials Science
Univetrsity of Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 07:57:52 2004

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Thank you all for the responses that I have received.

Just to clarify:
We had multiple field failures of the chips. The SEM examination
revealed some sort of coating on the fracture surfaces, which I believe is
the urethane coating. The transition from the side wall to the fracture
surface, on some of the chips, suggests that the chips could have had a
small cracks prior urethane coating.

Now, I am looking at the "Virgin" chips for any evidence of cracking
at the side wall and diaphragm transition, but my problem is that the Gold
coating does not coat the area well enough for me to resolve the crack. Due
to lack of coating that area is charging and I see only a black line.
I have coated it at least 3 times and rotate the chips to insure good
coatings in those areas, but it was not enough.

After SEM examination I would also like to cross section the chip to check
for the evidence of pre-cracks, but I am afraid to introduce the cracks
myself. Could you help me with a proper preparation procedure of the cross
sections? We have metallography lab. equipment and nothing special to
prepare the chip cross sections.

I have uploaded some more photos of the fracture surfaces of the failed
chips and Virgin chip that I am trying to image now.
http://www.atclabs.com/images/temp/MicrList_files/frame.htm

Sorry, it might be a little slow at showing the images due to their size.

Thanks for your help again,

Pavel

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]

What is the cross sectional construction like?
Is the die passivated? If it is, use MIL-STD-883 for
GLIT. If there is metal underneath the passivation,
and the passivation has voids, GLIT will show it
up big time. GLIT is glassivation layer integrity test.

gary g.

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]

Do you get charging at the crack due to a gap in the coating?
Otherwise,you should be able to see the break.

-----Original Message-----
} From: Jim Quinn [mailto:jquinn-at-www.matscieng.sunysb.edu]
Pavel

Your image is very low mag, so it is difficult to judge anything.

I suggest that you use a sacrificial chip and coat
it with about 10nm of gold. If your coater does not
rotate the sample, then you should manually rotate
the sample at 45 degrees atleast twice. This is
will help the gold to get into the perpendicular
surfaces.

Next use a Robinson BS detector. 10 or 15kV is sufficient.

Once you image the cracks, then you can go about
trying to image without the gold. Variable pressure
and voltage will reduce charging in uncoated samples.

JQ

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Pavel;

Having looked at more fractures in silicon and GaAs devices than I
care to remember, it's not generally a problem finding them and as
often with optical means as with EM.

If you would kindly provide the list with more specifics about your
samples and the nature of these "cracks?" That is, are they along
crystal planes or fractures that travel at random angles with respect to
the surface? Fractures, or cleaves perpendicular to the die surface, are
difficult to detect with EM but apparent with visible light microscopy.
How separated are both sides of the crack and why do you need to see into
them? Sounds like you only need to identify whether they exist or not.
How long are the cracks?

I have plenty of EM's I'd be happy to send you images of samples
that have fractured for various reasons, and there are multiple root
causes of this failure mechanism. I'm sure if you provide a little more
detail you'll get plenty of good suggestions on how to image your
samples.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Friday, May 14, 2004 4:10 PM
To: MicroscopyListServer (MicroscopyListServer)

Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 09:11:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Thank you so much for all of your advice. I received a large number of
great suggestions and almost everyone suggested using anti GFP antibody
and we are certainly going to go that route.

Thanks again and this is truly a great resource.

Best wishes,

Soumitra

*************************************************************
Soumitra Ghoshroy
College Associate Professor, Biology
Director, Electron Microscopy Lab
Box 3EML
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office), 646-3283 (lab)
Fax: 505-646-3282
e-mail:sghoshro-at-nmsu.edu
http://www.cs.nmsu.edu/~biology/Faculty%20&%20Staff/Ghoshroy/Ghoshroy.htm
http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 11:36:59 2004

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I think I can offer a few ideas and questions.

1) Can you say "stress concentration"? My academic background is in
Engineering Science and Mechanics. It looks like you have some very sharp
corners where the diaphragm meets the substrate. That is trouble waiting to
happen. I cannot tell if there is any pre-crack there. There might be hints
of one in slide 43. Either way, that geometry is going to lead to problems.
The stresses will be highest at the edges of the diaphragm. I think you
would prefer a gradual change in geometry there to avoid any concentration
and to help reinforce the edges. I don't know the fabrication process, and
it might be hard to implement, but it might be worth investigating.

Slides 38 and 42 show some jagged surfaces. I guess those are the edges of
the substrate and the diaphragm is on the bottom. If so, the nose of the
jaggie jutting out further into the opening will be a point of stress
concentration.

You may also want to consider round openings in the substrate. The corners
of the square holes don't help and might hurt. The highest stresses should
be in the middle of the edges.

2) You haven't said how prematurely these chips failed. Are they subjected
to a cyclic load? What fraction of their design load were they subjected
to? There may be hints of fatigue failure (slide 34?), but it seems to be
rather short cycle fatigue if it is fatigue at all. I have seen glass break
with such fractures in overload.

3) Slides 37, 40 and 41 show dark corners. I think that is the normal
appearance for an interior corner in secondary mode. An exterior corner
tends to show up bright in SE mode.

4) I can't quite tell where many of the photos were taken (e.g., slides 13
and 39). I usually use a three-fold step in magnification to easily follow
from one view to another. Also, the progressions 10, 30, 100, 300 or 15,
50, 150, 500 are easy to remember and to standardize on.

5) Did you copy these images into Powerpoint to make this presentation? My
computer took quite a while to load each slide, and I have a fast
connection. We routinely record our SEM images at 1024-pixels across and
store the files as JPGs. (Keep reading for the rationale.) Those files are
maybe 300 KB in size. If I use the Insert, Image, From_file function to add
the image to my document, it retains the JPG compression and gray nature
and requires only 300 KB. But, if I open those files in an imaging program
and copy them over they expand. The computer has the image rendered as a
bitmap in full color, the image gets copied with no compression and it now
consumes 2400 kB (1024x768 pixels times 3-bytes-per-pixel). That 8-fold
difference in size is noticeable. I know more and more users have broadband
connections; however these order-of-magnitude expansions start to add up. {g}

Hope this helps.

Warren

At 08:06 AM 5/17/2004, you wrote:

} Thank you all for the responses that I have received.
}
} Just to clarify:
} We had multiple field failures of the chips. The SEM
} examination
} revealed some sort of coating on the fracture surfaces, which I believe is
} the urethane coating. The transition from the side wall to the fracture
} surface, on some of the chips, suggests that the chips could have had a
} small cracks prior urethane coating.
}
} Now, I am looking at the "Virgin" chips for any evidence of cracking
} at the side wall and diaphragm transition, but my problem is that the Gold
} coating does not coat the area well enough for me to resolve the crack. Due
} to lack of coating that area is charging and I see only a black line.
} I have coated it at least 3 times and rotate the chips to insure good
} coatings in those areas, but it was not enough.
}
} After SEM examination I would also like to cross section the chip to check
} for the evidence of pre-cracks, but I am afraid to introduce the cracks
} myself. Could you help me with a proper preparation procedure of the cross
} sections? We have metallography lab. equipment and nothing special to
} prepare the chip cross sections.
}
} I have uploaded some more photos of the fracture surfaces of the failed
} chips and Virgin chip that I am trying to image now.
} http://www.atclabs.com/images/temp/MicrList_files/frame.htm
}
} Sorry, it might be a little slow at showing the images due to their size.
}
} Thanks for your help again,
}
} Pavel

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 11:44:19 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We look mostly at hydrated biological samples. We have a
tungsten gun XL30 ESEM TMP. For looking at bacteria and
cells a FEGESEM would be superior in terms of reduced
damage and improved resolution. I find it hard to get
medium/high resolution with wet biological samples. I feel
FEGESEM would make this a lot easier.

Dave

On Mon, 17 May 2004 17:21:33 +1200 Bryony James
{b.james-at-auckland.ac.nz} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hello listers,
}
} We are in the process of justifying, to the University, a proposal to
} purchase an ESEM. In prepapring the business case I am including the
} ten year financials for both FEG and Tungtsen filament machines. Given
} that we have to break even in that time, including covering our
} depreciation, the Tungsten instrument is easier to justify in a purely
} financial sense.
}
} From a scientific and operational viewpoint, though, I was hoping some
} of you could provide opinions on the relative merits of Tungsten or FEG.
} Our current conventional SEM is a Philips XL-30 S-FEG so we already know
} of the costs associated with the emitter.
}
} The range of samples we will be required to put in our ESEM will be
} anything you oculd possibly imagine from the Faculties of Engineering,
} Science and Medicine. Samples will inlcude food materials (big dairy
} industry in New Zealand), polymers, conducting polymers, mammalian
} tissue, bacteria, fruit and veg, fish and chips, superconductors,
} ceramic coatings and bees knees. We will definitely need a hot-stage.
}
} If you would like to contact me off list with your opinions please feel
} free.
}
} Kind regards
} Bryony James
} Research Centre for Surface and Materials Science
} Univetrsity of Auckland
} New Zealand
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 13:37:31 2004

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We are an independent commercial lab serving general industry. Unless
directed by a court order or we suspect misuse of our findings, all
information is strictly confidential to our client.

We have a situation with a small project we just completed. We detected the
presence of a toxic compound in product. While not the intended use, it is
conceivable that this product could be put into one's mouth which would
present a health concern.

Upon discovery of this compound, I called our client immediately and found
out that they submitted competitors' products. Our client is certainly
aware of this now, but they are not in a position to disclose to their
competitors that they were analyzing their products. Given that these
products are not intended to have oral contact, I doubt that the FDA has
any applicable regulations regarding the composition.

Any thoughts?

Alan Stone
ASTON Metallurgical Services

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 16:10:25 2004

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Dear Bryony,
The combined FE and ESED instruments are very pricey, expensive to maintain and,
since you already have a FE, perhaps a bit redundant. We have a two-year-old
tungsten variable-pressure and it is a popular workhorse that is in constant
use. It can do high resolution or ESED but not both at the same time. If you
need both at the same time, then you need FE-ESED. BTW, the thing we would most
like to have is a cold stage, to look at hydrated samples without having to go
to higher pressures.
Good luck.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Bryony James" {b.james-at-auckland.ac.nz}
To: {Microscopy-at-msa.microscopy.com}
Sent: Sunday, May 16, 2004 10:21 PM

Alan;

It sounds like you need legal advice and not scientific advice. You should consult with your corporate counsel on this issue.

Competitor analysis is done all the time and I don't see any issues with that. What you do with the data afterwards may be another matter and open to litigation so see the attorney.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: Alan Stone [mailto:as-at-astonmet.com]
Sent: Monday, May 17, 2004 2:47 PM
To: Microscopy-at-MSA.Microscopy.Com

We are an independent commercial lab serving general industry. Unless
directed by a court order or we suspect misuse of our findings, all
information is strictly confidential to our client.

We have a situation with a small project we just completed. We detected the
presence of a toxic compound in product. While not the intended use, it is
conceivable that this product could be put into one's mouth which would
present a health concern.

Upon discovery of this compound, I called our client immediately and found
out that they submitted competitors' products. Our client is certainly
aware of this now, but they are not in a position to disclose to their
competitors that they were analyzing their products. Given that these
products are not intended to have oral contact, I doubt that the FDA has
any applicable regulations regarding the composition.

Any thoughts?

Alan Stone
ASTON Metallurgical Services

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 07:02:20 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Pavel;

If you really need a x-section without the issues with mechanical polishing, try using an FIB [Focused Ion Beam].

Peter

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Monday, May 17, 2004 9:07 AM
To: MicroscopyListServer (MicroscopyListServer)

Thank you all for the responses that I have received.

Just to clarify:
We had multiple field failures of the chips. The SEM examination
revealed some sort of coating on the fracture surfaces, which I believe is
the urethane coating. The transition from the side wall to the fracture
surface, on some of the chips, suggests that the chips could have had a
small cracks prior urethane coating.

Now, I am looking at the "Virgin" chips for any evidence of cracking
at the side wall and diaphragm transition, but my problem is that the Gold
coating does not coat the area well enough for me to resolve the crack. Due
to lack of coating that area is charging and I see only a black line.
I have coated it at least 3 times and rotate the chips to insure good
coatings in those areas, but it was not enough.

After SEM examination I would also like to cross section the chip to check
for the evidence of pre-cracks, but I am afraid to introduce the cracks
myself. Could you help me with a proper preparation procedure of the cross
sections? We have metallography lab. equipment and nothing special to
prepare the chip cross sections.

I have uploaded some more photos of the fracture surfaces of the failed
chips and Virgin chip that I am trying to image now.
http://www.atclabs.com/images/temp/MicrList_files/frame.htm

Sorry, it might be a little slow at showing the images due to their size.

Thanks for your help again,

Pavel

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]

What is the cross sectional construction like?
Is the die passivated? If it is, use MIL-STD-883 for
GLIT. If there is metal underneath the passivation,
and the passivation has voids, GLIT will show it
up big time. GLIT is glassivation layer integrity test.

gary g.

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]

Do you get charging at the crack due to a gap in the coating?
Otherwise,you should be able to see the break.

-----Original Message-----
} From: Jim Quinn [mailto:jquinn-at-www.matscieng.sunysb.edu]
Pavel

Your image is very low mag, so it is difficult to judge anything.

I suggest that you use a sacrificial chip and coat
it with about 10nm of gold. If your coater does not
rotate the sample, then you should manually rotate
the sample at 45 degrees atleast twice. This is
will help the gold to get into the perpendicular
surfaces.

Next use a Robinson BS detector. 10 or 15kV is sufficient.

Once you image the cracks, then you can go about
trying to image without the gold. Variable pressure
and voltage will reduce charging in uncoated samples.

JQ

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Pavel;

Having looked at more fractures in silicon and GaAs devices than I
care to remember, it's not generally a problem finding them and as
often with optical means as with EM.

If you would kindly provide the list with more specifics about your
samples and the nature of these "cracks?" That is, are they along
crystal planes or fractures that travel at random angles with respect to
the surface? Fractures, or cleaves perpendicular to the die surface, are
difficult to detect with EM but apparent with visible light microscopy.
How separated are both sides of the crack and why do you need to see into
them? Sounds like you only need to identify whether they exist or not.
How long are the cracks?

I have plenty of EM's I'd be happy to send you images of samples
that have fractured for various reasons, and there are multiple root
causes of this failure mechanism. I'm sure if you provide a little more
detail you'll get plenty of good suggestions on how to image your
samples.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Friday, May 14, 2004 4:10 PM
To: MicroscopyListServer (MicroscopyListServer)

Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 07:15:34 2004

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Hello,
We want to image, by SEM, the surface of a HfO2 layer deposited on Si.
Is there a method to reveal the structure of the layer ?
for instance chemical etching or others....
We have tried on the as grown layer but we can see nothing, the image is
very smooth. By means of X-ray diffraction we know that
we have very small crystals, just a few nanometers. Now we wonder wether
there are larger structures than the crystals. We expect
something like polycrystalline grains...
Thank you for your help
Regards

--
Claude GRATTEPAIN / Bernard SERVET

THALES R & T France Tel : (+33 1) 69.33.91.13
Domaine de Corbeville Fax : (+33 1) 69.33.07.40

91404 Orsay Cedex, France mailto:claude.grattepain-at-thalesgroup.com
_____________________________________________________________________

"The information contained in this e-mail and any attachments are the
property of THALES and may be confidential. If you are not the
intended
recipient, please notify us immediately, send this message back to us
and
destroy it. You are hereby notified that any review, dissemination,
distribution, copying or otherwise use of this e-mail/fax is strictly
prohibited.

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:17:11 2004

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Dear All

We would like to get a centrifuge to separate viruses. What are you using in your TEM laboratory?
Suggestions and hints will be helpful.
Thanks

Since my UB mail address is not reliable please send
a copy of all urgent mail to

coetzeesh-at-yahoo.co.uk

Mr S. H. Coetzee
Electron Microscope Unit
University of Botswana
Private Bag 0022
Gaborone
Botswana
Phone : +267 355 2462/5222
Mobile : +267 714 55701 (Now active)
Fax : +267 318 5097
e-mail : coetzees-at-mopipi.ub.bw

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:46:08 2004

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Hello Listers,

I wanted to see if anyone has had any experience scanning negatives with the Canon Canoscan 9900F.
I have a low end Canoscan that I use for documents and the occasional photograph, which has given me
very good results, but is not set up for negatives. I have seen the recent posts about the Epson scanner,
but I am trying to keep it under a $1000 so that I do not have to treat it as a capital purchase. I have tried
for the last two years to get a Coolscan 8000 on the capital budget with no luck, and do not see any scanner
above $1000 as an option right now.

Thanks,
Steve

Steven Lee
Chief Technologists
Electron Microscopy Laboratory
Baylor University Medical Center
3500 Gaston Ave
Dallas, TX 750246
Ph: 214.820.3302
Fx: 214.820.4110
Em: stevenle-at-baylorhealth.edu

This e-mail, facsimile, or letter and any files or attachments transmitted with it contains information that is confidential and privileged. This information is intended only for the use of the individual(s) and entity(ies) to whom it is addressed. If you are the intended recipient, further disclosures are prohibited without proper authorization. If you are not the intended recipient, any disclosure, copying, printing, or use of this information is strictly prohibited and possibly a violation of federal or state law and regulations. If you have received this information in error, please notify Baylor Health Care System immediately at 1-866-402-1661 or via e-mail at privacy-at-baylorhealth.edu. Baylor Health Care System, its subsidiaries, and affiliates hereby claim all applicable privileges related to this information.

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:47:42 2004

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In my experience medium/high magnifications for wet
specimens are limited mostly by specimens themselves and not by a
type of emitter. While I can get a nice picture of gold on carbon
at x100k, for most of my "real life" specimens magnification is
limited by x20k (or less).

Vladimir

} We look mostly at hydrated biological samples. We have a
} tungsten gun XL30 ESEM TMP. For looking at bacteria and
} cells a FEGESEM would be superior in terms of reduced
} damage and improved resolution. I find it hard to get
} medium/high resolution with wet biological samples. I feel
} FEGESEM would make this a lot easier.
}
} Dave
}
} On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} {b.james-at-auckland.ac.nz} wrote:
}
} }
} }
} }
} ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} -----------------
} }
} } Hello listers,
} }
} } We are in the process of justifying, to the University, a
} proposal to
} } purchase an ESEM. In prepapring the business case I am
} including the
} } ten year financials for both FEG and Tungtsen filament
} machines. Given
} } that we have to break even in that time, including covering our
} } depreciation, the Tungsten instrument is easier to justify
} in a purely
} } financial sense.
} }
} } From a scientific and operational viewpoint, though, I was hoping
} } some
} } of you could provide opinions on the relative merits of
} Tungsten or FEG.
} } Our current conventional SEM is a Philips XL-30 S-FEG so we
} already know
} } of the costs associated with the emitter.
} }
} } The range of samples we will be required to put in our ESEM will be
} } anything you oculd possibly imagine from the Faculties of
} Engineering,
} } Science and Medicine. Samples will inlcude food materials
} (big dairy
} } industry in New Zealand), polymers, conducting polymers, mammalian
} } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } ceramic coatings and bees knees. We will definitely need a
} hot-stage.
} }
} } If you would like to contact me off list with your opinions please
} } feel
} } free.
} }
} } Kind regards
} } Bryony James
} } Research Centre for Surface and Materials Science
} } Univetrsity of Auckland
} } New Zealand
} }
} }
} }
} } This incoming email to UWE has been independently scanned
} for viruses
} } and any virus detected has been removed using McAfee anti-virus
} } software
} }
}
} ----------------------------------------
} Patton, David
} Email: David.Patton-at-uwe.ac.uk
} "University of the West of England"
}
}
}
} This email has been independently scanned for viruses and any
} virus detected has been removed using McAfee anti-virus software
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:51:20 2004

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Try EBSD. It will tell if you have grains
or if the layer is amorphous.

gary g.

At 05:24 AM 5/18/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 09:16:24 2004

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Depressing isn't it? I usually give up with cultured
cells and look at them after drying with HMDS and gold
coating. Have you (or anyone out there) ever taken/seen a
good picture of a hydrated cultured cell at x20,000 or
higher?

Dave

On Tue, 18 May 2004 08:55:19 -0500 "Dusevich, Vladimir"
{DusevichV-at-umkc.edu} wrote:

} In my experience medium/high magnifications for wet
} specimens are limited mostly by specimens themselves and not by a
} type of emitter. While I can get a nice picture of gold on carbon
} at x100k, for most of my "real life" specimens magnification is
} limited by x20k (or less).
}
} Vladimir
}
} } We look mostly at hydrated biological samples. We have a
} } tungsten gun XL30 ESEM TMP. For looking at bacteria and
} } cells a FEGESEM would be superior in terms of reduced
} } damage and improved resolution. I find it hard to get
} } medium/high resolution with wet biological samples. I feel
} } FEGESEM would make this a lot easier.
} }
} } Dave
} }
} } On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} } {b.james-at-auckland.ac.nz} wrote:
} }
} } }
} } }
} } }
} } ----------------------------------------------------------------------
} } } --------
} } } The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America
} } } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } --------------------------------------------------------------
} } -----------------
} } }
} } } Hello listers,
} } }
} } } We are in the process of justifying, to the University, a
} } proposal to
} } } purchase an ESEM. In prepapring the business case I am
} } including the
} } } ten year financials for both FEG and Tungtsen filament
} } machines. Given
} } } that we have to break even in that time, including covering our
} } } depreciation, the Tungsten instrument is easier to justify
} } in a purely
} } } financial sense.
} } }
} } } From a scientific and operational viewpoint, though, I was hoping
} } } some
} } } of you could provide opinions on the relative merits of
} } Tungsten or FEG.
} } } Our current conventional SEM is a Philips XL-30 S-FEG so we
} } already know
} } } of the costs associated with the emitter.
} } }
} } } The range of samples we will be required to put in our ESEM will be
} } } anything you oculd possibly imagine from the Faculties of
} } Engineering,
} } } Science and Medicine. Samples will inlcude food materials
} } (big dairy
} } } industry in New Zealand), polymers, conducting polymers, mammalian
} } } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } } ceramic coatings and bees knees. We will definitely need a
} } hot-stage.
} } }
} } } If you would like to contact me off list with your opinions please
} } } feel
} } } free.
} } }
} } } Kind regards
} } } Bryony James
} } } Research Centre for Surface and Materials Science
} } } Univetrsity of Auckland
} } } New Zealand
} } }
} } }
} } }
} } } This incoming email to UWE has been independently scanned
} } for viruses
} } } and any virus detected has been removed using McAfee anti-virus
} } } software
} } }
} }
} } ----------------------------------------
} } Patton, David
} } Email: David.Patton-at-uwe.ac.uk
} } "University of the West of England"
} }
} }
} }
} } This email has been independently scanned for viruses and any
} } virus detected has been removed using McAfee anti-virus software
} }
} }
} }
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 10:42:01 2004

Contents Retrieved from Microscopy Listserver Archives
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When choosing a scanner for negatives, an important parameter is the Dmax
(which is a log value so relatively small differences can be
significant). The Dmax needed for negs is a lot more than for most printed
images or documents.

At 08:55 AM 5/18/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 11:16:44 2004

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I agree that resolution is more dependent on sample than microscope. What a
microscope is capable of doing with an "ideal" sample often does not relate
to the real world of biological samples which are anything but ideal!

To get really good resolution you need to use higher kV values. These same
values will result in the primary electrons penetrating too far into the low
density biological sample resulting in substantial loss of signal in general
and se1 & se2's in particular. Resulting image will be low resolution and
often of much lesser quality than the same sample taken at a lower
magnification.

The problem of kV can be partially overcome by using a more coherent
beam with greater beam density, i.e. Field Emission. FE allows one to work
at lower kV values resulting in a se yield that is still adequate while
minimizing sample damage. Resulting images are likely to be higher
resolution (sharper with more detail) than comparable images at similar kVs
from a tungsten instrument.

However, there is a point where you go from useful magnification to
"empty " magnification regardless of the gun type. This is sample dependent
and must be determined accordingly. So it is unlikely that you will get any
additional information from a bacteria sample at 100k than at say 50K.
However you will most likely get a much sharper image at 20k with FE than
you could with a W filament.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 5/18/04 8:55 AM, "Dusevich, Vladimir" {DusevichV-at-umkc.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--}
-
}
} In my experience medium/high magnifications for wet
} specimens are limited mostly by specimens themselves and not by a
} type of emitter. While I can get a nice picture of gold on carbon
} at x100k, for most of my "real life" specimens magnification is
} limited by x20k (or less).
}
} Vladimir
}
} } We look mostly at hydrated biological samples. We have a
} } tungsten gun XL30 ESEM TMP. For looking at bacteria and
} } cells a FEGESEM would be superior in terms of reduced
} } damage and improved resolution. I find it hard to get
} } medium/high resolution with wet biological samples. I feel
} } FEGESEM would make this a lot easier.
} }
} } Dave
} }
} } On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} } {b.james-at-auckland.ac.nz} wrote:
} }
} } }
} } }
} } }
} } ----------------------------------------------------------------------
} } } --------
} } } The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America
} } } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } --------------------------------------------------------------
} } -----------------
} } }
} } } Hello listers,
} } }
} } } We are in the process of justifying, to the University, a
} } proposal to
} } } purchase an ESEM. In prepapring the business case I am
} } including the
} } } ten year financials for both FEG and Tungtsen filament
} } machines. Given
} } } that we have to break even in that time, including covering our
} } } depreciation, the Tungsten instrument is easier to justify
} } in a purely
} } } financial sense.
} } }
} } } From a scientific and operational viewpoint, though, I was hoping
} } } some
} } } of you could provide opinions on the relative merits of
} } Tungsten or FEG.
} } } Our current conventional SEM is a Philips XL-30 S-FEG so we
} } already know
} } } of the costs associated with the emitter.
} } }
} } } The range of samples we will be required to put in our ESEM will be
} } } anything you oculd possibly imagine from the Faculties of
} } Engineering,
} } } Science and Medicine. Samples will inlcude food materials
} } (big dairy
} } } industry in New Zealand), polymers, conducting polymers, mammalian
} } } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } } ceramic coatings and bees knees. We will definitely need a
} } hot-stage.
} } }
} } } If you would like to contact me off list with your opinions please
} } } feel
} } } free.
} } }
} } } Kind regards
} } } Bryony James
} } } Research Centre for Surface and Materials Science
} } } Univetrsity of Auckland
} } } New Zealand
} } }
} } }
} } }
} } } This incoming email to UWE has been independently scanned
} } for viruses
} } } and any virus detected has been removed using McAfee anti-virus
} } } software
} } }
} }
} } ----------------------------------------
} } Patton, David
} } Email: David.Patton-at-uwe.ac.uk
} } "University of the West of England"
} }
} }
} }
} } This email has been independently scanned for viruses and any
} } virus detected has been removed using McAfee anti-virus software
} }
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 11:19:50 2004

Contents Retrieved from Microscopy Listserver Archives
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I haven't tried the scanners you mentioned but you may want to check out this April 2004 review article in PCWorld online:

http://www.pcworld.com/reviews/article/0,aid,115075,00.asp

Gene P. Young
Sr. Analytical Technologist
Analytical Sciences, Polymer Characterization

The Dow Chemical Company
2301 N. Brazosport Blvd., B-1470
Freeport, Texas 77541-3257
Fax: (979) 238-0095

*(979) 238-1579 * gpyoung-at-dow.com

****************************************
Original message:

Hello Listers,

I wanted to see if anyone has had any experience scanning negatives with the Canon Canoscan 9900F.
I have a low end Canoscan that I use for documents and the occasional photograph, which has given me very good results, but is not set up for negatives. I have seen the recent posts about the Epson scanner, but I am trying to keep it under a $1000 so that I do not have to treat it as a capital purchase. I have tried for the last two years to get a Coolscan 8000 on the capital budget with no luck, and do not see any scanner above $1000 as an option right now.

Thanks,
Steve

Steven Lee
Chief Technologists
Electron Microscopy Laboratory
Baylor University Medical Center
3500 Gaston Ave
Dallas, TX 750246
Ph: 214.820.3302
Fx: 214.820.4110
Em: stevenle-at-baylorhealth.edu

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 02:44:19 2004

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}
} IbPRIA'2005
}
} 2nd Iberian Conference on Pattern Recognition and Image Analysis
}
} June 7-9, 2005 - Estoril, Portugal
}
} http://ibpria2005.isr.ist.utl.pt
}
}
} =================
} ABOUT IbPRIA'2005
} =================
} IbPRIA'2005 is the second edition of the Iberian Conference on Pattern
} Recognition and Image Analysis and will be held in Estoril (Portugal)
} in June 7-9, 2005.
}
} IbPRIA is an international event co-organised every two years, by the
} Spanish and Portuguese Associations for Pattern Recognition (AERFAI
} and APRP). Its mission is to bring together researchers from all over
} the world working in Pattern Recognition and in all areas of Video,
} Image and Signal Processing. Participants will have the opportunity to
} meet colleagues working in these areas, to attend oral sessions and to
} exchange ideas during poster sessions.
}
} IbPRIA'2005 is sponsored by IAPR-International Association for Pattern
} Recognition and the conference proceedings are planned to be published
} by Springer in LNCS series.
}
} ======
} TOPICS
} ======
} The topics of the conference include, but are not limited to:
}
} - Pattern Recognition
} - Image Analysis
} - Computer Vision
} - Multimedia Systems
} - Statistical & Structural Pattern Recognition
} - Neural Networks
} - Bioinformatics
} - Image Coding and Processing
} - Shape and Texture Analysis
} - Biomedical Pattern Analysis
} - Information Systems
} - Speech Recognition
} - Natural Language Analysis
} - Document Processing
} - Robotics
} - Remote Sensing
} - Industrial Applications of Pattern Recognition
} - Special Hardware Architectures
}
} =================
} PROGRAM COMMITTEE
} =================
} Jake Aggarwal, University of Texas, USA
} José Benedi, Polyt. University of Valencia, Spain
} Isabelle Bloch, ENST, France
} Hervé Bourlard, EPFL, Switzerland
} Patrick Bouthemy, IRISA, France
} Horst Bunke, University of Bern, Switzerland
} Aurélio Campilho, University of Porto, Portugal
} Gilles Celeux, Université Paris-Sud, France
} Luigi Cordella, University of Napoles, Italy
} Alberto Del Bimbo, University of Firenze, Italy
} Hervé Delinguette, INRIA, France
} Rachid Deriche, INRIA, France
} José Dias, Instituto Superior Técnico, Portugal
} Robert Duin, University of Delft, The Netherlands
} Mário Figueiredo, Instituto Superior Técnico, Portugal
} Ana Fred, Instituto Superior Técnico, Portugal
} Andrew Gee, University of Cambridge, UK
} Mohamed Kamel, University of Waterloo, Canada
} Aggelos Katsaggelos, Northwestern University, USA
} Joseph Kittler, University of Surrey, UK
} Seong-Whan Lee, University of Korea, Korea
} Ana Mendonça, University of Porto, Portugal
} Hermann Ney, University of Aachen, Germany
} Wiro Niessen, University of Utrecht, The Netherlands
} Maria Petrou, University of Surrey, UK
} Armando Pinho, University of Aveiro, Portugal
} Ioannis Pitas, University of Tessaloniki, Greece
} Filiberto Pla, University Jaume I, Spain
} Richard Prager, University of Cambridge, UK
} José Principe, University of Florida, USA
} Ian Reid, University of Oxford, UK
} Gabriella Sanniti di Baja, Istituto di Cibernética, Italy
} Beatriz Santos, University of Aveiro, Portugal
} Jose Santos-Victor, Inst. Superior Técnico, Portugal
} Joan Serrat, Aut. University of Barcelona, Spain
} Yoshiaki Shirai, Osaka University, Japan
} Pierre Soille, Joint Research Centre, Italy
} Karl Tombre, LORIA, France
} M. Ines Torres, Univ. of the Basque Country, Spain
} Emmanuele Trucco, Heriot-Watt University, UK
} Alessandro Verri, University of Genova, Italy
} Max Viergever, University of Utrecht, The Netherlands
} Joachim Weickert, Saarland University, Germany
}
} ======
} CHAIRS
} ======
} GENERAL CO-CHAIRS:
} Jorge S. Marques (Instituto Superior Técnico, Portugal)
} Nicolás Pérez de la Blanca (University of Granada, Spain)
}
} LOCAL CHAIR:
} Pedro Pina (Instituto Superior Técnico, Portugal)
}
} ====================
} ORGANISING COMMITTEE
} ====================
} Joăo Sanches, Joăo Paulo Costeira, Teresa Barata, Vitorino Ramos,
} José Saraiva, Michele Mengucci, Fernando Soares
}
}
} ===================================
} PAPER SUBMISSION AND REVIEW PROCESS
} ===================================
} Papers should describe original and unpublished work on the topics of
} the conference. Prospective authors should prepare a full paper,
} written in english, not exceeding 8 pages and must submit it
} electronically.
}
} All manuscripts will be blind-reviewed by at least two members of the
} program committee. Accepted papers are intended to appear in the
} Springer LNCS series which will be distributed to all participants at
} the Conference.
}
} Submission implies that at least one of the authors has to register
} and to present the communication at the conference if the paper is
} accepted.
}
} ===============
} IMPORTANT DATES
} ===============
} Submission of papers : Noverber 12, 2004
} Notification of acceptance: January 7, 2005
} Camera-ready : January 30, 2005
} Early registration : April 7, 2005
} Conference : June 7-9, 2005
}
} =====
} VENUE
} =====
} The conference will take place in Estoril, a beautiful village located
} at about 20 km of Lisbon centre.
}
} The conference will be held at a four star hotel (Hotel Eden), that
} disposes of adequate facilities for workshops and conferences.
}
} The international airport of Lisbon is about 40 minutes from the
} venue. There is a direct bus-shuttle from/to the airport to the Hotel
} every hour. Alternatively, participants can also easily reach the
} venue by train, car or taxi.
}
} ========
} CONTACTS
} ========
} IbPRIA'2005 Secretariat
} CVRM / Geo-Systems Centre
} Instituto Superior Técnico
} Av. Rovisco Pais
} 1049-001 Lisboa
} PORTUGAL
}
} URL : http://ibpria2005.isr.ist.utl.pt
} e-mail: ibpria2005-at-isr.ist.utl.pt
} Tel : +351-218417438
} Fax : +351-218417442
}

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 10:22:00 2004

Contents Retrieved from Microscopy Listserver Archives
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Fellow Listmembers,

Members in the Greater Orlando, Florida area are cordially invited to attend
a two day mini-workshop on "Cryomicrotomy and Cryoultramicrotomy for Materials
Sciences."

When:
Tuesday, June 8 and Wednesday, June 9, 2004, 9:00am-4:00pm

Where:
Room 101, Materials Characterization Facility
Advanced Materials Processing & Analysis Center
University of Central Florida
12443 Research Parkway
Orlando, FL 32826

What:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryomicrotomy and cryoultramicrotomy, including toolmaking (wire loops
and hair probes), glass knife making, evaluation of glass knives, care and
cleaning of diamond knives and operation of the cryomicrotome and
cryoultramicrotome.

Background:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing" at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

Important Info:
There is no charge for this workshop.
Meals and refreshments will be served!
Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryosectioning hands-on
sessions on the second day.

Contacts:
To RSVP and to reserve a spot for the hands-on sessions, please contact
either Ms. Kim Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} ,
800.552.2262) or Ms. Nancy Crouch at ICMAS, Inc. ( {nancy-at-icmas.com} , 865.984.8058)

Sponsors and Organizers:
University of Central Florida
Advanced Materials Processing & Analysis Center
Materials Characterization Facility
RMC Products Group, Boeckeler Instruments, Inc.

Hope to see you there!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 10:32:23 2004

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For ESEM in wet mode low voltage beam is not suitable,
even at 5 kV noise level is too high.

Vladimir

} I agree that resolution is more dependent on sample than
} microscope. What a microscope is capable of doing with an
} "ideal" sample often does not relate to the real world of
} biological samples which are anything but ideal!
}
} To get really good resolution you need to use higher kV
} values. These same values will result in the primary
} electrons penetrating too far into the low density biological
} sample resulting in substantial loss of signal in general and
} se1 & se2's in particular. Resulting image will be low
} resolution and often of much lesser quality than the same
} sample taken at a lower magnification.
}
} The problem of kV can be partially overcome by using a
} more coherent beam with greater beam density, i.e. Field
} Emission. FE allows one to work at lower kV values resulting
} in a se yield that is still adequate while minimizing sample
} damage. Resulting images are likely to be higher resolution
} (sharper with more detail) than comparable images at similar
} kVs from a tungsten instrument.
}
} However, there is a point where you go from useful
} magnification to "empty " magnification regardless of the gun
} type. This is sample dependent and must be determined
} accordingly. So it is unlikely that you will get any
} additional information from a bacteria sample at 100k than at
} say 50K. However you will most likely get a much sharper
} image at 20k with FE than you could with a W filament.
}
} Debby
}
}
}
} Debby Sherman, Manager Phone: 765-494-6666
} Life Science Microscopy Facility FAX: 765-494-5896
} Purdue University E-mail: dsherman-at-purdue.edu
} S-052 Whistler Building
} 170 S. University Street
} West Lafayette, IN 47907 http://www3.agriculture.purdue.edu/microscopy
}
}
} On 5/18/04 8:55 AM, "Dusevich, Vladimir" {DusevichV-at-umkc.edu} wrote:
}
} }
} }
} }
} ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} --------------
} --}
} -
} }
} } In my experience medium/high magnifications for wet specimens are
} } limited mostly by specimens themselves and not by a type of
} emitter.
} } While I can get a nice picture of gold on carbon at x100k,
} for most of
} } my "real life" specimens magnification is limited by x20k (or less).
} }
} } Vladimir
} }
} } } We look mostly at hydrated biological samples. We have a tungsten
} } } gun XL30 ESEM TMP. For looking at bacteria and cells a
} FEGESEM would
} } } be superior in terms of reduced damage and improved resolution. I
} } } find it hard to get medium/high resolution with wet biological
} } } samples. I feel FEGESEM would make this a lot easier.
} } }
} } } Dave
} } }
} } } On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} } } {b.james-at-auckland.ac.nz} wrote:
} } }
} } } }
} } } }
} } } }
} } }
} ---------------------------------------------------------------------
} } } -
} } } } --------
} } } } The Microscopy ListServer -- Sponsor: The Microscopy
} } } Society of America
} } } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } On-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } }
} } } --------------------------------------------------------------
} } } -----------------
} } } }
} } } } Hello listers,
} } } }
} } } } We are in the process of justifying, to the University, a
} } } proposal to
} } } } purchase an ESEM. In prepapring the business case I am
} } } including the
} } } } ten year financials for both FEG and Tungtsen filament
} } } machines. Given
} } } } that we have to break even in that time, including covering our
} } } } depreciation, the Tungsten instrument is easier to justify
} } } in a purely
} } } } financial sense.
} } } }
} } } } From a scientific and operational viewpoint, though, I
} was hoping
} } } } some of you could provide opinions on the relative merits of
} } } Tungsten or FEG.
} } } } Our current conventional SEM is a Philips XL-30 S-FEG so we
} } } already know
} } } } of the costs associated with the emitter.
} } } }
} } } } The range of samples we will be required to put in our
} ESEM will be
} } } } anything you oculd possibly imagine from the Faculties of
} } } Engineering,
} } } } Science and Medicine. Samples will inlcude food materials
} } } (big dairy
} } } } industry in New Zealand), polymers, conducting polymers,
} mammalian
} } } } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } } } ceramic coatings and bees knees. We will definitely need a
} } } hot-stage.
} } } }
} } } } If you would like to contact me off list with your
} opinions please
} } } } feel free.
} } } }
} } } } Kind regards
} } } } Bryony James
} } } } Research Centre for Surface and Materials Science Univetrsity of
} } } } Auckland New Zealand
} } } }
} } } }
} } } }
} } } } This incoming email to UWE has been independently scanned
} } } for viruses
} } } } and any virus detected has been removed using McAfee anti-virus
} } } } software
} } } }
} } }
} } } ----------------------------------------
} } } Patton, David
} } } Email: David.Patton-at-uwe.ac.uk
} } } "University of the West of England"
} } }
} } }
} } }
} } } This email has been independently scanned for viruses and
} any virus
} } } detected has been removed using McAfee anti-virus software
} } }
} } }
} } }
} }
} }
} }
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 14:24:44 2004

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Fellow Listmembers,

Members in the Greater Madison, Wisconsin area are cordially invited to
attend a two day mini-workshop on "Cryoultramicrotomy for Materials Sciences."

When:
Wednesday, June 2 and Thursday, June 3, 2004, 9:00am-4:00pm

Where:
Room 374, Truax Building
Madison Area Technical College
3550 Anderson Street
Madison, WI 53704

(Gated lot near Truax Bldg. has audio to Parking Department. Mention this
Workshop for entrance to parking lot. Enter left side of building, take main
elevator to third floor)

What:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair probes),
glass knife making, evaluation of glass knives, care and cleaning of diamond
knives and operation of the cryomicrotome and cryoultramicrotome.

Background:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing" at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

Important Info:
There is no charge for this workshop.
Meals and refreshments will be served!
Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryosectioning hands-on
sessions on the second day.

Contacts:
To RSVP and to reserve a spot for the hands-on sessions, please contact
either Kim Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262)
or Michael Kostrna at Madison Area Technical College
( {mkostrna-at-matcmadison.edu} , 608.246.6762).

Sponsors and Organizers:
Madison Area Technical College
(Electron Microscopy)
RMC Products Group, Boeckeler Instruments, Inc.
Doug D'Arcy, Midwest Regional Representative

See you in Madison!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 17:00:14 2004

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Hello Fellow List Members,

Iąd appreciate your collective wisdom and experiences for a project Iąm
starting. I need to create high resolution (250 Mb minimum) photo files of
current microprocessor die faces (pentium 4 type) to show the circuitry and
traces with as much detail as possible. Iąd like to do this using my Nikon
Optiphot and a yet to be purchased motorized positionable stage with
automation software to include my Fuji S2 still camera (34 Mb sized files
per image) with image stitching as an added option. I have extensive
experience in Photoshop and would use that to stitch the images if the
automation software package doesnąt include that. The stage travel only
needs to be about 3" (75mm) in the X and Y dimensions.

Iąve been reading about some of the software programs available to help
accomplish this. Iąve come across Image-Pro Plus with the Scope-Pro plugin
and the software program Metamorph in my Google searches. I donąt need
extensive filtering or analysis functions in the software, just the ability
to create multiple, tileable images in a repeatable manner.

What economical software and hardware (such as the MultiScan-4 Low Cost
Scanning Stage for example) do you have experience with in similar projects?

Do any of you have an older version of Image Pro Plus or similar software
program that is sitting abandoned and alone on a shelf that needs a new
home? How about a used basic scanning stage thatąs collecting dust?

Any and all advice would be appreciated. You can email me off-list if thatąs
easier.

Thanks,
Doug Baldwin
Baldwin Hi-Tech Photography
dougbaldwin-at-mindspring.com

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 19:03:05 2004

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The P4 BGA devices are like PPC G3, G4 and G5
products and are flip chip BGAs. Between the
inverted die and the multi layer ceramic package
is a thin layer of silicone. Through this layer
are many (700+) solder vias between the die and
package. Once the silicone is removed (and assuming
that you get the die off), the top layer greatly
masks the underlying 5-8 layers (depending on part
timeframe of manufacture) since it is used for interface
to the ceramic package.

This top-most layer must be removed to begin to
get at the actual interconnect layers. Once removed,
the underlying layers can be exposed by plasma
depassivation. Or, you can try wet etching.

These types of processors are face down rather than
face up. This is because they are too hot compared
to earlier CPUs.

The other factor is that you do not need high rez
image segments to make a high rez final image. To get
any reasonable image detail, you will likely need to
shoot at 500X or 1000X. At these mags, your field of
view is somewhere around 300u (guessing). For a 0.5cm
die, you will likely take 1,000 images (guessing again).
You can do the math. The point is that for a final high
rez image, it is made up of many low rez image segments.
The other problem you will face at high mag is the problem
of low DOF. The solution is to shoot with a SEM at high
tilt angle and dynamic focus. Then colorize the image.

If you need motorized and programmed stage movement,
Prior E103 is a good candidate and Soft Imaging analySIS
Opti is a good driving software product. Neither of
these items are free.

Anyway, I have found that it is not worth the effort.
But of course, YMMV.

gary g.

At 03:07 PM 5/19/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 04:11:37 2004

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Doug

given the complexity of what you are doing, would it not be possible to try another method. If the die faces are flat and of the right size, why not just use a very high resolution flat bed scanner and do the whole thing in one go.

I'm sure that HP, Epson, Canon all do better than 3000dpi (optical resolution. It might certainly be worth investigating if camera photography involves a horrendous amount of image stitching (especially given the edge distortion in even the best camera). The only problems may be the reflective light quality of the scanner or how much depth of field there would be in a scanner image if the die has lots of depth to its layers.

My apologies if I've missed some technical point.

Malc

Malcolm Haswell
e.m. unit
University of Sunderland
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Doug Baldwin {dougbaldwin-at-mindspring.com}

My thanks to everyone who replied to my legal/ethics query. After my
client became a bit more educated regarding the health risk we discovered
and checked with their counsel, they will do the right thing. The twist
here was that they were analyzing competitors' products which are made
overseas, so there are issues of diplomacy.

Alan Stone

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 09:52:22 2004

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Hi All,

I wish to set up a logging system to record instrument use.
Ideally it would log date and time users start and
finish work on a particular project on each of our
instruments so that we can assess use of our facility.

At present users fill in a log book when they use an
instrument. It is easy to get general data (25 sessions to
the page gives an idea of instrument use but not user). I
don't want to waste time transcribing the data from the 20
instrument log books into a computer. Neither do I want to
spend a lot of money on each machine to gather the
information, however, most machines already have a PC
attached running the instrument or some ancillary equipment
and these are all networked.

What systems are being used at other sites? Any suggestions
of inexpensive systems that would work on two sites 6 miles
apart?

Regards,
Ron

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 15:49:26 2004

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Hello Everyone
We have a Nonotech Semprep2 sputter coater which is so old the
company no longer exists. The glass cylinder has now got one more
gouge in it and it will have to lose at least 3 cm to grind it out.
Does anyone have any experience with where to buy a new glass
cylinder?

Many thanks
Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 17:26:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mocherla-at-eng.fsu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, May 20, 2004 at 10:43:53
---------------------------------------------------------------------------

Email: mocherla-at-eng.fsu.edu
Name: supriya

Organization: FSU

Title-Subject: [Microscopy] [Filtered] Liposome Grids

Question: Dear authors,

I really appreciate this group for their support in my work.

I observed that for negative staining, carbon coated Formvar grid was used mostly. I would like to know if there is any significance in using this particlular grid or Can I use Carbon support film on Copper or Gold grid.

Thanks!!

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 19:24:44 2004

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On May 20, 2004, at 3:35 PM, by way of MicroscopyListserver wrote:

} Title-Subject: [Microscopy] [Filtered] Liposome Grids
}
} Question: Dear authors,
}
} I really appreciate this group for their support in my work.
}
} I observed that for negative staining, carbon coated Formvar grid was
} used mostly. I would like to know if there is any significance in
} using this particlular grid or Can I use Carbon support film on Copper
} or Gold grid.
}
Dear Supriya,
The grids most often used for negative staining are copper grids on
which there is a layer of formvar and usually an additional layer of
carbon. These are often referred to as carbon-formvar grids or
carbon-coated formvar grids. It is much easier to use a carbon-formvar
support film than to use just a carbon film for support. The resulting
film is much stronger than plain carbon, and does not degrade the
images of negatively stained preps. The web sites of several of the EM
supply companies describe their carbon-formvar grids.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 20:04:13 2004

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Malcolm,

Interestingly, I had the same thought and tried this technique. I stopped by
one of the area's premier graphics arts service bureaus with an 8000+ dpi
flat bed scanner. We put the open faced CPU chip on the glass and proceeded
to scan it. It was awful. The main problem was that the light source on the
scanner was off-axis to the scanning array. This renders the face of the
chip dark and worthless.

Photos of microprocessors benefit from coaxial lighting since the metal
parts and traces reflect the light straight back to the lens and light
source. Lighting that's even slightly off-axis shows a marked drop off in
detail and reflectivity of the die faces.

The high dpi flat bed scanners are set up for flat artwork such as paintings
and drawings where side lighting is fine for rendering all the detail but
not for reflective metal parts.

Doug

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Doug
}
} given the complexity of what you are doing, would it not be possible to try
} another method. If the die faces are flat and of the right size, why not just
} use a very high resolution flat bed scanner and do the whole thing in one go.
}
} I'm sure that HP, Epson, Canon all do better than 3000dpi (optical resolution.
} It might certainly be worth investigating if camera photography involves a
} horrendous amount of image stitching (especially given the edge distortion in
} even the best camera). The only problems may be the reflective light quality
} of the scanner or how much depth of field there would be in a scanner image if
} the die has lots of depth to its layers.
}
} My apologies if I've missed some technical point.
}
} Malc
}
} Malcolm Haswell
} e.m. unit
} University of Sunderland
} UK
} e-mail: malcolm.haswell-at-sunderland.ac.uk
}
}
}
}
} ----- Original Message -----
} } From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} Date: Wednesday, May 19, 2004 11:07 pm
} Subject: [Microscopy] Hi-Res Microprocessor Photos
}
} }
} }
} } -------------------------------------------------------------------
} } -----------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } AmericaTo Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } -------------------------------------------------------------------
} } ----
} }
} } Hello Fellow List Members,
} }
} } IŹd appreciate your collective wisdom and experiences for a
} } project IŹm
} } starting. I need to create high resolution (250 Mb minimum) photo
} } files of
} } current microprocessor die faces (pentium 4 type) to show the
} } circuitry and
} } traces with as much detail as possible. IŹd like to do this using
} } my Nikon
} } Optiphot and a yet to be purchased motorized positionable stage with
} } automation software to include my Fuji S2 still camera (34 Mb
} } sized files
} } per image) with image stitching as an added option. I have extensive
} } experience in Photoshop and would use that to stitch the images if the
} } automation software package doesnŹt include that. The stage travel
} } onlyneeds to be about 3" (75mm) in the X and Y dimensions.
} }
} } IŹve been reading about some of the software programs available to
} } helpaccomplish this. IŹve come across Image-Pro Plus with the
} } Scope-Pro plugin
} } and the software program Metamorph in my Google searches. I donŹt need
} } extensive filtering or analysis functions in the software, just
} } the ability
} } to create multiple, tileable images in a repeatable manner.
} }
} } What economical software and hardware (such as the MultiScan-4 Low
} } CostScanning Stage for example) do you have experience with in
} } similar projects?
} }
} } Do any of you have an older version of Image Pro Plus or similar
} } softwareprogram that is sitting abandoned and alone on a shelf
} } that needs a new
} } home? How about a used basic scanning stage thatŹs collecting dust?
} }
} } Any and all advice would be appreciated. You can email me off-list
} } if thatŹs
} } easier.
} }
} } Thanks,
} } Doug Baldwin
} } Baldwin Hi-Tech Photography
} } dougbaldwin-at-mindspring.com
} }
} }
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 22:16:30 2004

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There is a photographer here in Oz who produces absolutely brilliant images
by scanning objects on a flat-bed scanner. They are very high resolution,
look as good as the images of leaves, flowers, insects (even very shiny
ones) we get using a good digital camera - Olympus DP70 or ProgRes or
similar, on a dissecting microscope. He's developed some ways of using the
scanner to get such great images. Name is Stuart Owen Fox, go here
http://www.smartstate.qld.gov.au/images/icase4g_2.jpg for an example.
cheers,
Rosemary

} From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} Date: Thu, 20 May 2004 18:10:14 -0700
} To: {microscopy-at-msa.microscopy.com}
} Cc: Malcolm Haswell {malcolm.haswell-at-sunderland.ac.uk}
} Subject: [Microscopy] Re: Hi-Res Microprocessor Photos
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Malcolm,
}
} Interestingly, I had the same thought and tried this technique. I stopped by
} one of the area's premier graphics arts service bureaus with an 8000+ dpi
} flat bed scanner. We put the open faced CPU chip on the glass and proceeded
} to scan it. It was awful. The main problem was that the light source on the
} scanner was off-axis to the scanning array. This renders the face of the
} chip dark and worthless.
}
} Photos of microprocessors benefit from coaxial lighting since the metal
} parts and traces reflect the light straight back to the lens and light
} source. Lighting that's even slightly off-axis shows a marked drop off in
} detail and reflectivity of the die faces.
}
} The high dpi flat bed scanners are set up for flat artwork such as paintings
} and drawings where side lighting is fine for rendering all the detail but
} not for reflective metal parts.
}
} Doug
}
}
} }
} }
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ----------------------------------------------------------------------------
} --} -
} }
} } Doug
} }
} } given the complexity of what you are doing, would it not be possible to try
} } another method. If the die faces are flat and of the right size, why not just
} } use a very high resolution flat bed scanner and do the whole thing in one go.
} }
} } I'm sure that HP, Epson, Canon all do better than 3000dpi (optical
} } resolution.
} } It might certainly be worth investigating if camera photography involves a
} } horrendous amount of image stitching (especially given the edge distortion in
} } even the best camera). The only problems may be the reflective light quality
} } of the scanner or how much depth of field there would be in a scanner image
} } if
} } the die has lots of depth to its layers.
} }
} } My apologies if I've missed some technical point.
} }
} } Malc
} }
} } Malcolm Haswell
} } e.m. unit
} } University of Sunderland
} } UK
} } e-mail: malcolm.haswell-at-sunderland.ac.uk
} }
} }
} }
} }
} } ----- Original Message -----
} } } From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} } Date: Wednesday, May 19, 2004 11:07 pm
} } Subject: [Microscopy] Hi-Res Microprocessor Photos
} }
} } }
} } }
} } } -------------------------------------------------------------------
} } } -----------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } AmericaTo Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } } -------------------------------------------------------------------
} } } ----
} } }
} } } Hello Fellow List Members,
} } }
} } } IŹd appreciate your collective wisdom and experiences for a
} } } project IŹm
} } } starting. I need to create high resolution (250 Mb minimum) photo
} } } files of
} } } current microprocessor die faces (pentium 4 type) to show the
} } } circuitry and
} } } traces with as much detail as possible. IŹd like to do this using
} } } my Nikon
} } } Optiphot and a yet to be purchased motorized positionable stage with
} } } automation software to include my Fuji S2 still camera (34 Mb
} } } sized files
} } } per image) with image stitching as an added option. I have extensive
} } } experience in Photoshop and would use that to stitch the images if the
} } } automation software package doesnŹt include that. The stage travel
} } } onlyneeds to be about 3" (75mm) in the X and Y dimensions.
} } }
} } } IŹve been reading about some of the software programs available to
} } } helpaccomplish this. IŹve come across Image-Pro Plus with the
} } } Scope-Pro plugin
} } } and the software program Metamorph in my Google searches. I donŹt need
} } } extensive filtering or analysis functions in the software, just
} } } the ability
} } } to create multiple, tileable images in a repeatable manner.
} } }
} } } What economical software and hardware (such as the MultiScan-4 Low
} } } CostScanning Stage for example) do you have experience with in
} } } similar projects?
} } }
} } } Do any of you have an older version of Image Pro Plus or similar
} } } softwareprogram that is sitting abandoned and alone on a shelf
} } } that needs a new
} } } home? How about a used basic scanning stage thatŹs collecting dust?
} } }
} } } Any and all advice would be appreciated. You can email me off-list
} } } if thatŹs
} } } easier.
} } }
} } } Thanks,
} } } Doug Baldwin
} } } Baldwin Hi-Tech Photography
} } } dougbaldwin-at-mindspring.com
} } }
} } }
} } }
} } }
} }
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 23:52:06 2004

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Hi all

Can anyone suggest a good text or reference for helping to identify
asbestos bodies in lung using an SEM, and using EDS.

Many thanks

Regards

Allan

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 00:26:15 2004

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Dear Elaine

A good glassblower can sort it.
Either by producing another or taking the gouge out.
I have done that in the past on a VERY OLD Edwards. Definitely cheaper than the scientific company's. The quality of the work was good and the new dome is still in operation after 6 years.

-----Original Message-----
} From: Elaine Humphrey [mailto:ech-at-interchange.ubc.ca]
Sent: Thursday, May 20, 2004 10:59 PM
To: microscopy-at-msa.microscopy.com

Hello Everyone
We have a Nonotech Semprep2 sputter coater which is so old the
company no longer exists. The glass cylinder has now got one more
gouge in it and it will have to lose at least 3 cm to grind it out.
Does anyone have any experience with where to buy a new glass
cylinder?

Many thanks
Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 03:55:22 2004

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Dear Doug,

Regarding stitching images, we have successfully stitched micrographs using
PanaVue ImageAssembler (www.panavue.com) as it works with flat perspective.
Have not tried to stitch very large numbers of images though.

With regards
Thor

Dr Thor Bostrom
Analytical EM Facility; and
School of Physical and Chemical Sciences,
Queensland University of Technology (QUT)
Brisbane, QLD 4001, Australia

----------Original
message-------------------------------------------------------

Hi all!

does anybody know how is the phase in AFM software Nanoscope III for
Dimension 2100 defined? Could the bright regions in the phase image be
assigned to the depressions, if we are working in the attractive force
regime? Thank's a lot for any hint.

Best regards!

--
__________________________________________________

Đenan Konjhodzic
Max-Planck-Institut für Kohlenforschung
Kaiser-Wilhelm-Platz 1
D-45470 Mülheim an der Ruhr

Phone: +49-208-306 2449
Fax: +49-208-306 2995
Mobile: +49-179-94 98 435
e-mail: denan-at-mpi-muelheim.mpg.de
___________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 06:54:26 2004

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Hi Allan,

I seriously doubt there is one as to unambiguously identify fibrous
asbestos is the job of TEM and (not or) an EDS on TEM.

****************************************
Chaoying Ni, PhD
The W.M. Keck Electron Microscope Facility
Facility location: 022 Spencer Laboratory
Mailing address:
201 duPont Hall
Dept of Matls Sci & Eng
University of Delaware
Newark, DE 19716
(302) 831-8354 (O); -2318(L); -4545(Fax)
http://eml.masc.udel.edu
*****************************************

On Fri, 21 May 2004, Allan Mitchell wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi all
}
} Can anyone suggest a good text or reference for helping to identify
} asbestos bodies in lung using an SEM, and using EDS.
}
} Many thanks
}
} Regards
}
} Allan
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 07:57:16 2004

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I have some cells in solution. Is there some general technique to preserve
them so that I can put some down on a carbon membrane coated TEM grid
without them shriveling up? Can anyone refer me to a good reference on TEM
sample prep of cells?

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 08:09:47 2004

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Allan,

The Mineralogical Society of America has a series of books on
mineralogical and geochemical topics. Volume 28 is titled "Health
Effects of Mineral Dusts" and covers a wide range of topics, from basic
asbestos mineralogy to cellular and molecular mechanisms for disease.
I'm not sure if it specifically deals with identifying asbestos bodies
in lung tissue specificaly but it should have some references, and there
should be useful information to help with EDS identification. It's
available at the MSA (the other MSA) website at
www.minsocam.org/MSA/RIM/ for a very reasonable price for the amount of
information contained ($32 US).

Best Regards,
Bryan Bandli

Allan Mitchell wrote:

}
}
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}
}
} Hi all
}
} Can anyone suggest a good text or reference for helping to identify
} asbestos bodies in lung using an SEM, and using EDS.
}
} Many thanks
}
} Regards
}
} Allan
}
}

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From MicroscopyL-request-at-ns.microscopy.com Fri May 21 10:48:40 2004

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I had a request recently to perform EDS on a presumed crysotile
crystal/shard that had been located with TEM on a grid. We have an
Oxford INCA system on our FEI Quanta 400, so I resurrected an old grid
holder from a salvaged RCA EMU4, mounted the grid in holder in the ESEM,
located the offending grid square and performed a point and ID on the
crystal in question.

As Chaoying suggests, this would not be in concert with NIOSH 7402
(TEM)
http://www.cdc.gov/niosh/nmam/pdfs/7402.pdf, or NIOSH 9000 (XRD)
http://www.cdc.gov/niosh/nmam/pdfs/7402.pdf, identifications of
asbestos, to give quick examples.

Other sources and possibilities for your problem(?):
SEM+:
http://sup.ultrakohl.com/News-nov/mesoth.htm

EBSD:

http://www.asbestostemlabs.com/staff.htm

SEM/EBSD
http://www.dxcicdd.com/01/pdf/D-075.pdf

I don't believe that EBSD/SEM has been approved for asbestos:

http://hyperphysics.phy-astr.gsu.edu/hbase/minerals/asbestos.html

But that doesn't mean that SEM can't be used in simple identifications
of morphology and composition. The real problem is to find it, if you
are looking in tissue. Mapping for the relevant elements should work,
but for very small crystals, you will be working at or above the 'good
result' window for EDS and mapping when you want to identify and image
at high mag.

Hope some of this helps,

Fred

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: Allan Mitchell [mailto:allan.mitchell-at-stonebow.otago.ac.nz]
Sent: Friday, May 21, 2004 1:01 AM
To: microscopy-at-msa.microscopy.com

Hi all

Can anyone suggest a good text or reference for helping to identify
asbestos bodies in lung using an SEM, and using EDS.

Many thanks

Regards

Allan

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 11:05:04 2004

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Do you want to just look at them whole, in a HVEM? No
embedding/sectioning? What do you want to see?

On Fri, 21 May 2004, Larsen, Michael (Research) wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
} I have some cells in solution. Is there some general technique to preserve
} them so that I can put some down on a carbon membrane coated TEM grid
} without them shriveling up? Can anyone refer me to a good reference on TEM
} sample prep of cells?
}
}

|--------------------------------------------------|
Tamara Howard
Department of Cell Biology and Physiology
University of New Mexico - Health Sciences Center
Albuquerque, NM 87131
thoward-at-unm.edu
|--------------------------------------------------|

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 11:51:52 2004

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Today's microprocessors have micron scale metal lines. You would require submicron resolution to distinguish the lines. A flat bed scanner that would resolve micron scale lines would need at least 25,000 DPI resolution just to detect the lines.

John Mardinly
Intel

-----Original Message-----
} From: Rosemary White [mailto:Rosemary.White-at-csiro.au]
Sent: Thursday, May 20, 2004 8:24 PM
To: Doug Baldwin; microscopy-at-msa.microscopy.com
Cc: Malcolm Haswell

There is a photographer here in Oz who produces absolutely brilliant images
by scanning objects on a flat-bed scanner. They are very high resolution,
look as good as the images of leaves, flowers, insects (even very shiny
ones) we get using a good digital camera - Olympus DP70 or ProgRes or
similar, on a dissecting microscope. He's developed some ways of using the
scanner to get such great images. Name is Stuart Owen Fox, go here
http://www.smartstate.qld.gov.au/images/icase4g_2.jpg for an example.
cheers,
Rosemary

} From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} Date: Thu, 20 May 2004 18:10:14 -0700
} To: {microscopy-at-msa.microscopy.com}
} Cc: Malcolm Haswell {malcolm.haswell-at-sunderland.ac.uk}
} Subject: [Microscopy] Re: Hi-Res Microprocessor Photos
}
}
}
} ------------------------------------------------------------------------------
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------------------------------------------------------------------------------}
-
}
} Malcolm,
}
} Interestingly, I had the same thought and tried this technique. I stopped by
} one of the area's premier graphics arts service bureaus with an 8000+ dpi
} flat bed scanner. We put the open faced CPU chip on the glass and proceeded
} to scan it. It was awful. The main problem was that the light source on the
} scanner was off-axis to the scanning array. This renders the face of the
} chip dark and worthless.
}
} Photos of microprocessors benefit from coaxial lighting since the metal
} parts and traces reflect the light straight back to the lens and light
} source. Lighting that's even slightly off-axis shows a marked drop off in
} detail and reflectivity of the die faces.
}
} The high dpi flat bed scanners are set up for flat artwork such as paintings
} and drawings where side lighting is fine for rendering all the detail but
} not for reflective metal parts.
}
} Doug
}
}
} }
} }
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
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} }
} ----------------------------------------------------------------------------
} --} -
} }
} } Doug
} }
} } given the complexity of what you are doing, would it not be possible to try
} } another method. If the die faces are flat and of the right size, why not just
} } use a very high resolution flat bed scanner and do the whole thing in one go.
} }
} } I'm sure that HP, Epson, Canon all do better than 3000dpi (optical
} } resolution.
} } It might certainly be worth investigating if camera photography involves a
} } horrendous amount of image stitching (especially given the edge distortion in
} } even the best camera). The only problems may be the reflective light quality
} } of the scanner or how much depth of field there would be in a scanner image
} } if
} } the die has lots of depth to its layers.
} }
} } My apologies if I've missed some technical point.
} }
} } Malc
} }
} } Malcolm Haswell
} } e.m. unit
} } University of Sunderland
} } UK
} } e-mail: malcolm.haswell-at-sunderland.ac.uk
} }
} }
} }
} }
} } ----- Original Message -----
} } } From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} } Date: Wednesday, May 19, 2004 11:07 pm
} } Subject: [Microscopy] Hi-Res Microprocessor Photos
} }
} } }
} } }
} } } -------------------------------------------------------------------
} } } -----------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } AmericaTo Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } } -------------------------------------------------------------------
} } } ----
} } }
} } } Hello Fellow List Members,
} } }
} } } IŹd appreciate your collective wisdom and experiences for a
} } } project IŹm
} } } starting. I need to create high resolution (250 Mb minimum) photo
} } } files of
} } } current microprocessor die faces (pentium 4 type) to show the
} } } circuitry and
} } } traces with as much detail as possible. IŹd like to do this using
} } } my Nikon
} } } Optiphot and a yet to be purchased motorized positionable stage with
} } } automation software to include my Fuji S2 still camera (34 Mb
} } } sized files
} } } per image) with image stitching as an added option. I have extensive
} } } experience in Photoshop and would use that to stitch the images if the
} } } automation software package doesnŹt include that. The stage travel
} } } onlyneeds to be about 3" (75mm) in the X and Y dimensions.
} } }
} } } IŹve been reading about some of the software programs available to
} } } helpaccomplish this. IŹve come across Image-Pro Plus with the
} } } Scope-Pro plugin
} } } and the software program Metamorph in my Google searches. I donŹt need
} } } extensive filtering or analysis functions in the software, just
} } } the ability
} } } to create multiple, tileable images in a repeatable manner.
} } }
} } } What economical software and hardware (such as the MultiScan-4 Low
} } } CostScanning Stage for example) do you have experience with in
} } } similar projects?
} } }
} } } Do any of you have an older version of Image Pro Plus or similar
} } } softwareprogram that is sitting abandoned and alone on a shelf
} } } that needs a new
} } } home? How about a used basic scanning stage thatŹs collecting dust?
} } }
} } } Any and all advice would be appreciated. You can email me off-list
} } } if thatŹs
} } } easier.
} } }
} } } Thanks,
} } } Doug Baldwin
} } } Baldwin Hi-Tech Photography
} } } dougbaldwin-at-mindspring.com
} } }
} } }
} } }
} } }
} }
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 14:17:27 2004

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Listers,

I'll try again. Does anyone have a Gatan model 626-300 cryoholder to
sell or donate to a university?
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 14:21:00 2004

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We would like to buy or trade in:
epi-fluorescence lamp housing and slider for Diaphot (inverted Nikon)
new or refurbished.

Vendors welcome!

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 14:48:08 2004

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Hi Doug,

Image-Pro Plus is a very good image analysis software with
extensive capabilities. But there is a another product from
Media Cybernetics which is "Image-Pro Discovery". This
is the smaller version of Image-Pro Plus and therefore
cheaper. It allows you to capture X-Y automatically in
combination with Scope-Pro. The software gives you the
possibility to select the order how you want to capture
the images and it stitches them automatically.
You also could capture Z-stacks automatically either by
moving the microscope stage or with a motorized objective
(Piezo) which gives you very precise results.

However if you want to work with an automatic x-y stage you
should work with a camera which is integrated in the
capturing software because then the software also captures
the images, then the stage moves on, the image is captured and so
on. With your Fuji camera you have to do the capturing
manually which is very cumbersome. You should use a digital
CCD camera which is connected to your computer and shows you
the live image on the computer monitor.

Please let me know if you have further questions.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

DB} ------------------------------------------------------------------------------
DB} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
DB} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
DB} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
DB} -------------------------------------------------------------------------------

DB} Hello Fellow List Members,

DB} Iąd appreciate your collective wisdom and experiences for a project Iąm
DB} starting. I need to create high resolution (250 Mb minimum) photo files of
DB} current microprocessor die faces (pentium 4 type) to show the circuitry and
DB} traces with as much detail as possible. Iąd like to do this using my Nikon
DB} Optiphot and a yet to be purchased motorized positionable stage with
DB} automation software to include my Fuji S2 still camera (34 Mb sized files
DB} per image) with image stitching as an added option. I have extensive
DB} experience in Photoshop and would use that to stitch the images if the
DB} automation software package doesnąt include that. The stage travel only
DB} needs to be about 3" (75mm) in the X and Y dimensions.

DB} Iąve been reading about some of the software programs available to help
DB} accomplish this. Iąve come across Image-Pro Plus with the Scope-Pro plugin
DB} and the software program Metamorph in my Google searches. I donąt need
DB} extensive filtering or analysis functions in the software, just the ability
DB} to create multiple, tileable images in a repeatable manner.

DB} What economical software and hardware (such as the MultiScan-4 Low Cost
DB} Scanning Stage for example) do you have experience with in similar projects?

DB} Do any of you have an older version of Image Pro Plus or similar software
DB} program that is sitting abandoned and alone on a shelf that needs a new
DB} home? How about a used basic scanning stage thatąs collecting dust?

DB} Any and all advice would be appreciated. You can email me off-list if thatąs
DB} easier.

DB} Thanks,
DB} Doug Baldwin
DB} Baldwin Hi-Tech Photography
DB} dougbaldwin-at-mindspring.com

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 15:19:40 2004

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Bill
I disagree with you: carbon coated Formvar film do degrade the image in
your words versus just carbon. Formvar film is quite thick in compare with
"plain carbon", so it "adsorbs" more electrons and therefore "degrade the
image"... Another problem with Formvar and other plastic support films is
that they change their properties under the beam which cause the image
drift... So, in my point of view, it's just wrong statement that carbon
coated Formvar film "does not degrade the images of negatively stained
preps". It's quite opposite: pure thin carbon film is very stable under
the beam, much thinner than any plastic film and therefore provides best
possible (for biological samples) support material in terms of stability
and "transparency" (to the electrons) for negative staining. Carbon coated
plastic support films are popular just because it's much easier to produce
in the Lab (and not necessary the best choice). In my Lab we routinely use
1.4-1.8 nm thick "pure" carbon support films over "holey" film. You may
not use such thin film for huge objects like whole cell, but it works great
for macromolecules of any sort. "Carbon over holey film" grids are
available thorough major EM suppliers. Interestingly, I never used carbon
coated Formvar films. I used to use carbon coating on cellulose-derivative
films like Parlodion (because it drifted so much without carbon) and I used
"naked" Formvar film because it's more stable under the beam than other
variety of films. Formvar film looks much "darker" in the scope than
Parlodion, so I prefer to use carbon coated Parlodion film if I could not
use "normal carbon": very contaminated samples with a lot of aggregates,
cells etc. Someone may need to try "naked" Parlodion (or similar) because
good hydrophilic properties of cellulose-deviated films if Formvar of
carbon is too hydrophobic to them (at the huge price of film instability in
the beam). I don't like glow-discharge, personally: I would rather use
poly-lysine coating. Have a great weekend, Sergey

At 05:39 PM 5/20/2004 -0700, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Fri May 21 16:18:31 2004

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Hi listers
I have a problem I am hoping that someone out there can help me with.
7 years ago our lab jointly bought a Photometrix SenSys PVCAM with
another lab. The labs are splitting up. We need to determine the
current value of the camera so that one lab can pay the other lab. Can
anybody point me to this data?
Thanx
David

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 17:29:47 2004

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Hi -

We have been using the Epson Perfection 3200 scanner for 8x10 cm TEM
negatives for about a year now, and find it excellent. The
resolution (3200 dpi optical) is almost as good as the 4000 dpi on
the Nikon 8000 etc., and we successfully scanned some very dense
(accidentally overexposed) negatives when our TEM's exposure meter
went on the fritz. We mount the negatives in the standard 4x5"
negative carrier. (The Nikon negative holder doesn't fit 8x10 cm
negatives without modification, or cutting the negatives down to
size.) The 3200 was listed at $299 on the Epson website the last
time I looked.

Cheers,
Tom Kosel

Original message:

Hello Listers,

I wanted to see if anyone has had any experience scanning negatives
with the Canon Canoscan 9900F.
I have a low end Canoscan that I use for documents and the occasional
photograph, which has given me
very good results, but is not set up for negatives. I have seen the
recent posts about the Epson scanner,
but I am trying to keep it under a $1000 so that I do not have to
treat it as a capital purchase. I have tried
for the last two years to get a Coolscan 8000 on the capital budget
with no luck, and do not see any scanner
above $1000 as an option right now.

Thanks,
Steve

Steven Lee
Chief Technologists
Electron Microscopy Laboratory
Baylor University Medical Center
3500 Gaston Ave
Dallas, TX 750246
Ph: 214.820.3302
Fx: 214.820.4110
Em: stevenle-at-baylorhealth.edu
--
*********************************
Thomas H. Kosel
Department of Electrical Engineering
University of Notre Dame
Notre Dame, IN 46556
(574) 631-5642 (201 Cushing)
(574) 631-4393 FAX
kosel-at-nd.edu
*********************************

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 19:08:23 2004

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Hi,

I want to find some papers or books which introduce the determination of
the direction of dislocation lines by TEM.

Thank you very much,

Regards,

Nina

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 02:05:24 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

"Electron Microscopy of Thin Crystals"
Hirsch, Howie, Nicholson, Pashley & Whelan
Pub: Robert E. Krieger
ISBN: 0-88275-376-2

"Transmission Electron Microscopy of Materials"
Thomas & Goringe
Pub: John Wiley & Sons
ISBN: 0-471-12244-0

"Defect Analysis in Electron Microscopy"
Loretto & Smallman
Pub: Chapman & Hall
ISBN: 0-470-54760-X

The latter, in particular, is quite detailed about dislocation
analysis with specific instructions. It also gives details of
weak-beam methods, which give much higher resolution images of
dislocations, very useful if you have closely packed dislocations.

Unfortunately, I suspect all are no longer in print.
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail
will automatically be deleted.
:-)

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 04:58:19 2004

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Dear microscopist experts,

When I read literatures, I have been all the time
confused by the resolution definition in transmission
electron microscopy. Could you please kindly help?

For a FEG-HRTEM, what is the "line resolution" as
opposed to the "information resolution"? What is the
difference between each other?

How could I achieve the "line resolution" and the
"information resolution" in TEM experiments? And, how
can I resolve (identify, or "see") the "line
resolution" and the "information resolution"
respectively from a state-of-the-art HREM image?

Thank you for your time. Wish you a nice weekend,

-Juha

__________________________________
Do you Yahoo!?
Yahoo! Domains – Claim yours for only $14.70/year
http://smallbusiness.promotions.yahoo.com/offer

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 09:13:06 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (antuni-at-aol.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, May 21, 2004 at 16:19:26
---------------------------------------------------------------------------

Email: antuni-at-aol.com
Name: Anthony Ribaudo

Organization: Consultant

Title-Subject: [Microscopy] [Filtered] Identifying Asbestos Using ptical Microscopy

Question: Can one identify asbestos only utilizing optical microscopy without the aid of electron diffraction/TEM ?

Anthony Ribaudo

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 09:14:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (christian_b_a-at-hotmail.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Friday, May 21, 2004 at 09:07:25
---------------------------------------------------------------------------

Email: christian_b_a-at-hotmail.com
Name: christian albano

Organization: Neuropsychiatric Research Institute

Education: Graduate College

Location: Fargo, ND, USA

Question: Does using the Fluoview Olympus LSCM for non-floresence degrade the equipment lifetime?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 11:52:37 2004

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Warning: Non scientific answer:

I remember an edition of "This Old House" or one of those types of shows
where they took some shingle samples to a lab for testing.

The lab used polarized microscopy to do at least an "initial" screening
and determine that the shingles "most likely" contained asbestos.

The "would do some additional testing" to verify (it was, and the house
needed to have a tent built around it, etc., etc.). I assume the
additional testing was something along the lines of TEM, etc.

The conclusion I drew was that if you had materials that you were
expecting asbestos, this (polarized examination) was a good screening
tool. If the fibers didn't change from one specific color to another as
the analyzer was rotated, you didn't have asbestos. If they did, you
probably have asbestos, but there are other fibers that may do the same
thing.

These were also fibers, not dust, and I don't know if that would affect
the results or not.

Sorry if this wasn't useful.

John R.

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
Sent: Saturday, May 22, 2004 9:23 AM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (antuni-at-aol.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday,
May 21, 2004 at 16:19:26
------------------------------------------------------------------------
---

Email: antuni-at-aol.com
Name: Anthony Ribaudo

Organization: Consultant

Title-Subject: [Microscopy] [Filtered] Identifying Asbestos Using ptical
Microscopy

Question: Can one identify asbestos only utilizing optical microscopy
without the aid of electron diffraction/TEM ?

Anthony Ribaudo

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 16:00:20 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Only one of the forms of asbestos is harmful to humans. Chrysotile
and then only if it is inhaled and the particle size is such it
lodges in the lung so it can form a site for cancer to get a start.
Chrysotile is only a small percentage of asbestos and the particle
size must fall in the 5 to 15 micron range to stay in the lungs.

These conditions are almost only found in asbestos worker and miners
and not in the general public. In the case of high exposure to
asbestos cigarette smoking is also a very large contributor to the
cancer caused by asbestos.

Had the asbestos studies been allowed to be fully peer reviewed
before legislation was passed we would probably still be using
asbestos in many applications today with more protection for
asbestos workers and minors and restrictions on some products such
as asbestos powder and asbestos cloth. Unfortunately the legislators
won't review thier laws once they are passed and the western world
is spending needless billions of dollars in asbestos abatement in
every old building that is renovated.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Chiphead" {chiphead-at-sbcglobal.net}

:
: Warning: Non scientific answer:
:
: I remember an edition of "This Old House" or one of those types of
shows
: where they took some shingle samples to a lab for testing.
:
: The lab used polarized microscopy to do at least an "initial"
screening
: and determine that the shingles "most likely" contained asbestos.
:
: The "would do some additional testing" to verify (it was, and the
house
: needed to have a tent built around it, etc., etc.). I assume the
: additional testing was something along the lines of TEM, etc.
:
: The conclusion I drew was that if you had materials that you were
: expecting asbestos, this (polarized examination) was a good
screening
: tool. If the fibers didn't change from one specific color to
another as
: the analyzer was rotated, you didn't have asbestos. If they did,
you
: probably have asbestos, but there are other fibers that may do the
same
: thing.
:
: These were also fibers, not dust, and I don't know if that would
affect
: the results or not.
:
: Sorry if this wasn't useful.
:
: John R.
:
: -----Original Message-----
: } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
: Sent: Saturday, May 22, 2004 9:23 AM
: To: microscopy-at-ns.microscopy.com
: Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
: Microscopy
:
:
:
: ------------------------------------------------------------------
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: Below is the result of your feedback form (NJZFM-ultra-55). It
was
: submitted by (antuni-at-aol.com) from
: http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday,
: May 21, 2004 at 16:19:26
: ------------------------------------------------------------------
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: ---
:
: Email: antuni-at-aol.com
: Name: Anthony Ribaudo
:
: Organization: Consultant
:
: Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
Using ptical
: Microscopy
:
: Question: Can one identify asbestos only utilizing optical
microscopy
: without the aid of electron diffraction/TEM ?
:
:
: Anthony Ribaudo
:
:
:
: ------------------------------------------------------------------
------
: ---
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 09:31:26 2004

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This is off the topic of identifying asbestos, but thought I should comment
that just yesterday there was a program on the radio (streaming audio
available at http://www.abc.net.au/rn/talks/bbing/, transcript available by
Thursday) about new cases of asbestosis and mesothelioma showing up. The
young people (20s and 30s) now getting this lived in high asbestos areas as
kids, were children of builders (and builders themselves) who demolished or
renovated fibro houses, etc. Perhaps just an Australian problem....
Rosemary

} From: "Gordon Couger" {gcouger-at-provalue.net}
} Date: Sat, 22 May 2004 16:09:06 -0500
} To: "Chiphead" {chiphead-at-sbcglobal.net} , "'by way of MicroscopyListserver'"
} {antuni-at-aol.com} , {microscopy-at-ns.microscopy.com}
} Subject: [Microscopy] Re: RE: viaWWW: Identifying Asbestos Using ptical
} Microscopy
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Only one of the forms of asbestos is harmful to humans. Chrysotile
} and then only if it is inhaled and the particle size is such it
} lodges in the lung so it can form a site for cancer to get a start.
} Chrysotile is only a small percentage of asbestos and the particle
} size must fall in the 5 to 15 micron range to stay in the lungs.
}
} These conditions are almost only found in asbestos worker and miners
} and not in the general public. In the case of high exposure to
} asbestos cigarette smoking is also a very large contributor to the
} cancer caused by asbestos.
}
} Had the asbestos studies been allowed to be fully peer reviewed
} before legislation was passed we would probably still be using
} asbestos in many applications today with more protection for
} asbestos workers and minors and restrictions on some products such
} as asbestos powder and asbestos cloth. Unfortunately the legislators
} won't review thier laws once they are passed and the western world
} is spending needless billions of dollars in asbestos abatement in
} every old building that is renovated.
}
} Gordon
} Gordon Couger gcc-at-couger.com
}
} I collect links on information related to light microscopes.
} http://www.couger.com/microscope/links/gclinks.html
} Please forward any links or information you think might be useful to
} others.
} Microscope Manual at www.science-info.org
}
} } From: "Chiphead" {chiphead-at-sbcglobal.net}
}
} :
} : Warning: Non scientific answer:
} :
} : I remember an edition of "This Old House" or one of those types of
} shows
} : where they took some shingle samples to a lab for testing.
} :
} : The lab used polarized microscopy to do at least an "initial"
} screening
} : and determine that the shingles "most likely" contained asbestos.
} :
} : The "would do some additional testing" to verify (it was, and the
} house
} : needed to have a tent built around it, etc., etc.). I assume the
} : additional testing was something along the lines of TEM, etc.
} :
} : The conclusion I drew was that if you had materials that you were
} : expecting asbestos, this (polarized examination) was a good
} screening
} : tool. If the fibers didn't change from one specific color to
} another as
} : the analyzer was rotated, you didn't have asbestos. If they did,
} you
} : probably have asbestos, but there are other fibers that may do the
} same
} : thing.
} :
} : These were also fibers, not dust, and I don't know if that would
} affect
} : the results or not.
} :
} : Sorry if this wasn't useful.
} :
} : John R.
} :
} : -----Original Message-----
} : } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
} : Sent: Saturday, May 22, 2004 9:23 AM
} : To: microscopy-at-ns.microscopy.com
} : Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
} : Microscopy
} :
} :
} :
} : ------------------------------------------------------------------
} ------
} : ------
} : The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} : To Subscribe/Unsubscribe --
} : http://www.msa.microscopy.com/MicroscopyListserver
} : On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} : ------------------------------------------------------------------
} ------
} : -------
} :
} : Below is the result of your feedback form (NJZFM-ultra-55). It
} was
} : submitted by (antuni-at-aol.com) from
} : http://microscopy.com/MicroscopyListserver/MLFormMail.html on
} Friday,
} : May 21, 2004 at 16:19:26
} : ------------------------------------------------------------------
} ------
} : ---
} :
} : Email: antuni-at-aol.com
} : Name: Anthony Ribaudo
} :
} : Organization: Consultant
} :
} : Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
} Using ptical
} : Microscopy
} :
} : Question: Can one identify asbestos only utilizing optical
} microscopy
} : without the aid of electron diffraction/TEM ?
} :
} :
} : Anthony Ribaudo
} :
} :
} :
} : ------------------------------------------------------------------
} ------
} : ---
} :
} :
} :
} :
} :
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 09:50:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Listers,

Sorry, I forgot to state that the cryoholder we're looking for would
be for a Hitachi S-900 in-lens FESEM, which uses a Hitachi TEM holder.

Phil
--
Philip Oshel
Supervisor, AMFSC and BBPIC microscopy facilities
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 11:14:18 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Gordon,

It is hard to believe other forms of asbestos: amosite asbestos(grunerite), actinolite-tremolite asbestos, anthophyllite (asbestos)and crocidolite asbestos(riebeckite) are not harmful. Have any studies been done on this? Chrysotile asbestos makes up to +90% of all asbestos in North America. (please correct if somebody has published figures on this).

Asbestos has been linked to mesothelioma and, also, asbestos is the cause of asbestosis(also harmful to humans). Isn't it?

I agree. If asbestos studies had been fully reviewed we would still using asbestos it has unique chemical and physical properties, especially for a mineral. The politicians used asbestos as a political football first scaring the public then passing legislation covering asbestos in schools, AHERA. Yes many problems have occurred as a result of this. The regulation should be reviewed and changed(if if hasn't already been).

Yes, asbestos can be identified by polarized light microscopy, not OLM or PCM. Using dispersion staining techniques to determine refractive indices, a properly prepared asbestos fiber can be identified, by PLM. Other measured properties: pleochroism, sign of elongation, and angle of extinction plus physical characteristic further aid the PLM analyst in the proper identification. Preparation of the fiber and proper training of the analyst are the critical factors here. Binder/matrix effects may hinder the analysis, for example chrysotile in vinyl floor tile.

Where are all the McCrone(ies) on this? Maybe this subject has been hashed out in the past. If so pardon me for the repeated redundancy.

Regards,

Timothy J. Bard, Scientist
Scanning Electron Microscopy
OSRAM SYLVANIA
Towanda, PA

U

-----Original Message-----
} From: Gordon Couger [mailto:gcouger-at-provalue.net]
Sent: Saturday, May 22, 2004 5:09 PM
To: Chiphead; 'by way of MicroscopyListserver';
microscopy-at-ns.microscopy.com

Only one of the forms of asbestos is harmful to humans. Chrysotile
and then only if it is inhaled and the particle size is such it
lodges in the lung so it can form a site for cancer to get a start.
Chrysotile is only a small percentage of asbestos and the particle
size must fall in the 5 to 15 micron range to stay in the lungs.

These conditions are almost only found in asbestos worker and miners
and not in the general public. In the case of high exposure to
asbestos cigarette smoking is also a very large contributor to the
cancer caused by asbestos.

Had the asbestos studies been allowed to be fully peer reviewed
before legislation was passed we would probably still be using
asbestos in many applications today with more protection for
asbestos workers and minors and restrictions on some products such
as asbestos powder and asbestos cloth. Unfortunately the legislators
won't review their laws once they are passed and the western world
is spending needless billions of dollars in asbestos abatement in
every old building that is renovated.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Chiphead" {chiphead-at-sbcglobal.net}

:
: Warning: Non scientific answer:
:
: I remember an edition of "This Old House" or one of those types of
shows
: where they took some shingle samples to a lab for testing.
:
: The lab used polarized microscopy to do at least an "initial"
screening
: and determine that the shingles "most likely" contained asbestos.
:
: The "would do some additional testing" to verify (it was, and the
house
: needed to have a tent built around it, etc., etc.). I assume the
: additional testing was something along the lines of TEM, etc.
:
: The conclusion I drew was that if you had materials that you were
: expecting asbestos, this (polarized examination) was a good
screening
: tool. If the fibers didn't change from one specific color to
another as
: the analyzer was rotated, you didn't have asbestos. If they did,
you
: probably have asbestos, but there are other fibers that may do the
same
: thing.
:
: These were also fibers, not dust, and I don't know if that would
affect
: the results or not.
:
: Sorry if this wasn't useful.
:
: John R.
:
: -----Original Message-----
: } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
: Sent: Saturday, May 22, 2004 9:23 AM
: To: microscopy-at-ns.microscopy.com
: Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
: Microscopy
:
:
:
: ------------------------------------------------------------------
------
: ------
: The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
: To Subscribe/Unsubscribe --
: http://www.msa.microscopy.com/MicroscopyListserver
: On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
: ------------------------------------------------------------------
------
: -------
:
: Below is the result of your feedback form (NJZFM-ultra-55). It
was
: submitted by (antuni-at-aol.com) from
: http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday,
: May 21, 2004 at 16:19:26
: ------------------------------------------------------------------
------
: ---
:
: Email: antuni-at-aol.com
: Name: Anthony Ribaudo
:
: Organization: Consultant
:
: Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
Using ptical
: Microscopy
:
: Question: Can one identify asbestos only utilizing optical
microscopy
: without the aid of electron diffraction/TEM ?
:
:
: Anthony Ribaudo
:
:
:
: ------------------------------------------------------------------
------
: ---
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 12:48:22 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have a student in my lab who wants to do immunohist on mouse skin. He
is looking at RPA. His current protocol for RPA is on cells. He was
able to get skin from mice treated with BPDE, he fixed the small strips
of skin in 4% paraformaldehyde in Dulbecco's PBS. He fixed it for 20-24
hours, then put it in 70% ethanol followed by routine paraffin
embedding.
Was the fixation time too long? I always fixed for 4-6 hours tops.
Will this affect his immunohist?
Thanks for any help or advice on this.

Stacey Andringa

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 12:52:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I work in Cincinnati and we are experiencing our 17 year cicada
invasion. I have never worked with insects and I am interested in
fixing some for light microscopy. What fixative would work on them and
how do I fix them - remove wings, pierce abdomen, etc.? This is for fun
as much as education.
Thanks for your help.

Stacey Andringa

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 12:53:49 2004

Contents Retrieved from Microscopy Listserver Archives
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On May 22, 2004, at 3:07 AM, Juha Dapper wrote:

} For a FEG-HRTEM, what is the "line resolution" as
} opposed to the "information resolution"? What is the
} difference between each other?
}
} How could I achieve the "line resolution" and the
} "information resolution" in TEM experiments? And, how
} can I resolve (identify, or "see") the "line
} resolution" and the "information resolution"
} respectively from a state-of-the-art HREM image?
}
Dear Juha,
The line resolution is the closest distance between two edges that can
be resolved, and it can be pretty confusing. A better measure is point
resolution, which can be determined from the first zero of the contrast
transfer function at Shertzer focus. The information limit is the
farthest extent of the Thon rings that can be achieved. To determine
the point resolution, put a thin amorphous carbon specimen in the
scope, adjust the height to eucentric height, make sure the scope is
aligned as well as possible, go to a sufficiently high magnification so
that the spatial frequency of the expected point resolution is larger
than two--or better three--pixels (on a CCD, the actual elements, on
film, the grain separation or resolution of a scanner), then take an
image. Determine the power spectrum by taking the FFT of the
image--easy on a CCD; on film, scan with a high-resolution scanner,
then take the FFT. The spatial frequency of the first zero is the
point resolution of the image. The better the scope is adjusted and
the better the area of the specimen, the closer you will come to the
true resolution of the scope. The information limit is best seen by
shifting the image during the exposure. This produces Young's fringes
in the power spectrum, which makes the extent of the Thon rings easier
to see. The service engineers who set up our scopes used a switch
attached to a shift coil to do this test. In order to achieve the best
resolution and information transfer possible, make sure your scope is
as well aligned as possible. If your specimen is too thick, or
otherwise unsuitable, you may not achieve the specified performance, so
don't blame the equipment in this case. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 13:59:59 2004

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OK, you sucked me in to asbestos and so here goes...........

Almost all of the minerals in existence were identified and
characterized by PLM at one time. Not all of these mineral were done as
well as the rest but still PLM is a powerful tool in the hands of an
experienced and trained microscopist. All of the legally defined asbestos
can be identified by PLM. Dispersion staining is a very useful tool for
this purpose. Vinyl tile, mortar, ceiling tiles, fluffy insulation, wall
plaster, and black or gray or green mastic - sample prep remains the
kingpin of all microscopical analysis just as it is in all analytical
testing.

My understanding is the current alert limits were based on measurements
made in asbestos mines and mills and extended to "normal" areas. This
level may be too low and in my opinion is a result of political games. It
seems some people have extreme sensitivity to asbestos and develop terminal
conditions at very low exposure levels. It is also my understanding these
studies were originally based on adults who were exposed as young adults
and older. I have not seen studies bases on exposure of children to
asbestos. So were do we draw the line? Yes, smoking makes it 400X more
likely to develop health complications (at least that was the number quote
when I did my asbestos certification training in Ohio. Not everyone who
was exposed to high levels developed health complications. I had a boss
who crawled through asbestos rewiring naval ships as summer work. He was a
long term chain smoker, and he lived into his 80's.

Government regulations created a industry of abatement and identification.
I have had the good fortune to participate at the identification and
quantification level for a number of years. The thing to remember is it
doesn't matter your personal beliefs or current scientific data when you're
compiling with a law, it is what the law says it is.

"Bard, Timothy
J." To: "Gordon Couger" {gcouger-at-provalue.net} ,
{Timothy.Bard-at-SYL "Microscopy (E-mail)" {microscopy-at-ns.microscopy.com}
VANIA.com} cc:
Subject: [Microscopy] RE: viaWWW: Identifying
05/24/2004 12:26 Asbestos Using optical Microscopy
PM

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Gordon,

It is hard to believe other forms of asbestos: amosite asbestos(grunerite),
actinolite-tremolite asbestos, anthophyllite (asbestos)and crocidolite
asbestos(riebeckite) are not harmful. Have any studies been done on this?
Chrysotile asbestos makes up to +90% of all asbestos in North America.
(please correct if somebody has published figures on this).

Asbestos has been linked to mesothelioma and, also, asbestos is the cause
of asbestosis(also harmful to humans). Isn't it?

I agree. If asbestos studies had been fully reviewed we would still using
asbestos it has unique chemical and physical properties, especially for a
mineral. The politicians used asbestos as a political football first
scaring the public then passing legislation covering asbestos in schools,
AHERA. Yes many problems have occurred as a result of this. The
regulation should be reviewed and changed(if if hasn't already been).

Yes, asbestos can be identified by polarized light microscopy, not OLM or
PCM. Using dispersion staining techniques to determine refractive indices,
a properly prepared asbestos fiber can be identified, by PLM. Other
measured properties: pleochroism, sign of elongation, and angle of
extinction plus physical characteristic further aid the PLM analyst in the
proper identification. Preparation of the fiber and proper training of the
analyst are the critical factors here. Binder/matrix effects may hinder
the analysis, for example chrysotile in vinyl floor tile.

Where are all the McCrone(ies) on this? Maybe this subject has been hashed
out in the past. If so pardon me for the repeated redundancy.

Regards,

Timothy J. Bard, Scientist
Scanning Electron Microscopy
OSRAM SYLVANIA
Towanda, PA

U

-----Original Message-----
} From: Gordon Couger [mailto:gcouger-at-provalue.net]
Sent: Saturday, May 22, 2004 5:09 PM
To: Chiphead; 'by way of MicroscopyListserver';
microscopy-at-ns.microscopy.com

Only one of the forms of asbestos is harmful to humans. Chrysotile
and then only if it is inhaled and the particle size is such it
lodges in the lung so it can form a site for cancer to get a start.
Chrysotile is only a small percentage of asbestos and the particle
size must fall in the 5 to 15 micron range to stay in the lungs.

These conditions are almost only found in asbestos worker and miners
and not in the general public. In the case of high exposure to
asbestos cigarette smoking is also a very large contributor to the
cancer caused by asbestos.

Had the asbestos studies been allowed to be fully peer reviewed
before legislation was passed we would probably still be using
asbestos in many applications today with more protection for
asbestos workers and minors and restrictions on some products such
as asbestos powder and asbestos cloth. Unfortunately the legislators
won't review their laws once they are passed and the western world
is spending needless billions of dollars in asbestos abatement in
every old building that is renovated.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Chiphead" {chiphead-at-sbcglobal.net}

:
: Warning: Non scientific answer:
:
: I remember an edition of "This Old House" or one of those types of
shows
: where they took some shingle samples to a lab for testing.
:
: The lab used polarized microscopy to do at least an "initial"
screening
: and determine that the shingles "most likely" contained asbestos.
:
: The "would do some additional testing" to verify (it was, and the
house
: needed to have a tent built around it, etc., etc.). I assume the
: additional testing was something along the lines of TEM, etc.
:
: The conclusion I drew was that if you had materials that you were
: expecting asbestos, this (polarized examination) was a good
screening
: tool. If the fibers didn't change from one specific color to
another as
: the analyzer was rotated, you didn't have asbestos. If they did,
you
: probably have asbestos, but there are other fibers that may do the
same
: thing.
:
: These were also fibers, not dust, and I don't know if that would
affect
: the results or not.
:
: Sorry if this wasn't useful.
:
: John R.
:
: -----Original Message-----
: } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
: Sent: Saturday, May 22, 2004 9:23 AM
: To: microscopy-at-ns.microscopy.com
: Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
: Microscopy
:
:
:
: ------------------------------------------------------------------
------
: ------
: The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
: To Subscribe/Unsubscribe --
: http://www.msa.microscopy.com/MicroscopyListserver
: On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
: ------------------------------------------------------------------
------
: -------
:
: Below is the result of your feedback form (NJZFM-ultra-55). It
was
: submitted by (antuni-at-aol.com) from
: http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday,
: May 21, 2004 at 16:19:26
: ------------------------------------------------------------------
------
: ---
:
: Email: antuni-at-aol.com
: Name: Anthony Ribaudo
:
: Organization: Consultant
:
: Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
Using ptical
: Microscopy
:
: Question: Can one identify asbestos only utilizing optical
microscopy
: without the aid of electron diffraction/TEM ?
:
:
: Anthony Ribaudo
:
:
:
: ------------------------------------------------------------------
------
: ---
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 14:15:01 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Juha,

There are three commonly employed definitions of "HRTEM resolution". All depend on
how information is transferred by the objective lens from the specimen
"exit-surface wave" to the image intensity spectrum (the Fourier transform of the
image intensity).

(1) "Fringe" resolution, or "line" resolution (sometimes called "lattice-plane"
resolution), is measured from the highest spatial frequency that is present in the
image intensity spectrum (and is thus detectable in the optical diffractogram). It
may include non-physical detail, since it may include components from a
"second-order" or "non-linear" interference generating a half-spacing term with
spatial frequency up to twice that of the highest-frequency diffracted beam passed
by the objective aperture and the convergence cross-coefficient envelope
["Resolution-damping functions in non-linear images", M.A. O'Keefe, in 37th Ann.
Proc. EMSA, San Antonio, Texas (1979) 556-557]. For a properly aligned microscope,
it is not affected by microscope spread-of-focus and depends only on factors such
as vibration or detector MTF.

(2) "Linear-image" resolution, or "information-limit" resolution, is measured by
the highest spatial frequency transferred linearly from the amplitude spectrum (the
specimen "exit-surface wave") to the image intensity spectrum with any old phase.
Transferred frequencies fall within one or more passbands, but other (lower)
frequencies may be blocked. Increased underfocus will push the convergence-limited
damping function to higher frequencies, thus this limit (often called just the
"information limit") to point resolution is a function of microscope
spread-of-focus. Spread of focus is a function of objective lens chromatic
aberration and variations in lens current and in electron beam energy (and of
vertical vibration of the specimen within the lens).

(3) "Scherzer" resolution, or "structure-image" resolution (sometimes called
"point" resolution or "point-to-point" resolution) is measured by the highest
linearly-transferred spatial
frequency that can be passed when no lower frequencies are blocked or passed with
opposite phase. The Scherzer image is important because it is (an approximation
to) a projection of the specimen structure (to a limited resolution) in the
direction of the incident beam. For images obtained at the Scherzer "optimum"
defocus, the Scherzer resolution is generally defined by the upper limit of the
low-frequency same-phase passband. Scherzer resolution is a function of objective
lens spherical aberration and electron wavelength.

FEG-HRTEMs can transfer spatial frequencies out to quite high values (their
information limits are much better than their Scherzer resolutions). Since we
know how linear transfer varies with objective lens defocus, we can use a series of
images to produce a single reconstructed image containing correctly-phased
components all the way out to the microscope information limit [see work by Van
Dyck, Coene and Thust]. The latest issue of Microscopy Today shows an example of a
reconstructed image with 0.78 Angstrom resolution, although the microscope used has
a Scherzer resolution of only 1.7 Angstrom.

While the phases of linearly-transferred image components can be corrected so they
can be used to extend resolution out to the microscope information limit, the
non-lnear components that create the "fringe resolution" usually transfer no new
information. These "cross-aperture" components can be frequency-doubled -- for
example, a 200 beam from the specimen may interfere with a -200 beam to create a
400 image component. Then we will see spacings of a/4 in the image even though no
information about the a/4 spacing was transferred from the specimen. If we managed
to "dis-entangle" the image's non-linear 400 component with its a/4 spacing, it
would still only provide us with information on a/2 spacings in the specimen.

So the short answer to your question is -- the difference between "line resolution"
as opposed to the "information resolution" is that an image can contain specimen
information out to the "information resolution", but any finer image spacings --
out to the "line resolution" -- are not new information about the specimen, but
were generated by non-linear interferences in the objective lens.

Mike O'Keefe

Juha Dapper wrote:

} ------------------------------------------------------------------------------
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} -------------------------------------------------------------------------------
}
} Dear microscopist experts,
}
} When I read literatures, I have been all the time
} confused by the resolution definition in transmission
} electron microscopy. Could you please kindly help?
}
} For a FEG-HRTEM, what is the "line resolution" as
} opposed to the "information resolution"? What is the
} difference between each other?
}
} How could I achieve the "line resolution" and the
} "information resolution" in TEM experiments? And, how
} can I resolve (identify, or "see") the "line
} resolution" and the "information resolution"
} respectively from a state-of-the-art HREM image?
}
} Thank you for your time. Wish you a nice weekend,
}
} -Juha
}
}
}
}
} __________________________________
} Do you Yahoo!?
} Yahoo! Domains – Claim yours for only $14.70/year
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From MicroscopyL-request-at-ns.microscopy.com Mon May 24 15:36:21 2004

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I have a water chiller from 1996 (Haskris RO75 with B H M + T options).

On checking the water level today, I noticed that the water was a bit green and
hence needed to be changed.
I drained the water storage tank, removed the nylon strainer,
replaced it with a clean spare
and as luck would have it I also needed to change the drain hose.

From experience I knew that when I first change the water, there is
normally a rinsing out
of the system and a noticeable amount of algae (? greenish gunk)
comes out of the discharge
pipe and I change the water another time before adding the
anti-algecid and closing up the system.

Today I got some air into the system and when I turned it back on the
water turned so turbid
that I could not see the bottom coils in the tank. I repeated the
draining/filling cycle at least
8 times until there was only a slight greenish cast to the water and
I gave up until tomorrow.

Does anyone have any idea why this would happen now and not before?
Is there any way that I can be assured that I have removed as much of
the algae from the
system as I can, other than to keep changing the water as long as I
can see small clumps
coming out into the water tank?

Thanks in advance,
Pat Connelly
Dept. of Biology
Univ. of PA
Philadelphia, PA 19104

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 15:48:37 2004

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Hi, Timothy:

I seem to recollect that Neal Rowlands, who was Shared Experimental
Facilities Manager in our Center some years ago, had done some asbestos
research at McGill U. along the lines of your question. I recall him
saying that the difference in lung damage caused by different forms of
asbestos had to do with the difference in crystal shape. The tiny-needle
shape was the nastiest.

Best regards,

Libby Shaw

} Subject: [Microscopy] RE: viaWWW: Identifying Asbestos Using optical
} Microscopy
} Date: Mon, 24 May 2004 12:26:01 -0400
} From: "Bard, Timothy J." {Timothy.Bard-at-SYLVANIA.com}
} To: "Gordon Couger" {gcouger-at-provalue.net} ,
} "Microscopy (E-mail)" {microscopy-at-ns.microscopy.com}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Address: MIT Room 13-4149 Tel: 617-253-5045
77 Massachusetts Avenue Email: elshaw-at-mit.edu
Cambridge, MA 02139 Fax: 617-258-6478
http://web.mit.edu/cmse/www/
****************************************************************

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 01:05:16 2004

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To Students attending M&M2004 in Savannah,
If you are a student that will be attending (or would like
to the attend) the M&M meeting in Savannah this summer, we
would appreciate your help by assisting at the sessions.
You would be volunteering as a "projectionist" for various
sessions, most likely ones you would attend anyway. There
is a training session Sunday afternoon (details when you
volunteer).

What are the benefits of volunteering? Volunteers will be
given free registration--a badge, opening night reception
ticket and a CD of the abstracts.

Who to contact:
John Shields (see address below) at jshields-at-cb.uga.edu

--
John Shields
E.M. Lab, 151 Barrow Hall
University of Georgia
Athens, GA 30602
706-542-4080

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 03:13:08 2004

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Hi,

I just want to get this clear and look at the consequences of what you
write.

If a nonlinear component of frequency 2f is present in an image, will it
have been damped by the ctf-envelope just like the corresponding linear
component of frequency f? In that case the presence of a high-resolution
component doesn't say much about the quality of a microscope or a
micrograph as long as it is unclear whether the component is linear or
frequency doubled.
Now for the practical consequences:
With what sort of specimens would you expect frequency doubling? Could
it happen with protein crystals (10-20 nm thick) using a 200 or 300 kV
microscope?

Philip

-----Original Message-----
} From: Michael O'Keefe [mailto:MAOKeefe-at-lbl.gov]

(1) "Fringe" resolution, or "line" resolution (sometimes called
"lattice-plane" resolution), is measured from the highest spatial
frequency that is present in the image intensity spectrum (and is thus
detectable in the optical diffractogram). It may include non-physical
detail, since it may include components from a "second-order" or
"non-linear" interference generating a half-spacing term with spatial
frequency up to twice that of the highest-frequency diffracted beam
passed by the objective aperture and the convergence cross-coefficient
envelope

While the phases of linearly-transferred image components can be
corrected so they can be used to extend resolution out to the microscope
information limit, the non-linear components that create the "fringe
resolution" usually transfer no new information. These "cross-aperture"
components can be frequency-doubled -- for example, a 200 beam from the
specimen may interfere with a -200 beam to create a 400 image component.
Then we will see spacings of a/4 in the image even though no information
about the a/4 spacing was transferred from the specimen. If we managed
to "dis-entangle" the image's non-linear 400 component with its a/4
spacing, it would still only provide us with information on a/2 spacings
in the specimen.

So the short answer to your question is -- the difference between "line
resolution" as opposed to the "information resolution" is that an image
can contain specimen information out to the "information resolution",
but any finer image spacings -- out to the "line resolution" -- are not
new information about the specimen, but were generated by non-linear
interferences in the objective lens.

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 05:02:13 2004

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On May 24, 2004, at 1:48 PM, Pat Connelly wrote:

} From experience I knew that when I first change the water, there is
} normally a rinsing out
} of the system and a noticeable amount of algae (? greenish gunk) comes
} out of the discharge
} pipe and I change the water another time before adding the
} anti-algecid and closing up the system.
}
Dear Pat,
Are you sure that the gunk is algae and not Cu oxide? If the latter,
you should consider adding a corrosion inhibitor to the water.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 06:08:07 2004

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Hi,

I thought some people might be interested in a follow-up of this
discussion.
(Don't tell me if your not, just ignore me.)

I've taken some images of carbon film on our CM120 with a brand new
LaB6-filament just to get an idea of the limitations of this microscope.

I get information limits between 15 and 5 Angstrom depending on
magnification and defocus (only "biological" defocus values) and the
information limit does not improve with decreasing magnification as
suggested by CTF-explorer. In fact the opposite is true (at least for
constant exposure levels). Some similar data for a FEG would be
interesting.

One thing is clear: Reaching 10 Angstrom and slightly better should not
be a problem with a well maintained LaB6 microscope.

For the details see the link "reference data for the CM120" at
http://www.csb.ki.se/users/philip/philown.html. This is a big word file
so you have to be patient when you download it.

Philip

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 06:31:39 2004

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Hi Bill,

That's exactly what I was thinking, as well. Do you have any good
recommendations for use as a corrosion inhibitor?

Thanks,

David

David Bell
Scientist
Electron Microscopy Lab
Millipore Corporation
80 Ashby Road
Bedford, MA 01730
(781) 533-2108

Bill Tivol {tivol-at-caltech.edu}
05/24/2004 06:24 PM

To: microscopy-at-msa.microscopy.com
cc:
Subject: [Microscopy] [Detected by Millipore as possible Spam] Re: Haskris water
chiller/recycler

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

On May 24, 2004, at 1:48 PM, Pat Connelly wrote:

} From experience I knew that when I first change the water, there is
} normally a rinsing out
} of the system and a noticeable amount of algae (? greenish gunk) comes
} out of the discharge
} pipe and I change the water another time before adding the
} anti-algecid and closing up the system.
}
Dear Pat,
Are you sure that the gunk is algae and not Cu oxide? If
the latter,
you should consider adding a corrosion inhibitor to the water.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 07:53:51 2004

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Bill
I'm pretty sure I have Cu oxide along the walls of my Haskris
chiller as it won't come off. What corrosion inhibitor do you suggest
and how do I remove the Cu oxide already present?

Tony Greco

--
Anthony M. Greco
Electron Microscope Manager
College of Marine Science
University of South Florida
140 7th Avenue S.
St. Petersburg, Fl 33701

voice: (727) 553-1595
email: tgreco-at-marine.usf.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 08:53:39 2004

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I'm glad that this issue is still being addressed. I have a Haskris chiller
(since 1988) which services our Philips CM10 TEM. We continually have this
"green algae" in the water and which seems to collect around the filter unit
in the system. I have been concerned about this in the past, and asked our
service engineer, but it doesn't appear to impede the flow of water or the
operation of the chiller. (We have had other minor problems with the
chiller that B & G has fixed, but nothing connected to the water). I was
interested to hear about the possibility of it due to Cu oxide. I would
also like to know what corrosion inhibitor can be added to the water.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: David_Bell-at-millipore.com [mailto:David_Bell-at-millipore.com]
Sent: Tuesday, May 25, 2004 7:43 AM
To: Bill Tivol
Cc: microscopy-at-msa.microscopy.com

Hi Bill,

That's exactly what I was thinking, as well. Do you have any good
recommendations for use as a corrosion inhibitor?

Thanks,

David

David Bell
Scientist
Electron Microscopy Lab
Millipore Corporation
80 Ashby Road
Bedford, MA 01730
(781) 533-2108

Bill Tivol {tivol-at-caltech.edu}
05/24/2004 06:24 PM

To: microscopy-at-msa.microscopy.com
cc:
Subject: [Microscopy] [Detected by Millipore as possible
Spam] Re: Haskris water
chiller/recycler

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

On May 24, 2004, at 1:48 PM, Pat Connelly wrote:

} From experience I knew that when I first change the water, there is
} normally a rinsing out
} of the system and a noticeable amount of algae (? greenish gunk) comes
} out of the discharge
} pipe and I change the water another time before adding the
} anti-algecid and closing up the system.
}
Dear Pat,
Are you sure that the gunk is algae and not Cu oxide? If
the latter,
you should consider adding a corrosion inhibitor to the water.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 08:56:31 2004

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Thank you, Michael and Bill, for your kind reply. I
really appreciate your remarkable answers to my
questions.

After carefully reading your answers, I've got more
questions.

1. If the "line resolution" is so confusing and
untrustworthy, why TEM manufactures used to apply it
to claim the quality of a microscope?

2. If an HREM iamge was taken without a certain
objective aperture, how can we tell if a
high-frequency spacing present in the image (or the
corresponding spot in its FFT) is due to linear
transfer or just by "cross-aperture" non-linear
interference?

3. About the "non-linear interferences". Do they
happen already during the process of electron-specimen
interaction, or after the back-focal plane of the
objective lens during the electron wave propagation?

4. In Michael's email, it is said "Since we know how
linear transfer varies with objective lens defocus, we
can use a series of images to produce a single
reconstructed image containing correctly-phased
components all the way out to the microscope
information limit [see work by Van Dyck, Coene and
Thust]."

Did you mean that the reconstruction method using a
focal-series can only apply to the linear transfer
case, i.e. the case of a weak phase object? If not,
how the non-linear interference effects are treated?

5. In Bill's email, you mentioned that "The
information limit is best seen by shifting the image
during the exposure. This produces Young's fringes in
the power spectrum,".

Could you please tell me in more details about how to
"shift the image to produce Young's fringes"? This
may be very practical and helpful to me.

Again thank you very much for your instructions.

-juha

__________________________________
Do you Yahoo!?
Friends. Fun. Try the all-new Yahoo! Messenger.
http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 10:42:49 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society
of America On May 24, 2004, at 1:48 PM,
Pat Connelly {psconnel-at-sas.upenn.edu} wrote:
} } From experience I knew that when I first change the water,
there is normally a rinsing out of the system and
a noticeable amount of algae (? greenish gunk) comes out
of the discharge pipe and I change the water another time
before adding the anti-algecid and closing up the system. etc.
} }
} Dear Pat,
} Are you sure that the gunk is algae and not Cu oxide?
} If the latter, you should consider adding a corrosion
} inhibitor to the water.
} Bill Tivol, PhD
} EM Scientist and Manager
} Cryo-Electron Microscopy Facility
} Broad Center, Mail Code 114-96
} California Institute of Technology
} Pasadena CA 91125
} (626) 395-8833 tivol-at-caltech.edu
=======
Bill,
I took a sample from the fourth change of water and examined it
under a light microscope. I saw mostly tiny cellular clumps and
cellular sheets with a few very small, redish, spike like, crystals
embedded into them and that is why I thought of algae.
I do agree that the green color most likely comes from the copper
because there is no light in the system for photosynthesis.
I have sprinkled dichlorophene onto the water each time that
I have changed it since the first fill-up. The label states that
it is both a fungicide and a bactericide.
As the water supply, I use reverse osmosis water and some
Philadelphia tap water so that there are some ions.
The ph of both sources is usually acid, running about pH 5.5.
I did not check the pH of the water that I drained yesterday
but after rinning overnight the water resevoir is now also at
pH 5.5.

I am interested in your response as to a corrosion inhibitor.
Pat Connelly

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 12:24:55 2004

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Rosemary;
My recollection from the asbestos work I did at Lockheed was
that most of the asbestos fibers could produce mesothelioma, but that in
North America, chrysotile is the predominant type of asbestos. Sources
of exposure vary, but the connection to mesothelioma was first noticed
after WWII when a significant population that also smoked heavily was
involved in refitting steam ships that had large amounts of asbestos
insulation. The death of actor Steve McQueen highlighted the fact that
even something like dirt bike riding in areas naturally high in asbestos
could lead to a high risk exposure.

John Mardinly
Intel

-----Original Message-----
} From: Rosemary White [mailto:Rosemary.White-at-csiro.au]
Sent: Sunday, May 23, 2004 4:28 PM
To: microscopy-at-msa.microscopy.com

This is off the topic of identifying asbestos, but thought I should
comment
that just yesterday there was a program on the radio (streaming audio
available at http://www.abc.net.au/rn/talks/bbing/, transcript available
by
Thursday) about new cases of asbestosis and mesothelioma showing up.
The
young people (20s and 30s) now getting this lived in high asbestos areas
as
kids, were children of builders (and builders themselves) who demolished
or
renovated fibro houses, etc. Perhaps just an Australian problem....
Rosemary

} From: "Gordon Couger" {gcouger-at-provalue.net}
} Date: Sat, 22 May 2004 16:09:06 -0500
} To: "Chiphead" {chiphead-at-sbcglobal.net} , "'by way of
MicroscopyListserver'"
} {antuni-at-aol.com} , {microscopy-at-ns.microscopy.com}
} Subject: [Microscopy] Re: RE: viaWWW: Identifying Asbestos Using
ptical
} Microscopy
}
}
}
}
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America
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------}
-
}
} Only one of the forms of asbestos is harmful to humans. Chrysotile
} and then only if it is inhaled and the particle size is such it
} lodges in the lung so it can form a site for cancer to get a start.
} Chrysotile is only a small percentage of asbestos and the particle
} size must fall in the 5 to 15 micron range to stay in the lungs.
}
} These conditions are almost only found in asbestos worker and miners
} and not in the general public. In the case of high exposure to
} asbestos cigarette smoking is also a very large contributor to the
} cancer caused by asbestos.
}
} Had the asbestos studies been allowed to be fully peer reviewed
} before legislation was passed we would probably still be using
} asbestos in many applications today with more protection for
} asbestos workers and minors and restrictions on some products such
} as asbestos powder and asbestos cloth. Unfortunately the legislators
} won't review thier laws once they are passed and the western world
} is spending needless billions of dollars in asbestos abatement in
} every old building that is renovated.
}
} Gordon
} Gordon Couger gcc-at-couger.com
}
} I collect links on information related to light microscopes.
} http://www.couger.com/microscope/links/gclinks.html
} Please forward any links or information you think might be useful to
} others.
} Microscope Manual at www.science-info.org
}
} } From: "Chiphead" {chiphead-at-sbcglobal.net}
}
} :
} : Warning: Non scientific answer:
} :
} : I remember an edition of "This Old House" or one of those types of
} shows
} : where they took some shingle samples to a lab for testing.
} :
} : The lab used polarized microscopy to do at least an "initial"
} screening
} : and determine that the shingles "most likely" contained asbestos.
} :
} : The "would do some additional testing" to verify (it was, and the
} house
} : needed to have a tent built around it, etc., etc.). I assume the
} : additional testing was something along the lines of TEM, etc.
} :
} : The conclusion I drew was that if you had materials that you were
} : expecting asbestos, this (polarized examination) was a good
} screening
} : tool. If the fibers didn't change from one specific color to
} another as
} : the analyzer was rotated, you didn't have asbestos. If they did,
} you
} : probably have asbestos, but there are other fibers that may do the
} same
} : thing.
} :
} : These were also fibers, not dust, and I don't know if that would
} affect
} : the results or not.
} :
} : Sorry if this wasn't useful.
} :
} : John R.
} :
} : -----Original Message-----
} : } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
} : Sent: Saturday, May 22, 2004 9:23 AM
} : To: microscopy-at-ns.microscopy.com
} : Subject: [Microscopy] viaWWW: Identifying Asbestos Using
ptical
} : Microscopy
} :
} :
} :
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} was
} : submitted by (antuni-at-aol.com) from
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} Friday,
} : May 21, 2004 at 16:19:26
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} : ---
} :
} : Email: antuni-at-aol.com
} : Name: Anthony Ribaudo
} :
} : Organization: Consultant
} :
} : Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
} Using ptical
} : Microscopy
} :
} : Question: Can one identify asbestos only utilizing optical
} microscopy
} : without the aid of electron diffraction/TEM ?
} :
} :
} : Anthony Ribaudo
} :
} :
} :
} : ------------------------------------------------------------------
} ------
} : ---
} :
} :
} :
} :
} :
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 12:56:12 2004

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Dear Listers,

Does anyone else think it might be a useful exercise to try and
establish expiration dates for chemicals used in microscopy labs? I
understand that chemicals "expire" based upon what they are, what use
they are intended for, how they are used, what level of
accuracy/repeatability/etc. is expected from their use, how they are
stored, and many other factors. I have also read Rande Kline's
discussion of the problem in the July/August 2000 Microscopy Today on
the difficulties of establishing such dates (recommended).

The problem is that some work requires lab certification and strict
laboratory guidelines requiring that all chemicals be labeled with
expiration dates----whether or not those dates have any meaningful or
consistent basis in "reality". So far, I've been unable to find any
such set of standards and my strong impression is that labs set up their
own arbitrary chemical rotation regimen.

It might reasonably be suggested that MSA could be a clearinghouse for
establishing such standards for microscopy-related research. If enough
people think this is a useful project, I would be willing (please
somebody, stop me!!) to volunteer to put together a draft proposal. As
a starter, it would be useful to know how other labs handle this issue
and why.

Any thoughts?

Thanks,
Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 13:36:42 2004

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I've had a similar problem with my chiller system, though mine got clogged
up pretty well before I figured out what was going on. The turbo pump in my
SEM was the culprit, I think. The water jacket on the turbo is aluminum and
there are lots of brass fittings in the Haskris and the heat sinks in the
SEM. I got a bunch of stuff that looked like green kitty litter out of the
system that proved to have high aluminum and copper levels in it. I think
there is some sort of an electrochemical gradient set up that causes some
sort of corrosion product to build up over time (I'm a biologist, not a
chemist). Small amounts of it look like green sand in the bottom of the
reservoir. I cleaned the bigger clogs out of the water jacket with
alternating dilute HCl and NaOH using a big syringe and Tygon tubing,
rinsing with DIW in between (Rube Goldberg lives on). It's been fine for a
few months now, but I keep an eye on the flow rates.

Robert Simmons

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 14:18:48 2004

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On May 25, 2004, at 4:43 AM, David_Bell-at-millipore.com wrote:

} That's exactly what I was thinking, as well. Do you have any good
} recommendations for use as a corrosion inhibitor?
}
Dear David,
When I was at Albany NY, we used a product called Aquatreet 42, a
Mo-based inhibitor, and, judging from measurements of the water flow
through the lenses each year, there was little corrosion build-up.
That product can be obtained in a minimum of 5 gal--enough to last a
lifetime--from Aqua Labs, Inc., P.O. Box 645, Amesbury MA 01913. I
just spoke recently with Tom Cass, (800) 343-0213, and they still sell
the product to people in your area. He also told me that Skasol makes
a comparable product for the West Coast people. David Marchman, (800)
839-1000, is the contact for Skasol, and Chris Killian, (310) 749-8807
is the technical person. I have no affiliation with Aqua except as a
satisfied customer, and none with Skasol except as a potentially
satisfied customer.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 14:25:29 2004

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Hi,
Try dissolving it in 10% HCl. If it disappears its a Cu compound.

Best Regards,

Steve

Steve Buckingham
Service Manager
Kratos Analytical Inc.,
100 Red Schoolhouse Road, Bldg A
Chestnut Ridge, NY 10977
ph (845) 426 6700 ext 202
fx (845) 818 {mailto:4095steve-at-kratos.com} 4095

steve-at-kratos.com

-----Original Message-----
} From: psconnel-at-sas.upenn.edu [mailto:psconnel-at-sas.upenn.edu]
Sent: Tuesday, May 25, 2004 11:54 AM
To: Bill Tivol
Cc: Microscopy-at-msa.microscopy.com

----------------------------------------------------------------------------
--
The Microscopy ListServer -- Sponsor: The Microscopy Society
of America On May 24, 2004, at 1:48 PM,
Pat Connelly {psconnel-at-sas.upenn.edu} wrote:
} } From experience I knew that when I first change the water,
there is normally a rinsing out of the system and
a noticeable amount of algae (? greenish gunk) comes out
of the discharge pipe and I change the water another time
before adding the anti-algecid and closing up the system. etc.
} }
} Dear Pat,
} Are you sure that the gunk is algae and not Cu oxide?
} If the latter, you should consider adding a corrosion
} inhibitor to the water.
} Bill Tivol, PhD
} EM Scientist and Manager
} Cryo-Electron Microscopy Facility
} Broad Center, Mail Code 114-96
} California Institute of Technology
} Pasadena CA 91125
} (626) 395-8833 tivol-at-caltech.edu
=======
Bill,
I took a sample from the fourth change of water and examined it
under a light microscope. I saw mostly tiny cellular clumps and
cellular sheets with a few very small, redish, spike like, crystals
embedded into them and that is why I thought of algae.
I do agree that the green color most likely comes from the copper
because there is no light in the system for photosynthesis.
I have sprinkled dichlorophene onto the water each time that
I have changed it since the first fill-up. The label states that
it is both a fungicide and a bactericide.
As the water supply, I use reverse osmosis water and some
Philadelphia tap water so that there are some ions.
The ph of both sources is usually acid, running about pH 5.5.
I did not check the pH of the water that I drained yesterday
but after rinning overnight the water resevoir is now also at
pH 5.5.

I am interested in your response as to a corrosion inhibitor.
Pat Connelly

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 14:33:40 2004

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On May 25, 2004, at 4:11 AM, Philip Koeck wrote:

} I get information limits between 15 and 5 Angstrom depending on
} magnification and defocus (only "biological" defocus values) and the
} information limit does not improve with decreasing magnification as
} suggested by CTF-explorer. In fact the opposite is true (at least for
} constant exposure levels). Some similar data for a FEG would be
} interesting.
}
Dear Philip,
One of the acceptance tests for our Tecnai F30H was that we had to see
30 Thon rings at 2 um underfocus on a thin C specimen, which is
slightly beyond the 0.34 nm graphite spacing. We redo this test
periodically to be sure that the coherence of the beam is still up to
par. In fact, the service engineers were able to get many more Thon
rings than that. The spec on the info limit is 0.14 nm, but we can't
get Thon rings that far out at 2 um underfocus. To get the 30 Thon
rings, one has to find a good area of the C film, so we don't expect
that good a performance for biological specimens.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 15:42:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (amcelwai-at-bucknell.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 25, 2004 at 14:55:05
---------------------------------------------------------------------------

Email: amcelwai-at-bucknell.edu
Name: Andrew

Organization: Bucknell University Biology Department

Title-Subject: [Microscopy] [Filtered] MListserver: New Text/Manual

Question: Hi all,

I am a graduate student at Bucknell University and I am currently studying amphibian physiology. My thesis project involves studying skeletal muscles and liver tissue using both transmission electron microscopy, and light microscopy. I am interested in learning about new techniques in microscopy, or histology and I was hoping that someone could recommend a book that covers curent methodologies and, or the best ways of doing histology/microscopy research. All of the literature I have is from the 70's and the 80's and some of my colleagues suggested to me that my sources of information are a tad bit outdated.

I would appreciate any feedback. Thanks.

-Andrew

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 17:22:31 2004

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Hi everyone

I need some help.

I have used nanoplast resin for the first time following instructions
provided with the kit. When I came to examine the sections I found there
had been poor infiltration. I would welcome any suggestions from people
that have worked with the resin that could resolve this plus any other help
tips. Do I need to do a resin infiltration series similar to Araldite. I
did email Pelco (manufacturer of the resin) about this but so far not had a
response.

thanks Therese

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 19:14:18 2004

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Dear Tony,

I had an Ice Wagon and a Nesslab chiller system. The green color you see
MIGHT BE algae. Everyone blames the green color on algae.

I know from chiller experience and being a chemist that copper pipes
corrode first to a black thin film of copper oxide material on the walls of
chiller copper pipes. Next a deposit of copper carbonate forms over the
initial copper oxide coating and on PE cartridge filters. The black color
only forms on copper surfaces.

Green deposits in chiller lines in my lab were always thicker AFTER going
through a diffusion pump. We had whole house filters before the DPs and
they collected a green scale. The lines between the filter and the DP
inlet were relatively clear of green deposits. Seems backwards, doesn't
it? FYI.

TESTING:
Remove the scale and look under a microscope as you add dilute HCl. If it
bubbles, it's most likely lime green copper carbonate, as I had. To find
out if it was copper and carboante, I would use the regular green water to
test for copper ions first. Take the green chiller solution and add HCl.
It will dissolve the turbidity and form a nice clear green solution. Add
enough ammonium hydroxide to make the solution fairly basic. If copper
ions are present, the solution will turn deep blue. Algae do not do this.
Next add more HCL and the solution will turn green again. If your solution
does this, it's copper carbonate. If you would like to reconfirm the blue
color again, you can repeat the NH4OH treatment on the same sample of
water. This reversible color change is not possible with algae. IMHO.

To test for carbonate, add some HCl to a new sample to just barely get a
clear solution. Adjust the pH to 7-9 with ammonium hydroxide. Don't use
NaOH as it has carbonate in it. Add some clear barium chloride solution to
this basic solution. Enough carbonate ions will remain dissolved to cause
a white precipitate of BaCO3 to form. That probably confirms the gas was
originally CO2. If you then add HCl, the white barium carbonate
precipitate disappears to form carbonic acid and barium chloride. This
chemical behavior confirms CO3 for sure.

If you find the problem is algae, then you can add a small amount of a
quaternary ammonium salt. This extremely long named chemical will end with
quaternary ammonium salt and can be bought at any swimming pool supply as
an algicide. Estimate the volume of your system and add the recommended
amount. As I recall, a quart treats about 5,000 to 10,000 gallons of pool
water. So you will add a very small amount, like teaspoons or tablespoons
of it. It will kill the algae, if that's really the problem. Any pool
owner can help you that uses iso-cyanurates for hypochlorous acid
(chlorine) disinfection. He might give you a few mls and save you the trip
to the pool store for a 40 year chiller supply of QAS long chained
surfactant.

You can state, "I have plastic pipes, so where is the copper coming from in
my system?" Our chiller coils were made of copper tubing and the reservoir
tank had copper tubing showing in our units. They're the source of the
copper ions. In our system we also had copper supply lines going to
various labs. A mistake! There are other copper sources too. Ask your
serviceman about potential EM sources like embedded lens cooling lines of
fittings.
Air is normally the source of the CO2 because the tank is normally open to
air.

} From experience, we learned the hard way to run distilled water. I then
put a tablespoon of bicarbonate of soda in the water in case the chiller
water tried to go acidic. This trace ion concentration cuts down on the
corrosive nature of pure distilled water. This bicarb is not necessary,
unless you know the pH in your system drops over time. "Isn't that the
source of the carbonate?" No, we had the problem when we used chloramine-T
and no bicarb. We used bicarb after we switched to distilled water for
trace ions and to slow down any decrease in pH.

You can get into a green color spiral with chloramine-T (CT). You add CT
and the water eventually turns green. You measure the available chlorine
after awhile and it's too low. You add more CT and the available chlorine
goes up. After some time the available chlorine drops and the green color
intensity increases. You add more CT. The water keeps 'growing algae' and
turning a darker green all the time. Copper levels continue to climb and
precipitate.
We went this route and finally I said, "There is no way we logically have
this bad an algae problem." I had saved samples along the way and so I ran
AA on them and did the blue-green test. I found out that the more CT we
added, the more the copper ion concentration increased along with the
darker green color. All this led me to the correct answer.
It's copper carbonate in the water and on the walls of the pipes, not algae!

We replaced the coppper lines to labs and I saved the green scale from
inside the copper pipes. After 4 years, the dried 'green algae' are still
green because the green scale is really copper carbonate.

Disclaimer: Some algae might be present with the carbonate but AA
confirmed the copper increased with CT addition and time. This green color
can develop with pure distilled water also. It just takes longer.

Everything you ever wanted to know about green chiller water but were
afraid to ask.

What do you do if you have reduced flow through your TEM or SEM lens
cooling lines, DP lines, rubber hoses, or electronic heat sinks? Check
with your serviceman. Let him do those jobs and assume the risk.

Paul Beauregard
Senior Research Associate
travail chasse

At 08:57 AM 05/25/04 -0400, Tony Greco wrote:
}
}
} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 04:18:27 2004

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That's another question I've just come across.

I have some test images (defocus around 1000 nm) from a FEG-TEM where
Young fringes seem to extend up to twice as far as Thon rings. Is that
usual and if so which of the two defines the information limit?
What do manufacturers mean by information limit?
Do Young fringes really show up to which resolution I can get useful
information from a micrograph?
At least in TEM of non-periodic biological specimens you normally don't
expect anything beyond the last clearly visible Thon ring.

Philip

-----Original Message-----
} From: Juha Dapper [mailto:juha_dapper-at-yahoo.com]

5. In Bill's email, you mentioned that "The
information limit is best seen by shifting the image
during the exposure. This produces Young's fringes in
the power spectrum,".

Could you please tell me in more details about how to
"shift the image to produce Young's fringes"? This
may be very practical and helpful to me.

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 05:21:43 2004

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I think this is a good idea. I am still using chemicals
that predate my start here (1989). I had to renew some
sodium phosphate this year when the plastic container
disintegrated! More seriously I have started making up
sodium cacodylate 0.2M stock and adding a set volume of HCL
(from Glauert's book) just before use. As my flagon of HCL
is over 15yrs old I replaced it this week with a supply
from a lab with a higher turnover. I plan to replace the
HCL annually unless someone comes up with an informed
suggestion!

Dave

On Tue, 25 May 2004 13:08:29 -0500 "Tindall, Randy D."
{TindallR-at-missouri.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear Listers,
}
} Does anyone else think it might be a useful exercise to try and
} establish expiration dates for chemicals used in microscopy labs? I
} understand that chemicals "expire" based upon what they are, what use
} they are intended for, how they are used, what level of
} accuracy/repeatability/etc. is expected from their use, how they are
} stored, and many other factors. I have also read Rande Kline's
} discussion of the problem in the July/August 2000 Microscopy Today on
} the difficulties of establishing such dates (recommended).
}
} The problem is that some work requires lab certification and strict
} laboratory guidelines requiring that all chemicals be labeled with
} expiration dates----whether or not those dates have any meaningful or
} consistent basis in "reality". So far, I've been unable to find any
} such set of standards and my strong impression is that labs set up their
} own arbitrary chemical rotation regimen.
}
} It might reasonably be suggested that MSA could be a clearinghouse for
} establishing such standards for microscopy-related research. If enough
} people think this is a useful project, I would be willing (please
} somebody, stop me!!) to volunteer to put together a draft proposal. As
} a starter, it would be useful to know how other labs handle this issue
} and why.
}
} Any thoughts?
}
} Thanks,
} Randy
}
} Randy Tindall
} EM Specialist
} Electron Microscopy Core Facility---We Do Small Well!
} W122 Veterinary Medicine
} University of Missouri
} Columbia, MO 65211
} Tel: (573) 882-8304
} Fax: (573) 884-5414
} Email: tindallr-at-missouri.edu
} Web: http://www.biotech.missouri.edu/emc/
}
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 07:45:01 2004

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Hi, Philip,

According to the previous email by Mike O'Keefe,
"Increased underfocus will push the
convergence-limited damping function to higher
frequencies," and in my own opinion, magnification
should be high enough to show up the information
limit. Did you compare Young fringes and Thon rings on
the same scale with high enough MAG and underfocus?

By the way, could you describe how to produce Young
fringes with your microscope? Thanks.

Juha

--- Philip Koeck {Philip.Koeck-at-biosci.ki.se} wrote:
}
}
}
------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------
}
} That's another question I've just come across.
}
} I have some test images (defocus around 1000 nm)
} from a FEG-TEM where
} Young fringes seem to extend up to twice as far as
} Thon rings. Is that
} usual and if so which of the two defines the
} information limit?
} What do manufacturers mean by information limit?
} Do Young fringes really show up to which resolution
} I can get useful
} information from a micrograph?
} At least in TEM of non-periodic biological specimens
} you normally don't
} expect anything beyond the last clearly visible Thon
} ring.
}
} Philip
}
} -----Original Message-----
} } From: Juha Dapper [mailto:juha_dapper-at-yahoo.com]
}
}
} 5. In Bill's email, you mentioned that "The
} information limit is best seen by shifting the image
} during the exposure. This produces Young's fringes
} in
} the power spectrum,".
}
} Could you please tell me in more details about how
} to
} "shift the image to produce Young's fringes"? This
} may be very practical and helpful to me.
}
}
}

__________________________________
Do you Yahoo!?
Friends. Fun. Try the all-new Yahoo! Messenger.
http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 13:53:32 2004

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I have been watching the discussion on TEM resolution with great interest and am very impressed by the power of some of the more recent models of TEM.

As a contribution to this discussion, I think it is important to remind everyone that instrument resolution is only half of the story. We must also take into account the resolution available in the specimen. For the people using these modern microscopes and imaging biological specimens at high resolutions it is taken for granted that optimal specimen preparation has occurred. Usually this means that small particles have been vitrified in the thin film of water and then imaged while still frozen.

For most people who use aldehyde-fixed and embedded sections, or for people who are just starting in EM, it is important to remember that high resolution electron microscopes are not much use for examining their samples. The reason being that the aldehyde fixation and subsequent dehydration at ambient temperature will either extract or condense the biological molecules. The end result is that there is no high resolution detail to examine in the specimens.

Better specimen preparation protocols are available for resin sectioners but they come at a price. Recent work has clearly shown that high pressure freezing followed by freeze substitution is able to preserve biological material better than the conventional methods. This approach may become the routine specimen preparation method of the future.

Until then, we have to keep our eyes open for the many fixation artifacts, including extraction and condensation, that are common in the scientific literature. There is a large community of scientists who know very little about EM but who are in positions where they review scientific literature and reseach grants. They need to know our strengths and limitations.

Regards,

Paul Webster.

Paul Webster, Ph.D.
House Ear Institute
2100 West Third Street
Los Angeles
CA 90057
phone (213) 273 8026
fax (213) 413 6739
email: pwebster-at-hei.org

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 16:44:51 2004

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Fellow List Members,

The Midwest Microscopy and Microanalysis Society has held student poster
competitions in the past, and would like to begin doing so again. The
Executive Council plans to review our previous practices and those of
the MSA, but we would also like input from Affiliate Societies or other
groups about guidelines for sponsoring a successful student poster
competition. Suggestions as to how you handle issues such as
eligibility, format judging, combining or separating materials science
and biological, etc., would be welcome.

Please send replies directly to me at eschumacher-at-mccrone.com. Your
input is very much appreciated.

Elaine Schumacher
Materials Science Director
Midwest Microscopy and Microanalysis Society

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 17:13:59 2004

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Fellow Listmembers,

Our Mini-Workshop Series on "Cryoultramicrotomy for Materials Sciences" is
coming to Texas!

The first session will be held at the University of Texas-Austin. Details
are given below.

When:
Wednesday, June 16 and Thursday, June 17, 2004, 9:00am-4:00pm

Where:
Department of Chemical Engineering
Room 2.222, Chemical and Petroleum Engineering Building
(Ground Floor)
Speedway and Dean Keeton Streets
University of Texas at Austin
Austin, TX 78712

(Parking structure is located just across Speedway from the Chemical and
Petroleum Engineering Building. Pay as you leave; credit cards accepted.)

What:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair
probes), glass knife making, evaluation of glass knives, care and cleaning of
diamond knives and operation of the cryoultramicrotome.

Attendees are welcome to bring specimens to the workshop. If you will be
bringing specimens, please let us know the nature of your specimens when you RSVP
and reserve a place in the workshop (see below).

Background:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing" at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

Important Info:
There is no charge for this workshop.
Meals and refreshments will be served!
Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryoultramicrotomy
hands-on sessions on the second day.

Contacts:
To RSVP and to reserve a spot for the hands-on sessions, please contact
either Kim Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262)
or Graham Bird at Atomic Spectroscopy Instruments, Inc.
( {grbird-at-thegateway.net} , 512-695-8865).

Sponsors and Organizers:
University of Texas at Austin
Department of Chemical Engineering (Dr. Don Paul's Group)
RMC Products Group, Boeckeler Instruments, Inc.
Atomic Spectroscopy Instruments, Inc.

See you in Austin!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 17:34:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (maloneyb-at-fiu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 26, 2004 at 13:57:23
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Email: maloneyb-at-fiu.edu
Name: Barb

Organization: FIU/FCAEM

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Group: what are the advantages to having a Pana CL and a cold stage hooked up to your LV SEM? I'm asking for all applications across the board, not just semi-conductors, etc. would like to see biological applications too.
Thanks
Barb

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From MicroscopyL-request-at-ns.microscopy.com Wed May 26 18:30:00 2004

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In a message dated 5/26/04 7:04:06 PM Eastern Daylight Time,
eschumacher-at-mccrone.com writes:

{ {we would also like input from Affiliate Societies or other
groups about guidelines for sponsoring a successful student poster
competition} }

Elaine:

This is how we judged the posters at the NESM Spring Symposium at Woods Hole.

{ {
Judging Criteria:
The posters are not judged on their scientific merit!
The Point Scale ranges from 1-5 for each Judging Category. If the presenter
does not wish to be included in the competition, indicate "d".

Microscope Adjustment: Do the photomicrographs or images illustrate that the
microscope was properly adjusted? Is the specimen in focus? For SEM images,
did the sample charge up? Was the proper accelerating voltage used? For
light microscopes, is there a uniform field of illumination? For AFM, DIC,
Confocal, or other techniques, are the images free of distortions or artifacts?
Quality of Images: Is the subject properly in the field of view? Are the
images relatively free of lines or dust specks? Was the film or digital image
correctly printed? Is there a scale?
Clarity of Graphics: Are the graphics well-drawn? Are the axes of any
graphs labeled? Is color or black & white used effectively? Do the graphics stand
alone, or must one refer to the text?
Clarity of Text: Does the text tell the story clearly and concisely? Is any
necessary jargon clearly explained? Are complete sentences used?
Layout of Poster: Is the poster easy to follow? Are arrows or numbers used
to guide the reader from one part of the poster to the other? Is the title
and subject of the poster obvious?
Interaction with Judges: Is the presenter enthusiastic and personable? Is
the presenter professionally attired and groomed? Does the presenter answer
simple questions in a clear, concise and knowledgeable manner? (Suggestions:
What microscopes did you use for this work? When and how were they calibrated?)
} }

Steve Stokowski
President-elect
New England Society for Microscopy

Contact Information:
Stone Products Consultants
10 Clark St., Ste. A
Ashland, Mass. 01721-2145
508-881-6364 (ph. & fax)

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 20:21:57 2004

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Hi Juha,

You certainly raise some interesting questions!

1. Well, if you had to sell a microscope with a point-to-point resolution of 2.4
Angstrom and an information limit of 1.4 Angstrom and a "line resolution" of 0.8
Angstrom, which figure would you mention to a customer who wanted the best high
resolution? Especially if your competitor's brochure quoted their microscope's
"line resolution". :-)

2. As you suggest, the best way is to use an objective aperture of a known size --
then any higher-frequency spots in the diffractogram of the image must be due to
"cross-aperture" non-linear interferences. A less direct way is to compare images
with simulations for a well-known specimen, assuming you have a good idea of the
microscope parameters and the specimen parameters (thickness...). Of course,
there's holography, if you have a biprism.

3. The "non-linear interferences" are part of the imaging process and will not be
present in the diffraction pattern (which is an "image" of electron distribution at
the back focal plane). The convolution that produces the interferences in the
image intensity spectrum in k-space comes from the squaring of the image amplitude
to form the image intensity in real space. Thinking another way, electrons leaving
the same position at the specimen have not yet been brought together at the back
focal plane (although electrons leaving the specimen at the same scattering angle
have).

4. The "paraboloid method" is able to extract just the linear contributions to the
images in the focal series because these contributions (sums of interferences)
occupy different positions to those of the non-linears in the 3-space generated by
the 3-D FFT of a set of images "stacked" in order of defocus. The 3-D "super
diffractogram" has the usual u and v axes (in the x,y planes of the images) while
the vertical w axis has the dimension of one over defocus. Then the linears lie on
a paraboloid in this space, while the non-linears are off the paraboloid and can be
filtered out, allowing the reconstruction of the exit-surface wave from just the
linear terms. See, for example, M&M 2002, (Quebec, Canada) 474-475 by Tadahiro
Kawasaki and Yoshizo Taka, and reference [16] at
http://nano.cirse.nagoya-u.ac.jp/kawa-paperlist.html

5. One way is to take two exposures with a shift of 10 or so Angstrom between
them, then add and FFT. Another is to introduce an abrupt image shift halfway
through the exposure of a single image, then FFT. A shift with the image-shift
coils avoids the danger of vibration that could occur with a shift of the
specimen. Young's fringes will occur at frequencies where features in the two
images are correlated -- the high-frequency noise will be different in each image
and thus not produce fringes. However, any second-order (non-linear) detail will
be present in both images. I think an image shift of 10 Angstrom will produce 10
fringes out to the 1 Angstrom point in the diffractogram.

I look forward to the next set of questions!

Michael

Juha Dapper wrote:

} ------------------------------------------------------------------------------
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} -------------------------------------------------------------------------------
}
} Thank you, Michael and Bill, for your kind reply. I
} really appreciate your remarkable answers to my
} questions.
}
} After carefully reading your answers, I've got more
} questions.
}
} 1. If the "line resolution" is so confusing and
} untrustworthy, why TEM manufactures used to apply it
} to claim the quality of a microscope?
}
} 2. If an HREM iamge was taken without a certain
} objective aperture, how can we tell if a
} high-frequency spacing present in the image (or the
} corresponding spot in its FFT) is due to linear
} transfer or just by "cross-aperture" non-linear
} interference?
}
} 3. About the "non-linear interferences". Do they
} happen already during the process of electron-specimen
} interaction, or after the back-focal plane of the
} objective lens during the electron wave propagation?
}
} 4. In Michael's email, it is said "Since we know how
} linear transfer varies with objective lens defocus, we
} can use a series of images to produce a single
} reconstructed image containing correctly-phased
} components all the way out to the microscope
} information limit [see work by Van Dyck, Coene and
} Thust]."
}
} Did you mean that the reconstruction method using a
} focal-series can only apply to the linear transfer
} case, i.e. the case of a weak phase object? If not,
} how the non-linear interference effects are treated?
}
} 5. In Bill's email, you mentioned that "The
} information limit is best seen by shifting the image
} during the exposure. This produces Young's fringes in
} the power spectrum,".
}
} Could you please tell me in more details about how to
} "shift the image to produce Young's fringes"? This
} may be very practical and helpful to me.
}
} Again thank you very much for your instructions.
}
} -juha
}
}
}
} __________________________________
} Do you Yahoo!?
} Friends. Fun. Try the all-new Yahoo! Messenger.
} http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 04:30:37 2004

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Barb writes ...

} Question: Dear Group: what are the advantages to having
} a Pana CL and a coldstage hooked up to your LV SEM? I'm
} asking for all applications across the board, not just
} semi-conductors, etc. would like to see biological
} applications too.

Speaking for CL from quartz, a cold stage does indeed increase the
luminescence, but we found it disapponiting. That is, it didn't raise the
CL from unique areas, (rather than from everywhere), and contrast from
regions of unique emission was reduced. Moderate gain can come from
lowering the temp to a range of 0 to -30C, but I imagine this can be
accomplished with Peltier cooling rather than LN2.

hth & genuinely ... michael shaffer :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 05:20:06 2004

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Hi again,

I think I need to restate my question about expiration dates on lab
chemicals, since I may have been unclear in my first posting.

I know that expiration dates are arbitrary and maybe even meaningless in
many cases, because they depend on so many variables. However,
sometimes we are required to put them on our reagents because of rules
regarding certain research projects.

For example, if a lab should perform electron microscopy as part of a
project involving a pharmaceutical company, chances are that the company
will require certain types of documentation, traceability, instrument
calibration, standardization of methods, etc. Expiration dates on
chemicals are often (maybe always) part of such requirements.
Diagnostic work is another probable example.

My question or proposal is this: Given that we are sometimes REQUIRED to
use expiration dates, wouldn't it be reasonable if there was some
consensus in our field we could point to and say "Our lab follows the
(for example) MSA standards on chemical usage."? As it is, I have not
yet been able to locate a set of standards to guide us in any sort of
meaningful compliance with such outside requirements. Phil Oshel has
suggested that the histotech community has been dealing with this for
some time, so I'm checking this out now (thanks for the suggestion,
Phil).

On the other hand, maybe this is something that doesn't need fixing,
because it ain't broke. I'm just curious what others think about it.

Thanks all.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 08:29:40 2004

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After following this discussion for a few days now, I could no longer
resist the
temptation to participate in what still, after all these years, appears
to be a
subject with a wide variety of opinions.

I spent a few years in the testing end of the asbestos business, with
most of
my time spent on a PLM. It is indeed an excellent tool for identifying
asbestos,
and, according to Mr. McCrone, just about anything that can be made to fit
on to a microscope slide. However, I must admit that it is highly
dependant
on the abilities of the microscopist, and good quality control is a
must. Having
completed one of Mr. McCrone's PLM courses, it is difficult to argue
against
even the most impressive claims regarding the PLM's capabilities, but that
was with Mr. McCrone himself at the helm, and no one knows the PLM the
way he does. (I guess that makes me a "McCrone(ie)").

My biggest concern in this discussion is the comment that only one form of
asbestos is harmful to humans. During my time in the industry I went to
a lot
of seminars and read a lot of literature on asbestos, and although I
have been
out of the business for many years now, I would be very surprised to
find out
that amosite, crocidolite and the other forms of asbestos had been found
to be
harmless. All of the minerals in the asbestos family have a similar
crystal structure.
It is that unique structure that produces the very fine fibers that get
trapped in the
lungs and, under the now considered rare conditions, causes cancer and
mesothelioma. It is true that crysotile was the most commonly used form of
asbestos, but the others are every bit as dangerous.

I have been very pleased to see that a much more reasonable approach has
been adopted by the regulatory agencies that control the industry and
originally
created such a panic throughout the country, however a part of me still
feels
that getting asbestos out of the schools might have been the one good thing
that resulted from that panic. There is obviously still a lot we do not
know
about asbestos and it's long term effects. Removing it from the
buildings that
our children spend so much time in was a reasonable precaution at the time.

Doug Price

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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 10:05:16 2004

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Dear Members,

Question: In the TEM, the exit wave (the wave leaving
the specimen)is complex-valued in general, which can
be written as g = f1 + i*f2, where f1 and f2 are real
numbers. Is it true/false that f2 has no sign changes,
i.e. if positive, always positive?

With best regards,

Zhongyi Liu
Argonne National Lab
Argonne, IL60439

____________________________________________________________
Yahoo! Messenger - Communicate instantly..."Ping"
your friends today! Download Messenger Now
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From MicroscopyL-request-at-ns.microscopy.com Thu May 27 10:21:38 2004

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Elaine,

The International Metallographic Society and ASM International have been
cosponsoring the International Metallographic Contest and Exhibit since
1972. The contest is held in conjunction with the annual convention of the
International Metallographic Society, which, since 2002, has become an
intrical part of the M&M annual meeting. Entries, in the form of posters,
use photographs and captions to describe how metallography helped solve a
problem or to introduce a unique, unusual, or new metallographic technique.
The entries are mailed rather than presented, but perhaps some of the rules
and judging criteria would be applicable to your contest.

There are twelve different classes of competition in order to give everybody
a fair chance. For example light microscopy is separate from electron
microscopy, metals and their alloys are separate from other materials,
color is separate from black and white. Students are welcome to enter any of
the classes, but they are encouraged to enter the two specifically for
undergrads. That way the students are not competing directly with
professionals in their individual classes.

Please visit www.metallography.com/ims/contest.htm for additional details or
download www.metallography.com/ims/imcjudges.doc for a history of the
contest and some insight into the judging process. This year's contest is
scheduled for Saturday, July 31 in Savannah. Deadline for entries is July
19. All entries will be on exhibit for the duration of the M&M meeting. If
you'll be attending the meeting, I invite you to come visit the display.

Best regards,

Jeff Stewart
International Metallographic Contest Chair
Metallographic Laboratory Manager
Stern-Leach Co.
49 Pearl Street
Attleboro, MA 02703 USA
Phone: 508-222-7400 extension 1329
Fax: 508-699-4030
E-mail: jeff-at-metallography.com

----- Original Message -----
} From: "Elaine F. Schumacher" {eschumacher-at-mccrone.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 26, 2004 5:56 PM

Dear Michael,

Thank you for your crystal answers that really cheer
me up by clarifying those doubts hanging around my
mind so far. Your papers in Ultramicroscopy 89 (2001)
215–241 helps a lot too in understanding those
questions.

I do have another few very fundamental questions. I
really hesitate to ask without your encouragement.

In your first email, and also in the article I listed
above,(actually all people say so): at the Scherzer
defocus, there is a largest passband where all linear
spacial frequescy components are transfered to the
image with the "same sign", or say the "same-phase
passband" transfer.

To be clear,I put my questions into three as follows
although they are much related.

1. In my understanding, the phase shift that are
imposed by the objective lens on a diffracted beam is
a function of spacial frequescy (k). It means each k
component will be shifted (displaced) in the image by
a unique amount, even within the Scherzer passband. So
what does the "same-sign transfer" really mean here?
Is it true that "the same sign is in the same way"?

2. For a certain focus condition, it seems we can
divided those transfer into just two portions (in
additon to those zero-cross): "+ sign" transfer and "-
sign" transfer. However, from "+ sign" to "- sign",
the difference in phase-shift can be very little, for
instance, from 179(degree) to 181(degree). So what and
how large difference may we expect from the sign
transfer of the two k components that just transit
from + (179) to - (181)?

3. As I described above, even within the Scherzer
passband, different k components will be displaced in
the image by different amounts depending on the phase
shifts they suffer from the lens. So how to estimate
delocalization effect in a Scherzer image, especially
with a non-periodic object. And, more important, how
the delocalization effect is handled in FEG-HREM
focal-series reconstruction where such effect can be
really serious?

Thank you again.

-juha

--- Michael O'Keefe {MAOKeefe-at-lbl.gov} wrote:
}
}
}
------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
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}
-------------------------------------------------------------------------------
}
} Hi Juha,
}
} You certainly raise some interesting questions!
}
} 1. Well, if you had to sell a microscope with a
} point-to-point resolution of 2.4
} Angstrom and an information limit of 1.4 Angstrom
} and a "line resolution" of 0.8
} Angstrom, which figure would you mention to a
} customer who wanted the best high
} resolution? Especially if your competitor's
} brochure quoted their microscope's
} "line resolution". :-)
}
} 2. As you suggest, the best way is to use an
} objective aperture of a known size --
} then any higher-frequency spots in the diffractogram
} of the image must be due to
} "cross-aperture" non-linear interferences. A less
} direct way is to compare images
} with simulations for a well-known specimen, assuming
} you have a good idea of the
} microscope parameters and the specimen parameters
} (thickness...). Of course,
} there's holography, if you have a biprism.
}
} 3. The "non-linear interferences" are part of the
} imaging process and will not be
} present in the diffraction pattern (which is an
} "image" of electron distribution at
} the back focal plane). The convolution that
} produces the interferences in the
} image intensity spectrum in k-space comes from the
} squaring of the image amplitude
} to form the image intensity in real space. Thinking
} another way, electrons leaving
} the same position at the specimen have not yet been
} brought together at the back
} focal plane (although electrons leaving the specimen
} at the same scattering angle
} have).
}
} 4. The "paraboloid method" is able to extract just
} the linear contributions to the
} images in the focal series because these
} contributions (sums of interferences)
} occupy different positions to those of the
} non-linears in the 3-space generated by
} the 3-D FFT of a set of images "stacked" in order of
} defocus. The 3-D "super
} diffractogram" has the usual u and v axes (in the
} x,y planes of the images) while
} the vertical w axis has the dimension of one over
} defocus. Then the linears lie on
} a paraboloid in this space, while the non-linears
} are off the paraboloid and can be
} filtered out, allowing the reconstruction of the
} exit-surface wave from just the
} linear terms. See, for example, M&M 2002, (Quebec,
} Canada) 474-475 by Tadahiro
} Kawasaki and Yoshizo Taka, and reference [16] at
} http://nano.cirse.nagoya-u.ac.jp/kawa-paperlist.html
}
} 5. One way is to take two exposures with a shift of
} 10 or so Angstrom between
} them, then add and FFT. Another is to introduce an
} abrupt image shift halfway
} through the exposure of a single image, then FFT. A
} shift with the image-shift
} coils avoids the danger of vibration that could
} occur with a shift of the
} specimen. Young's fringes will occur at frequencies
} where features in the two
} images are correlated -- the high-frequency noise
} will be different in each image
} and thus not produce fringes. However, any
} second-order (non-linear) detail will
} be present in both images. I think an image shift
} of 10 Angstrom will produce 10
} fringes out to the 1 Angstrom point in the
} diffractogram.
}
} I look forward to the next set of questions!
}
} Michael
}
} Juha Dapper wrote:
}
} }
}
------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
}
-------------------------------------------------------------------------------
} }
} } Thank you, Michael and Bill, for your kind reply.
} I
} } really appreciate your remarkable answers to my
} } questions.
} }
} } After carefully reading your answers, I've got
} more
} } questions.
} }
} } 1. If the "line resolution" is so confusing and
} } untrustworthy, why TEM manufactures used to apply
} it
} } to claim the quality of a microscope?
} }
} } 2. If an HREM iamge was taken without a certain
} } objective aperture, how can we tell if a
} } high-frequency spacing present in the image (or
} the
} } corresponding spot in its FFT) is due to linear
} } transfer or just by "cross-aperture" non-linear
} } interference?
} }
} } 3. About the "non-linear interferences". Do they
} } happen already during the process of
} electron-specimen
} } interaction, or after the back-focal plane of the
} } objective lens during the electron wave
} propagation?
} }
} } 4. In Michael's email, it is said "Since we know
} how
} } linear transfer varies with objective lens
} defocus, we
} } can use a series of images to produce a single
} } reconstructed image containing correctly-phased
} } components all the way out to the microscope
} } information limit [see work by Van Dyck, Coene and
} } Thust]."
} }
} } Did you mean that the reconstruction method using
} a
} } focal-series can only apply to the linear transfer
} } case, i.e. the case of a weak phase object? If
} not,
} } how the non-linear interference effects are
} treated?
} }
} } 5. In Bill's email, you mentioned that "The
} } information limit is best seen by shifting the
} image
} } during the exposure. This produces Young's fringes
} in
} } the power spectrum,".
} }
} } Could you please tell me in more details about how
} to
} } "shift the image to produce Young's fringes"?
} This
} } may be very practical and helpful to me.
} }
} } Again thank you very much for your instructions.
} }
} } -juha
} }
} }
} }
} } __________________________________
} } Do you Yahoo!?
} } Friends. Fun. Try the all-new Yahoo! Messenger.
} } http://messenger.yahoo.com/
}
}

__________________________________
Do you Yahoo!?
Friends. Fun. Try the all-new Yahoo! Messenger.
http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 10:46:49 2004

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randy

on the virology/tissue culture side of things we are very compulsive
about our chemistry. on the EM side we are much more lax. i have
chemicals that are up to 35 years old - no, not my glutaraldehyde and
osmium.... periodically i go on a cleaning spree and get rid of old
organics, solvents, and bottles of DMP-30. at the first hint of
moisture in acetone, ethanol or dichloroethane i discard the contents or
ship the bottles off to chemical safety for appropriate disposal. once
a year i clean out all accumulated preparations of negative and positive
stains, small as those stocks are. but i have ancient bottles of UA,
uranyl sulfate, etc. which i use to make those stains and most other
solutions.

but what is expiry, and what is a good basis for change. it is not
universally established. as an example, dogma states that PTA and UA
are only good for short periods of time, 2-3 months. i know from
controlled tests that PTA and UA are good for negative staining for up
to a year if stored correctly, but i still have them replaced every 2-3
months, although i sometimes get debate on this from the techs, an
action which i encourage.

my lab is probably very normal - especially for those headed up by my
fellow dinosaurs, who have been doing this for 30+ years.

your points are very valid, and deserve some follow up. i hope you will
post what you find from the histology community.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 11:14:28 2004

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Hi Andrew:

The princples of tissue preparation for light and/or electron
microscopy are ancient, at least by the standards your "colleagues" seem
to be using (I hope theses colleagues are not on the faculty, condeming
work based solely on the date of publication is demonstrates
ignorance). For electron microscopy, glutaradehyde fixation followed by
osmium post-fixation was worked out in the early 1960's, embedding in
epoxy resins dates from the late 1950s. Of course, the basic methods for
light microscopy are much older.
So the question is, what exactly are you trying to do? Are you
interested in applying a new technique to an older problem? If so, the
technique you select should show some promise of answering the question
you are asking! That may seem very obvious, but as all researchers
(should) know, "the road to hell is paved with good intentions." A good
experiment does not have to be fancy or use the latest hot technique.
The best work is often rather simple, the elegance residing in the
concepts of mating the question with the method used to answer it. Plus
a lot of hard work.

Geoff

by way of MicroscopyListserver wrote:

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--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 11:35:07 2004

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I've noticed over the past few months that I needed to set my ultramicrotome
thicker and thicker to get the same thin sections [using an Ultracut-E].
Finally I often ended up having to cut using the "thick" setting, and
cutting about 1.1 micrometers according to that microtome to cut thin
sections.

This was using a DDK knife that I've used for 11 years, with about 5 or 6
years on the same side of the knife. But yesterday I changed knives to a
resharpened knife, and found that I only need to set my ultratome at about
76 nanometers to get my same silver/gold sections.

Is this really what happens when one's diamond knife gets dull? - or is
this just a coincidence? This is the first time in 20 years that I've
observed this phenomenon. I'd be interested in hearing about the
experiences of others on this.

Garry Burgess

Charge Technologist
Electron Microscopy Laboratory MS-336
Department of Pathology
Health Sciences Centre
820 Sherbrook Street
Winnipeg, Manitoba, Canada
R3A 1R9

Phone: (204) - 787 -1508
Fax: (204) - 787- 2381

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 12:15:46 2004

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Dear listers,

About 2 years ago we upgraded our WDS microspec 2a unit with Oxford system,
but the old system was still operational at the time. If anyone is
interested in acquiring the old unit please contact me offline.

Regards,

Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 14:04:40 2004

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I could be wrong, but 5 or 6 years on a knife, without sharpening, seems a long
stretch. How much use does it get?

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Garry Burgess [mailto:GBurgess-at-exchange.hsc.mb.ca]
Sent: Thursday, May 27, 2004 12:47 PM
To: 'Microscopy-at-MSA.Microscopy.com'

I've noticed over the past few months that I needed to set my ultramicrotome
thicker and thicker to get the same thin sections [using an Ultracut-E].
Finally I often ended up having to cut using the "thick" setting, and
cutting about 1.1 micrometers according to that microtome to cut thin
sections.

This was using a DDK knife that I've used for 11 years, with about 5 or 6
years on the same side of the knife. But yesterday I changed knives to a
resharpened knife, and found that I only need to set my ultratome at about
76 nanometers to get my same silver/gold sections.

Is this really what happens when one's diamond knife gets dull? - or is
this just a coincidence? This is the first time in 20 years that I've
observed this phenomenon. I'd be interested in hearing about the
experiences of others on this.

Garry Burgess

Charge Technologist
Electron Microscopy Laboratory MS-336
Department of Pathology
Health Sciences Centre
820 Sherbrook Street
Winnipeg, Manitoba, Canada
R3A 1R9

Phone: (204) - 787 -1508
Fax: (204) - 787- 2381

This e-mail and/or any documents in this transmission is intended for the
address(s) only and may contain legally privileged or confidential information.
Any unauthorized use, disclosure, distribution, copying or dissemination is
strictly prohibited. If you receive this transmission in error, please notify
the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 16:25:21 2004

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Hi,

I was wondering if it is possible to buy sharpened scanning tunnel
microscope tips? I have a colleague who is having trouble getting a
sharp tip from Pt/Ir wire.

Bettye

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 17:20:08 2004

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False.
At least in simulated exit-waves.
For example, in simulations for GaN at 300keV, the exit-wave Argand-plane vector at
the Ga position starts at f2 = 0 for zero thickness, then describes an approximate
circle that extends from f2 = +1.3 to -1.5 electrons.
Mike

Zhongyi Liu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear Members,
}
} Question: In the TEM, the exit wave (the wave leaving
} the specimen)is complex-valued in general, which can
} be written as g = f1 + i*f2, where f1 and f2 are real
} numbers. Is it true/false that f2 has no sign changes,
} i.e. if positive, always positive?
}
} With best regards,
}
} Zhongyi Liu
} Argonne National Lab
} Argonne, IL60439
}
}
}
}
}
} ____________________________________________________________
} Yahoo! Messenger - Communicate instantly..."Ping"
} your friends today! Download Messenger Now
} http://uk.messenger.yahoo.com/download/index.html

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 17:57:57 2004

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Hi, Listers and Posters

Does anyone have any experience, positive or negative, with cleaning EPMA analysing
crystals?

TAP and PET, I suspect, as the LIF deals with harder X-Rays.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 19:00:21 2004

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}
} I've noticed over the past few months that I needed to set my ultramicrotome
} thicker and thicker to get the same thin sections [using an Ultracut-E].
} Finally I often ended up having to cut using the "thick" setting, and
} cutting about 1.1 micrometers according to that microtome to cut thin
} sections.
}
} This was using a DDK knife that I've used for 11 years, with about 5 or 6
} years on the same side of the knife. But yesterday I changed knives to a
} resharpened knife, and found that I only need to set my ultratome at about
} 76 nanometers to get my same silver/gold sections.
}
} Is this really what happens when one's diamond knife gets dull? - or is
} this just a coincidence? This is the first time in 20 years that I've
} observed this phenomenon. I'd be interested in hearing about the
} experiences of others on this.
}
} Garry Burgess
}
Garry -

Not enough information here. What sort of samples do you cut? How
did you clean the old knife? Do both knives have the same clearance
and cutting angles?

Caroline

--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 19:39:18 2004

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You may be amused that this e-mail, with the original title reference
to "Thick and Thicker", was flagged by my system's spam detector.
Cute.

} From: "Sherwood, Margaret " {MSHERWOOD-at-PARTNERS.ORG}
To: "'Garry Burgess'" {GBurgess-at-exchange.hsc.mb.ca} ,
"'Microscopy-at-MSA.Microscopy.com'" {Microscopy-at-msa.microscopy.com}

You can arbitrary reference the phase. If the phase is referenced to an
undisturbed wave at the same plane (wave if there is no specimen) then I
would say yes - the imaginary part for weak phase specimens should be
always negative. Any material has positive inner potential. When the
electron wave traverses the area of the specimen it will experience a
negative phase shift due to the positive potential in that area (phase
retardation). If the magnitude of the phase shift is small (less than
Pi) then f2 in your expression will always be negative.

Regards,

Rado

} -----Original Message-----
} From: Michael O'Keefe [mailto:MAOKeefe-at-lbl.gov]
} Sent: Friday, May 28, 2004 7:32 AM
} To: Zhongyi Liu
} Cc: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] Re: imaginary part of exit wave
}
}
}
}
} --------------------------------------------------------------
} ----------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line
} Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} --------------------------------------------------------------
} -----------------
}
} False.
} At least in simulated exit-waves.
} For example, in simulations for GaN at 300keV, the exit-wave
} Argand-plane vector at the Ga position starts at f2 = 0 for
} zero thickness, then describes an approximate circle that
} extends from f2 = +1.3 to -1.5 electrons. Mike
}
} Zhongyi Liu wrote:
}
} }
} ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line
} Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} -----------------
} }
} } Dear Members,
} }
} } Question: In the TEM, the exit wave (the wave leaving
} } the specimen)is complex-valued in general, which can
} } be written as g = f1 + i*f2, where f1 and f2 are real
} numbers. Is it
} } true/false that f2 has no sign changes, i.e. if positive, always
} } positive?
} }
} } With best regards,
} }
} } Zhongyi Liu
} } Argonne National Lab
} } Argonne, IL60439
} }
} }
} }
} }
} }
} } ____________________________________________________________
} } Yahoo! Messenger - Communicate instantly..."Ping"
} } your friends today! Download Messenger Now
} } http://uk.messenger.yahoo.com/download/index.html
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 08:00:01 2004

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Dear Microscopists,

According to the research of Andrew Churg of the University of British Columbia's Department of Pathology, the average 60 year old North American's lung contains about 400,000 fibers of asbestos. 20% of those fibers are of the "carcinogenic" amphibole variety. The balance being harmless chrysotile asbestos. See "Health Effects of Mineral Dusts" Mineralogical Society of America Reviews in Mineralogy Volume 28.

"Asbestos" has become an antique term of convenience value only. It referred to fibrous silicate minerals in two groups. Those were the serpentine group (chrysotile) and the amphibole group (amesite, riebeckite ((crocidolite)) etc.).

The better term is "asbestosform" minerals. This term includes the most hazardous fibrous silicates which are in the zeolite group of minerals. Offretite and erionite are brittle, very finely fibrous minerals which are known to occur in large zeolitized lake-bed deposits, often near human inhabitation. Their aspect ratio and stiffness is ideally suited to create lesions in the lungs. Many human deaths in Turkey are associated with offretite and erionite. Similar deposits occur in the U.S., but are not near population centers.

Chyrsotile is a relatively benign material with remarkably useful physical properties that are NOT duplicated by any other material. Yet the regulators have taken it away from us. Brake linings made from chrysotile are far more fade resistant than those made from chrysotile's replacement. PIG HAIR !!! And beware, most other modern and synthetic substitutes have unknown health factors.

Nevertheless, it is only amphibole "asbestos" that has been shown to be carcinogenic by classic studies. Its major source was South Africa. Amphibole asbestos was far more expensive than chrysotile asbestos and was only used for high temperature applications such as ship boilers. Chysotile converts to brittle forsterite at 800 degrees C whereas amphibole asbestos stay fibrous above 1300 degrees C. This makes it more suitable for high temp boiler applications. At the end of WW II there were stockpiles of amphibole asbestos which were sold off at chrysotile prices. In this way some harmful amphibole asbestos found its way into residential applications. A "glitter" ceiling (mica with asbestos binder) installed pre-1950 may be dangerous, but not the later ones since the stockpiles of amphibole asbestos were generally spent.

Amphibole asbestos has been in the news recently due to media play on the former vermiculite mines in Libby, Montana. There the amphibole is richterite and occurs intergrown with the vermiculite in trace quantities. Mining operations placed the fibers in the air and asbestosis has resulted mostly among the mine workers, but some evidence shows asbestosis and mesothelioma among the families of mine workers. Tavern talk indicates that the mine workers often cut holes in their respirators to facilitate the insertion of cigarettes. Cigarette smoking is usually a key associated behavior in the contraction of fatal mesothelioma. One Libby mine worker / smoker has indignantly shown his chest x-ray to the media as proof of the mining company's irresponsible actions. He was 83 three years ago. We should all live so long.

I have much more should anyone be interested in contacting me offline.

Bart Cannon
Cannon Microprobe
Seattle

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 08:20:48 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mpendleton-at-mic.tamu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, May 27, 2004 at 11:25:06
---------------------------------------------------------------------------

Email: mpendleton-at-mic.tamu.edu
Name: Mike Pendleton

Organization: Texas A&M U. Micros. & Imaging Center

Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to 8bit tif

Question: With our image capture system used for the JEOL 6400 SEM we need a windows based system to convert 16 bit Sun Raster grayscale images into 8 bit grayscale tif images. I use the free XnView program to convert 8 bit grayscale Sun Raster images to 8 bit grayscale tif images so I can cut down on the tedious conversion process I am currently using, but still have to make the 16 to 8 bit conversion using the Sun program connected to the scope. I think the new version of Photoshop will convert 16 bit Sun Raster to 8 bit tif, but this is costly just to be able to convert files. Is there an inexpensive program to convert 16 bit Sun Raster images to 8 bit tif images? I would appreciate any information to solve this problem. Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 11:01:13 2004

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(5/28/04 8:33) by way of MicroscopyListserver {mpendleton-at-mic.tamu.edu} wrote:

} Email: mpendleton-at-mic.tamu.edu
} Name: Mike Pendleton
}
} Organization: Texas A&M U. Micros. & Imaging Center
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to 8bit tif
}
} Question: With our image capture system used for the JEOL 6400 SEM we need a windows based system to convert 16 bit Sun Raster
} grayscale images into 8 bit grayscale tif images. I use the free XnView program to convert 8 bit grayscale Sun Raster images to 8
} bit grayscale tif images so I can cut down on the tedious conversion process I am currently using, but still have to make the 16 to 8
} bit conversion using the Sun program connected to the scope. I think the new version of Photoshop will convert 16 bit Sun Raster to
} 8 bit tif, but this is costly just to be able to convert files. Is there an inexpensive program to convert 16 bit Sun Raster images to 8
} bit tif images? I would appreciate any information to solve this problem. Thanks.

Mike,

You are correct that Photoshop will do this. You might find, however, that Photoshop isn't as expensive as you think. It has been my experience that many universities these days have negotiated site licenses with Adobe, so that installing Photoshop on a university-owned machine is essentially free. You'd want to speak with your campus IT department to see if that is the case. Even if you don't have a site license, you will probably be able to get the educational version of Photoshop through your student bookstore, which is incredibly cheap.

This does beg the question of why you're wanting to throw away those 8-bits of data. I realize that SEM isn't going to give you much more than 8 bits of real data, but are you sure that the conversion isn't throwing away an equal amount of signal as noise? We usually recommend to folks that if they're getting 16 bits out, they should do their processing and measurement on that 16-bit image. This is especially important if you want to do any Fourier processing, for obvious reasons. When people ask me about the differences between Fovea Pro and the Image Processing Tool Kit, this usually comes up, since Fovea supports 16-bit images in Photoshop.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 11:01:29 2004

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You might try looking at Graphic Converter. There are two versions out
there.

One is for the PC at Version 2.5. Go to http://www.graphic-converter.net/.
It converts 30 file formats. It's hard to tell if it reads Sun Raster file
formats, the site is rather brief in its descriptions. The software is
available online for $19.95

One is for the Mac at Version 5.1.1. Go to
http://www.lemkesoft.de/en/index.htm. This software imports 175 file formats
and exports 75 formats. This version will import Sun Raster file format in 8
or 24 bit per pixel. The software is available online for $35 ($30 w/o CD).

} Email: mpendleton-at-mic.tamu.edu
} Name: Mike Pendleton
}
} Organization: Texas A&M U. Micros. & Imaging Center
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to
} 8bit tif
}
} Question: With our image capture system used for the JEOL 6400 SEM we need a
} windows based system to convert 16 bit Sun Raster grayscale images into 8 bit
} grayscale tif images. I use the free XnView program to convert 8 bit
} grayscale Sun Raster images to 8 bit grayscale tif images so I can cut down on
} the tedious conversion process I am currently using, but still have to make
} the 16 to 8 bit conversion using the Sun program connected to the scope. I
} think the new version of Photoshop will convert 16 bit Sun Raster to 8 bit
} tif, but this is costly just to be able to convert files. Is there an
} inexpensive program to convert 16 bit Sun Raster images to 8 bit tif images?
} I would appreciate any information to solve this problem. Thanks.
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 11:43:03 2004

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On May 25, 2004, at 11:08 AM, Tindall, Randy D. wrote:

} Does anyone else think it might be a useful exercise to try and
} establish expiration dates for chemicals used in microscopy labs? I
} understand that chemicals "expire" based upon what they are, what use
} they are intended for, how they are used, what level of
} accuracy/repeatability/etc. is expected from their use, how they are
} stored, and many other factors. I have also read Rande Kline's
} discussion of the problem in the July/August 2000 Microscopy Today on
} the difficulties of establishing such dates (recommended).
}
} The problem is that some work requires lab certification and strict
} laboratory guidelines requiring that all chemicals be labeled with
} expiration dates----whether or not those dates have any meaningful or
} consistent basis in "reality". So far, I've been unable to find any
} such set of standards and my strong impression is that labs set up
} their
} own arbitrary chemical rotation regimen.
}
Dear Randy,
Count me as one of the interested parties. Especially since there are
several chemicals that we use sporadically, we need to know what must
be made up fresh, and how long things keep.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 13:51:55 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I would also like to see something done with this. We have recently been
advise that we should not keep 'useless' chemicals around the lab. Its a
long story, the rest of this message summarizes some our experiences.

We are being treated to a series of regulatory inspections. First, it was
by an agency concerned about 'hazardous waste'. Now it is by agencies
looking at the way we ship and receive goods to and from campus.

The hazardous waste guys might have been the EPA, but I'm not sure. We (the
campus) were given the opportunity to do a 'self audit'. In a self audit,
our EH&S guys got to go around and get everyone up to speed on proper
disposal and storage methods for hazardous waste. Mostly, it was the normal
stuff, but a new wrinkle for me was that I may no longer keep anything
marked as 'waste' in the lab for more than 6 months. Has something to do
with accumulation rules and shipping it off campus.

The deal with the 'self audit' is that you get one 'get out of jail free'
card, sort of. If you do a good job and come clean with any violations,
then those violations will not be held against you if they ever do an
official audit. Official audits can be big time trouble, expensive and a
pain. For example, fines, big ones, may be assessed and you may be told to
fix something right now, whether there is money to do it or not. We just
barely beat a bad situation by having the proper hoods and venting for the
storage of some special compound. Had we not had it right, the EH&S guys
said the inspector could have demanded that we install an expensive system
within something like 90 days, or abandon the use of that compound.

As a sideline to the audit thing, our EH&S folks are encouraging us to get
rid of anything we don't need or use regularly. They say,'It will never get
cheaper to dispose of hazardous waste than it is today'. The cost of
disposal will only go up, so if you aren't going to use it, get rid of it.
I wonder about this because I tend to keep some old stuff around in case a
starving student needs something like embedding resin. I have a bunch left
over from various kits, but can I trust it? If not, it should go, but its
hard to toss things that may be useful.

We are currently involved in another 'self audit'. This one being done to
check on what and how we ship things to and from campus. Dept. of Commerce
and Homeland Security have lists of things that are not allowed, like wet
suits to North Korea, etc. The list is pages, maybe hundreds, long with
some of the weirdest things. Lots of things like chemicals and biological
samples show up. Same deal, admit to any wrong doing and say how you will
correct it will keep you off the hook. Forget something or make a mistake
after the audit and you could go to jail.

So, in the interest of staying out of jail, not paying fines, and keeping
our EH&S staff happy, I would like to get some ideas about how long to keep
things around before moving them out. I will just have to deal with the
guilt of tossing perfectly good materials on my own.

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 14:11:44 2004

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On May 26, 2004, at 2:30 AM, Philip Koeck wrote:

} I have some test images (defocus around 1000 nm) from a FEG-TEM where
} Young fringes seem to extend up to twice as far as Thon rings. Is that
} usual and if so which of the two defines the information limit?
} What do manufacturers mean by information limit?
} Do Young fringes really show up to which resolution I can get useful
} information from a micrograph?
} At least in TEM of non-periodic biological specimens you normally don't
} expect anything beyond the last clearly visible Thon ring.
}
Dear Philip,
Do you generate the Young's fringes by shifting the image in the scope
during the exposure, or do you use a computer to generate a shifted
image and sum it with the unshifted image? In the latter case, the
noise, which does not have a CTF related to the lenses, is perfectly
correlated, so there will be fringes, but no rings. In the former
case, the noise is independent for the shifted and unshifted parts of
the image, so it will not add as much intensity to the fringes (there
will be some correlation of random noise, so some intensity). The
information limit is measured by the Thon rings. Whether the
information from Thon rings beyond the first zero of the CTF is useful
depends on the nature of the specimen, the accuracy with which the
exact value of the defocus can be measured, and the processing
algorithm used to compensate for the CTF. For thick, non-periodic
biological specimens, the defocus varies through the specimen, the
contrast is low, and the dose is low, so the S/N is low. It is still a
matter of discussion whether such techniques as CTF compensation or
focal series reconstruction are of benefit.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 14:33:22 2004

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At the moment, Photoshop 7 can be obtained on the net for $60.
Photoshop 7 is a perfectly respectable version and is available
inexpensively because Photoshop 8 (or CS) is out. You however will love
Photoshop 7 as well.
Just a thought,
Judy Murphy

Doug Baldwin wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} You might try looking at Graphic Converter. There are two versions out
} there.
}
} One is for the PC at Version 2.5. Go to http://www.graphic-converter.net/.
} It converts 30 file formats. It's hard to tell if it reads Sun Raster file
} formats, the site is rather brief in its descriptions. The software is
} available online for $19.95
}
} One is for the Mac at Version 5.1.1. Go to
} http://www.lemkesoft.de/en/index.htm. This software imports 175 file formats
} and exports 75 formats. This version will import Sun Raster file format in 8
} or 24 bit per pixel. The software is available online for $35 ($30 w/o CD).
}
} } Email: mpendleton-at-mic.tamu.edu
} } Name: Mike Pendleton
} }
} } Organization: Texas A&M U. Micros. & Imaging Center
} }
} } Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to
} } 8bit tif
} }
} } Question: With our image capture system used for the JEOL 6400 SEM we need a
} } windows based system to convert 16 bit Sun Raster grayscale images into 8 bit
} } grayscale tif images. I use the free XnView program to convert 8 bit
} } grayscale Sun Raster images to 8 bit grayscale tif images so I can cut down on
} } the tedious conversion process I am currently using, but still have to make
} } the 16 to 8 bit conversion using the Sun program connected to the scope. I
} } think the new version of Photoshop will convert 16 bit Sun Raster to 8 bit
} } tif, but this is costly just to be able to convert files. Is there an
} } inexpensive program to convert 16 bit Sun Raster images to 8 bit tif images?
} } I would appreciate any information to solve this problem. Thanks.
} }
} } ---------------------------------------------------------------------------
} }

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 14:48:06 2004

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Randy,

I agree that this is an important issue and that some standard re: expiration
of chemicals would be great. But is it reasonable?

I don't think it is--manufacturers of chemicals and reagents are a good source:
they test these chemicals and assign a shelf-life. But, ultimately it depends
on how the user handles the chemical. For example, our lab uses
photosensitizers, which need to be kept at -20 in the dark. If you aliquot the
photosensitizer and keep them at -20, only using what you need, then it will
(probably) be OK. But, if you don't, and open the vial (even in the dark),
every day to take an aliquot, then each time it is opened, it loses it's
efficacy.

We also know that most chemicals are still OK even if the expiration date listed
on the bottle has passed. I believe most of us have to use our own judgment:
if the procedure is critical (i.e. immunohistochemistry-antibodies), aliquot
them, store according to MSDS and use a fresh aliquot, if the procedure is not
(routine buffers using basic compounds), continue to use the chemical: it is
pretty stable. This method is not good, or scientific, but it's probably the
best we can do.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Tindall, Randy D. [mailto:TindallR-at-missouri.edu]
Sent: Thursday, May 27, 2004 9:35 AM
To: microscopy-at-sparc5.microscopy.com

Hi again,

I think I need to restate my question about expiration dates on lab
chemicals, since I may have been unclear in my first posting.

I know that expiration dates are arbitrary and maybe even meaningless in
many cases, because they depend on so many variables. However,
sometimes we are required to put them on our reagents because of rules
regarding certain research projects.

For example, if a lab should perform electron microscopy as part of a
project involving a pharmaceutical company, chances are that the company
will require certain types of documentation, traceability, instrument
calibration, standardization of methods, etc. Expiration dates on
chemicals are often (maybe always) part of such requirements.
Diagnostic work is another probable example.

My question or proposal is this: Given that we are sometimes REQUIRED to
use expiration dates, wouldn't it be reasonable if there was some
consensus in our field we could point to and say "Our lab follows the
(for example) MSA standards on chemical usage."? As it is, I have not
yet been able to locate a set of standards to guide us in any sort of
meaningful compliance with such outside requirements. Phil Oshel has
suggested that the histotech community has been dealing with this for
some time, so I'm checking this out now (thanks for the suggestion,
Phil).

On the other hand, maybe this is something that doesn't need fixing,
because it ain't broke. I'm just curious what others think about it.

Thanks all.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 15:15:13 2004

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My first EM job was at a hospital. Coindentially, I
started work in the midst of a CAP inspection. I
checked and doubled checked all the reagents for
proper labeling. Reagents that were formulated in the
lab were given a 6-month expiration date from the prep
date. Most of the time, reagents 'keep' beyond the
expiration date. When making reagents, I try to make
a minimum volume that would generally last for 6
months. It helps to make minimum volumes to reduce
waste, too. And, unless your lab is especially
problem free when it comes to solution viability, it
helps to keep reagents for a set time in order to
maximize specimen quality during processing, staining,
etc. Hope that helps.
Sara Goldston

Bill Tivol {tivol-at-caltech.edu} wrote:

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Society of America

On May 25, 2004, at 11:08 AM, Tindall, Randy D. wrote:

} Does anyone else think it might be a useful exercise
to try and
} establish expiration dates for chemicals used in
microscopy labs? I
} understand that chemicals "expire" based upon what
they are, what use
} they are intended for, how they are used, what level
of
} accuracy/repeatability/etc. is expected from their
use, how they are
} stored, and many other factors. I have also read
Rande Kline's
} discussion of the problem in the July/August 2000
Microscopy Today on
} the difficulties of establishing such dates
(recommended).
}
} The problem is that some work requires lab
certification and strict
} laboratory guidelines requiring that all chemicals
be labeled with
} expiration dates----whether or not those dates have
any meaningful or
} consistent basis in "reality". So far, I've been
unable to find any
} such set of standards and my strong impression is
that labs set up
} their
} own arbitrary chemical rotation regimen.
}
Dear Randy,
Count me as one of the interested parties. Especially
since there are
several chemicals that we use sporadically, we need to
know what must
be made up fresh, and how long things keep.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

__________________________________
Do you Yahoo!?
Friends. Fun. Try the all-new Yahoo! Messenger.
http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 16:17:45 2004

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Dear Members,

Anyone knowing how to calculate models for amorphous
structure mentioned in Wharton's email? Thanks.
Zhongyi, ANL.

--- "Sinkler, Wharton" {Wharton.Sinkler-at-uop.com}
wrote: }
} Zhongyi,
}
} For an amorphous structure much of the same argument
} applies: If you drop
} the assumption about the atomic columns then you'll
} generally have some
} non-atom-like bound state functions, which oscillate
} in precisely the same
} way. However the eigenvalues (which determine the
} frequency of the
} oscillations) will be considerably smaller. Thus
} the oscillatory behavior
} won't show up until significantly larger thickness.
} Unfortunately I don't
} offhand know of any calculations for models of
} amorphous structures which
} specify the period of the oscillation for the
} deepest channeling state (a
} topic for a paper?, or maybe someone else on the
} list will be able to help).
}
}
} Wharton
}
}
} -----Original Message-----
} From: Zhongyi Liu [mailto:liu_zhongyi-at-yahoo.com]
} Sent: Thursday, May 27, 2004 2:23 PM
} To: Sinkler, Wharton
} Subject: [Microscopy] RE: imaginary part of exit
} wave
}
}
} Dear Wharton,
}
} Thank you very much for the answer. I will consult
} with your paper for details. A quick question again:
} if the specimen is an amorphous object (without
} well-defined atomic columns like crystals),and it
} cannot be approximated as weak phase object
} (metallic
} material and tens of nanometers in thickness), any
} idea how f2 will behave in this case, anything
} different from a general case?
}
} Thanks again.
}
} Zhongyi
}
} --- "Sinkler, Wharton" {Wharton.Sinkler-at-uop.com}
} wrote: }
} } Zhongyi,
} }
} } It is not generally true that the imaginary part
} of
} } the wave is always
} } positive (as it is by convention for a weak phase
} } object).
} }
} } A nice way to consider this is electron channeling
} } theory, a kind of
} } simplified dynamical theory which is approximately
} } correct for high
} } energies, and is most useful in the case that the
} } electron beam is aligned
} } with well-defined atomic columns. In this theory
} } the exit wave at an atomic
} } column looks like the column's projected
} potential,
} } but is modulated by a
} } function (exp(ik'z)-1). Here z goes through the
} } sample thickness and k' is
} } a constant which depends on what atoms occupy the
} } column.
} }
} } (Actually this is for the scattered part of the
} } wave, or y(r)-1, where the 1
} } represents the incident beam intensity)
} }
} } As you can see, when the argument of the
} exponential
} } is small everything is
} } zero (nothing is scattered yet). As z gets bigger
} } the imaginary part gets
} } positive at first (like the weak phase object
} } approximation), but then
} } swings around and becomes negative. For a typical
} } inorganic sample
} } containing say a column of first-row transition
} } metals, the function will
} } oscillate several times in a typical
} high-resolution
} } sample thickness of one
} } or two hundred angstroms, so this is not some
} } esoteric case but really
} } occurs in standard TEM conditions.
} }
} } This is a simplified model, but the agreement with
} } full dynamical
} } calculations is quite good. If you'd like to see
} a comparison (as
} } well as convince yourself that f2 does indeed go
} negative)
} } you can read more for
} } example in a paper by myself and Laurie Marks, J.
} } Microscopy vol. 194
} } (1999). Or if you have access to a multislice
} wave
} } simulation you can try
} } it for yourself.
} }
} } Best Regards,
} }
} } Wharton
} }
} }
}
****************************************************************
} } Wharton Sinkler, PhD.
} } UOP LLC
} } 25 E. Algonquin Rd.
} } Des Plaines, IL 60017-5017
} } tel. 847-391-3878
} } fax. 847-391-3719
} } mailto Wharton.Sinkler-at-uop.com
} }
} }
} }
} } -----Original Message-----
} } From: Zhongyi Liu [mailto:liu_zhongyi-at-yahoo.com]
} } Sent: Thursday, May 27, 2004 10:18 AM
} } To: Microscopy-at-MSA.Microscopy.Com
} } Subject: [Microscopy] imaginary part of exit wave
} }
} }
} }
} }
} }
}
----------------------------------------------------------------------------
} } --
} } The Microscopy ListServer -- Sponsor: The
} } Microscopy Society of America To
} } Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} }
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
}
----------------------------------------------------------------------------
} } ---
} }
} } Dear Members,
} }
} } Question: In the TEM, the exit wave (the wave
} } leaving
} } the specimen)is complex-valued in general, which
} can
} } be written as g = f1 + i*f2, where f1 and f2 are
} } real
} } numbers. Is it true/false that f2 has no sign
} } changes,
} } i.e. if positive, always positive?
} }
} }
} } With best regards,
} }
} } Zhongyi Liu
} } Argonne National Lab
} } Argonne, IL60439
} }
} }
} }
} }
} }
} }
} }
}
____________________________________________________________
} } Yahoo! Messenger - Communicate instantly..."Ping"
} } your friends today! Download Messenger Now
} } http://uk.messenger.yahoo.com/download/index.html
}
}
}
}
}
}
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Yahoo! Messenger - Communicate instantly..."Ping"
your friends today! Download Messenger Now
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From MicroscopyL-request-at-ns.microscopy.com Fri May 28 17:11:11 2004

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our EHS office has equally tough rules on how long we can keep "used
materials" which is what the rest of the world calls waste. we can't have
any "waste" since we are qualified to assess it. i got dinged for having a
metal can for "waste razor blades". but, on the other hand, my EHS office
did one great thing and I encourage you all to get you own schools to do
it. They have a building with chemicals that are no longer needed by an
individual lab. rather than my storing some "potassium permanganate" or
"lead nitrate" that I would never use again, they take it and keep it for
any faculty member who wants it. I go over a couple of times a year and
get a "free" bottle of some chemical that i am sure is not outdated. this
includes osmium in sealed ampules, lead nitrate, etc. They keep a running
total of how much they "save" consumers so they look good to the
administration but they are also saving disposal costs, minimizing unused
hazardous chemicals kept in labs that don't need them, and helping to save
the environment. check out the website at
http://www.missouri.edu/~muehs/recycling.htm and then tell your EHS people
to start their own Chemical Recycling program.

At 11:57 AM 05/28/04 -0700, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 20:23:55 2004

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This has been an interesting thread. I'd like to offer a couple of
observations:

My basic premise is that each laboratory needs to have at least minimal
documentation that lists reagents that are critical to the analysis where
expiration dates have been documented to be important and what those dates
are. Additionally, the laboratory quality system needs to have a minimal
complaint/anomaly recording-tracking system where either an investigator or
a client can question a result. When a result is questioned, the samples,
reagents, procedures, and instruments are scrutinized for bias. This process
can lead to refinement of the list of critical reagents. Every quality
system our company has used over the years has required something like this.
The "minimalist system" we now use requires just this. Auditors have always
been "data driven" and been satisfied when I had records that showed I did
what I said I did... By the way, an enthusiastic attitude helps here. A
belligerent attitude is a big mistake.

Like others have noted before, over the years we have noticed some reagents
are more sensitive than others. Our most frequent problem these days is
water contamination of solvents for casting uniform support films for TEM.

On the other hand, we have some reasonably old reagents that still work
well. We have some epoxy embedding resins that are approaching ten years
old. We found that by doubling the hardener from the levels we used "new"
that we still get good results. Just this week I floated several holey
cellulose acetate butyrate films that I had prepared on the slide in August,
1990. (When we make them, we make a lot of them...) The resulting holey
carbon films were just as sturdy as the films I floated back in 1990. I also
have an ethanol dispersion of graphitic carbon originally prepared back in
1982 from a small amount of graphitic carbon that I obtained from a vendor
application specialist who used to work for a carbon company. Any time I
need a test specimen, I sonicate the dispersion and spot some on a new holey
carbon support film. Each of these has been stored properly and is stable.

The key in all this is understanding the materials one uses, being alert to
variability, and keeping appropriate records of observed anomalies. This is
simply good laboratory practice that should have been stressed in our first
lab classes. Now we realize why our high school chemistry teachers collected
our lab notebooks and graded them (big grin.)

John Minter
jrminter-at-rochester.rr.com

From MicroscopyL-request-at-ns.microscopy.com Sat May 29 02:19:19 2004

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Last days for Fluorescence School in Genoa
Visit www.lambs.it and link to Fluorescence School on the opening page.
All my best
Alberto

------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat May 29 09:13:27 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (alvarobq-at-fcien.edu.uy) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Friday, May 28, 2004 at 09:41:06
---------------------------------------------------------------------------

Email: alvarobq-at-fcien.edu.uy
Name: Alvaro D. Olivera

Organization: Science Faculty

Education: Graduate College

Location: Montevideo, Uruguay

Question: I achieved a flat embedding (in Durcupan, Fluka)for TEM (over a glass slide)with immuno peroxidase - DAb(ABC Kit, Vector)tested tissue pieces of 50 microns and obtained very good results under light microscopy. After dissected the interest area, sticked it on a Araldite block. I cut 60 nm sections and mounted over 200 mesh Cu grids covered with Coat-Pen, and stained whith Uranyl acetate 5% in Ethanol(15 minutes)and after that with ReynoldĄs Lead citrate(7 minutes). When we observed under TEM (80 KV) it was good stained but we canĄt be sure to recognize the reaction correctly.I suppose what the electron density of the reaction itĄs not enough.
So what can I do? Do you use any enhancement kit?
Many thanks for your response. Alvaro.

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From MicroscopyL-request-at-ns.microscopy.com Sun May 30 12:25:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ottagonosole-at-tiscali.it) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, May 29, 2004 at 15:15:22
---------------------------------------------------------------------------

Email: ottagonosole-at-tiscali.it
Name: giovanni de caro

Organization: museo laboratorio di scienze naturali "S. Eugenio de Mazenod" - Ripalimosani - Italia

Title-Subject: [Microscopy] [Filtered] MListserver: AMR 1000 A SEM parts wanted

Question: "THE "S. EUGENIO DE MAZENOD" NATURAL SCIENCE MUSEUM AND LABORATORY IS A NO PROFIT SELF FUNDED PROJECT BASED IN SOUTHERN ITALY CREATED WITH THE AIM TO FOSTER SCIENTIFIC EDUCATION OF YOUNGSTERS (SEE OUR WEBSITE: http://web.tiscali.it/bimbononno). WE HAVE BEEN DONATED AN OLD AMR-LEITZ 1000 A SCANNING ELECTRON MICROSCOPE WHICH WE WISH TO RESTORE AND USE FOR OUR TEACHING ACTIVITIES. THE INSTRUMENT IS NOT WORKING; WE NEED SOME SPARE PARTS TO RESTART IT. IF ANYONE CAN HELP US PLEASE CONTACT US AT : ottagonosole-at-tiscali.it.
THANK YOU".

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 30 14:49:04 2004

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We would like to purchase a filter slider for epi-illuminator on Nikon Diaphot .

From MicroscopyL-request-at-ns.microscopy.com Mon May 31 08:43:12 2004

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Alvaro,
You should try either staining with uranyl acetate (aqueous) alone
or look at unstained samples, sometimes the full staining
(UA + PB) may hide the DAB product (by bringing up the rest
of the sample). Also try cutting thicker samples (0.15-.2
um) to have more reaction product. good luck.

Michael Delannoy

----- Original Message -----
} From: alvarobq-at-fcien.edu.uy (by way of MicroscopyListserver)

Colleagues

The April Archives are now on-line.

http://www.microscopy.com/MicroscopyListserver

Nestor
Your Friendly Neighborhood SysOop

From MicroscopyL-request-at-ns.microscopy.com Sat May 1 08:59:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (esem1-at-traceevidence.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, May 1, 2004 at 08:36:12
---------------------------------------------------------------------------

Email: esem1-at-traceevidence.org
Name: David Spence

Organization: Southwestern Institute of Forensic Sciences

Title-Subject: [Microscopy] [Filtered] MListserver:Looking For Used SEM, EDS and Coating Equipment

Question: I am looking for used SEM, EDS, sputter/carbon coater and related equipment. If you have or know of any equipment that is serviceable and available for haul-off or very inexpensive, please let me know. I am specifically looking for an older quality SEM with a motorized stage that is suitable for automated gunshot residue analysis.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 13:14:45 2004

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Dear Colleagues,

I am involved with a consortium that is being partially funded by the
NSF-ATE program. The main project involves the development of 3-D
images related to various science, math, engineering and technology
areas (from molecules to organs to CAD/architecture) so that they can
be projected (stereographic projection). Each institution
participating in the project will have a 3-D theatre built so that
SMET classes can be brought in for demonstrations of course specific
images (the theatre will house a Barco 3-D projector driven by a SGI
UNIX-based workstation and a special screen that retains
polarization). Students and faculty from the partner institutions
will also be trained in a residential program at Brookhaven National
Lab by their 3-D Visualization Team.

Since I have been teaching TEM and SEM courses at NCC for almost 20
years, I thought that it would be an interesting project to render
student and my own SEM & TEM images for 3-D projection. I have seen
many threads on 3-D imaging on this listserver and I would appreciate
some advice on where to begin. Initially, I am supposed to identify
some software applications that would be suitable for rendering 3-D
images of my micrographs. I am aware of some of the applications that
are used at BNL for their 3-D theatre such as OpenDX, Open GL and
Visualization ToolKit (VTK).

Can anyone suggest an application (UNIX based ideally) that I might
get started with? As a novice in this area I realize that the concept
of 3-D imaging and stereographic projection are probably two entirely
different principles. I would appreciate any references (articles,
books, websites) that will help me to understand the concepts.

Thanks for any assistance you can provide!

Steve
--
Stephen J. Beck
Professor
Bio-Imaging Center/Electron Microscopy
Department of Biology
Nassau Community College
Garden City, NY 11530
Voice Mail: (516) 572-7829
Email: {becks-at-sunynassau.edu}
URL: {http://www.sunynassau.edu/webpages/biology/becks.htm}

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 15:13:18 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (yuansheng-sun-at-uiowa.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Sunday, May 2, 2004 at 14:45:18
---------------------------------------------------------------------------

Email: yuansheng-sun-at-uiowa.edu
Name: Yuansheng Sun

Organization: University of Iowa

Education: Graduate College

Location: Iowa city, IA, USA

Question: Dear Madam or Sir:

I am doing a project on deconvolution for 3D phase contrast microscopy. As you know, it is very hard to measure a real psf. So I am wondering how to construct a theoretical psf based on the experimental parameters. Could you give me some infomation on this like some books or papers or technology documents. Thanks!
best from yuansheng

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From MicroscopyL-request-at-ns.microscopy.com Sun May 2 16:07:25 2004

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I have been using ImageJ and the VolumeJ plugin (for surface
rendering) to generate 3D anaglyphs (red/green stereo) as animations.
As has been mentioned in this group before, ImageJ is a free program
that has been ported from NIH-Image to the Java platform so that it
will work on almost any machine. You can get more information on
ImageJ at http://rsb.info.nih.gov/ij/

You can download a couple of the anaglyphs at
http://astro.temple.edu/~jbs/research/Anaglyphs. Remember that you
will need red/green glasses to get the full effect.

Joel

The images were originally obtained as z-series with a Leica confocal
microscope.

Date sent: Sun, 02 May 2004 14:17:59 -0400
} From: Steve Beck {becks-at-sunynassau.edu}

I second Joel's suggestion of ImageJ/VolumeJ. You might also want to take a look at VisBio (http://www.loci.wisc.edu/VisBio). VisBio is a open-source JAVA based image analysis tool for multidimensional biological image data. Features include measurement, volume rendering, and arbitrary image stack slicing. Integration with ImageJ is under development.

best regards,
kevin

Kevin W. Eliceiri
Laboratory for Optical and Computational Instrumentation
http://www.loci.wisc.edu
Room 271 Animal Sciences
1675 Observatory Drive
Madison, WI 53706
Phone: 608-263-6288
Fax: 608-265-3083

From MicroscopyL-request-at-ns.microscopy.com Sun May 2 19:05:12 2004

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Dear Steve,

I guess you know about the GeoWall (http://geowall.geo.lsa.umich.edu/)
projects. This is for geologists, but quite amenable to any type of 3D
projection really. Somewhat different to the setup you're proposing,
because it's PC- or Mac-based, but same principles. There's even a company
(VRCO) that sells turnkey systems. There is a bit of background information
on the GeoWall site, but more info on some of the link sites.

cheers,
Rosemmary

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

} From: Steve Beck {becks-at-sunynassau.edu}
} Date: Sun, 02 May 2004 14:17:59 -0400
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] 3-D Imaging & Projection
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
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-
}
} Dear Colleagues,
}
} I am involved with a consortium that is being partially funded by the
} NSF-ATE program. The main project involves the development of 3-D
} images related to various science, math, engineering and technology
} areas (from molecules to organs to CAD/architecture) so that they can
} be projected (stereographic projection). Each institution
} participating in the project will have a 3-D theatre built so that
} SMET classes can be brought in for demonstrations of course specific
} images (the theatre will house a Barco 3-D projector driven by a SGI
} UNIX-based workstation and a special screen that retains
} polarization). Students and faculty from the partner institutions
} will also be trained in a residential program at Brookhaven National
} Lab by their 3-D Visualization Team.
}
} Since I have been teaching TEM and SEM courses at NCC for almost 20
} years, I thought that it would be an interesting project to render
} student and my own SEM & TEM images for 3-D projection. I have seen
} many threads on 3-D imaging on this listserver and I would appreciate
} some advice on where to begin. Initially, I am supposed to identify
} some software applications that would be suitable for rendering 3-D
} images of my micrographs. I am aware of some of the applications that
} are used at BNL for their 3-D theatre such as OpenDX, Open GL and
} Visualization ToolKit (VTK).
}
} Can anyone suggest an application (UNIX based ideally) that I might
} get started with? As a novice in this area I realize that the concept
} of 3-D imaging and stereographic projection are probably two entirely
} different principles. I would appreciate any references (articles,
} books, websites) that will help me to understand the concepts.
}
} Thanks for any assistance you can provide!
}
} Steve
} --
} Stephen J. Beck
} Professor
} Bio-Imaging Center/Electron Microscopy
} Department of Biology
} Nassau Community College
} Garden City, NY 11530
} Voice Mail: (516) 572-7829
} Email: {becks-at-sunynassau.edu}
} URL: {http://www.sunynassau.edu/webpages/biology/becks.htm}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 08:17:48 2004

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Hi all-

I've just completed a great semester of teaching EM techniques. The
student projects that were required are quite interesting.
If you have a chance, please review the student's work at this URL:

http://xray.optics.rochester.edu/workgroups/cml/opt307/index.html

Thanks!
Brian

_________________________________________________
Brian McIntyre
Univ. of Rochester
The Institute of Optics
River Campus EMLab
585-275-3058/4875
585-244-4936 (fax)

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 08:36:45 2004

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Hi

Please help me. I'm really in trouble.
Just burned the second filament after 3 hours. Previously, I had about 200 h. Now the current is very unstable.
Before burning, is slowly going down and after that a quick increase up to 170 uA and bang.
We have a Jeol 1010 (1 year old).

Many thanks,
Luci
_________________________________________
Lucian Barbu-Tudoran
Electron Microscopy Center
Faculty of Biology & Geology
Babes-Bolyai University of Cluj-Napoca
5-7 Clinicilor Str., 3400 Cluj-Napoca, Romania
Tel/Fax: +40 264 598700
{http://hasdeu.ubbcluj.ro/emc/lucian_barbu_tudoran.htm} http://hasdeu.ubbcluj.ro/emc/lucian_barbu_tudoran.htm

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 08:43:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mcintyre-at-optics.rochester.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, May 3, 2004 at 08:10:50
---------------------------------------------------------------------------

Email: mcintyre-at-optics.rochester.edu
Name: Brian McIntyre

Organization: Univ.of Rochester

Title-Subject: [Microscopy] [Filtered] Review of Student Projects

Question: Hi all-

I've just concluded a great semester of teaching EM techniques to a mixed group of undergrads and grads. They've put together some interesting projects that are posted on the web here:

http://xray.optics.rochester.edu/workgroups/cml/opt307/index.html

Please take a look and provide feedback to them and me.

Thanks!
Brian

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 09:12:16 2004

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} Dear Listserver,
}
} I have recently processed Hela cells grown on covertslips by
} conventional chemical fixation( 2.5% formaldehyde plus 2.5% glutaraldehyde
} for 2h and postfixation in 1.5% Osmium in 0.1M sodium cacodylate buffer,
} dehydrated in a series of concentrations of ethanol over a period of 90
} minutes and then infiltrated in Epon-aradite). After sectioning, I stained
} the sections with 2% uranyl acetate in distill water for 10 min and lead
} citrate for 5 min. I could hardly visualize the membrane structrue,
} particularly nuclear membrane, plasma membrane, Golgi apparatus and ER
} membranes. However the other structures were well preserved. I am here
} asking for your advice and greatly appreciate any suggestions!
}
} Thank you very much in advance!
}
} Guofeng Zhang, Ph.D
} Division of Bioengineering & Physical Sciences
} National Institute of Health
} Bethesda, MD 20892
} Tel: 301-451-3856
} Email: zhangguo-at-mail.nih.gov
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 12:14:15 2004

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Hello,

I'm trying accquire EDS spectra of various posphors and am having
difficulty. There are peaks that do not seem to match any known elements,
and all of the peaks shift up and down in energy from one spectrum to the
next. I'm wondering if this is a common phenomenon with phosphors, or is my
system out to lunch? All ideas are welcome!

Diane Ciaburri

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 12:33:56 2004

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Guofeng

Having been around for what seems like forever, I really did not write
up some of the old literature as some of our students have suggested.
But there are old reports of just this problem. The conclusion was that
osmication does not adequately stabilize membranes against extraction
during ethanol dehydration. The reference is a bit fuzzy, but I believe
it was Dan Pease’s book ‘Histological Techniques for Electron
Microscopy’, 2nd edition, 1964. It was also never clear whether it was
the ethanol or the propylene oxide intermediate which was responsible
for membrane extraction. We have tested this out and confirmed that,
for whatever reason, in our hands we will see the loss of membranes you
describe if we use the procedures as you list.

There are two solutions. First, post-fixation in uranyl acetate.
Uranyl acetate will stabilize membranes. We wash 1x in buffer and 3x in
filtered water after the osmication step, and then fix in 2% UA. Our
monolayers and free suspensions are usually only fixed for a couple of
hours, but we do leave them in UA for up to several days without noting
any deleterious effect. This step usually improves stabilization of
membranes in our hands.

The second solution is to dehydrate in acetone. There are two reasons,
first is that acetone is not reported to extract membranes, and second,
you do not need an intermediate step such as propylene oxide, but go
directly into graded acetone:plastic for infiltration. This second
reason saves on costs, reduces turnaround, and is a little more
environmentally friendly. In fact, we have found that using acetone is,
by itself, sufficient to ensure good membrane stabilization.

Our normal procedure now is to use both UA en bloc postfixation followed
by acetone dehydration. Our results are usually very good, and we never
lose membranes.

Hope these ideas help.

Paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 13:07:05 2004

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On May 2, 2004, at 11:17 AM, Steve Beck wrote:

} Can anyone suggest an application (UNIX based ideally) that I might
} get started with? As a novice in this area I realize that the concept
} of 3-D imaging and stereographic projection are probably two entirely
} different principles. I would appreciate any references (articles,
} books, websites) that will help me to understand the concepts.
}
Dear Steve,
If you do not get sufficient info from this list, try the 3dem list:

} ADMINISTRIVIA
}
} To post to this list, send mail to
}
} 3dem-at-ucsd.edu
}
} To subscribe to this list, send mail to
}
} majordomo-at-3dem.ucsd.edu
}
} with the text
}
} subscribe 3dem
}
} in the body of the message (not in the Subject:).
}
} To unsubscribe from this list, send mail to
}
} majordomo-at-3dem.ucsd.edu
}
} with the text
}
} unsubscribe 3dem
}
} in the body of the message (not in the Subject:).

I also know that the group at the Wadsworth Center in Albany NY has
prepared stereo images from 3-D reconstructions, so you might want to
contact them.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 13:38:17 2004

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} } I have recently processed Hela cells grown on covertslips by
} } conventional chemical fixation( 2.5% formaldehyde plus 2.5% glutaraldehyde
} } for 2h and postfixation in 1.5% Osmium in 0.1M sodium cacodylate buffer,
} } dehydrated in a series of concentrations of ethanol over a period of 90
} } minutes and then infiltrated in Epon-aradite). After sectioning, I stained
} } the sections with 2% uranyl acetate in distill water for 10 min and lead
} } citrate for 5 min. I could hardly visualize the membrane structrue,
} } particularly nuclear membrane, plasma membrane, Golgi apparatus and ER
} } membranes. However the other structures were well preserved. I am here
} } asking for your advice and greatly appreciate any suggestions!

Try increasing the time in uranyl acetate to 25 or more minutes, and
decrease the time in lead citrate to 3 minutes. Unintuitively, sometimes
longer times in the lead citrate causes bleaching rather than staining!

On the other hand, I've also had success with 10 minutes in each, and with
5 minutes in lead followed by 10 minutes in UA followed by another 10
minutes in lead, and many other variations. Try several approaches and see
what works for you!

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 14:08:00 2004

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Dear Guofeng. I have worked on many cell culture preps. I normally use
microwave processing however for bench processing I would recommend that
you shorten all your processing steps. I would bench fix in glut and
osmium for 20 mins each at room temperature for example. I use 2%
glutaraldehyde on 0.1 M cacodylate buffer. I wash in 0.1M cacodylate
buffer with 0.3M sucrose added. I also add 0.3 M sucrose to the post fix.
The cells are very thin and not like a tissue chunk. Also, dehydration
times should be very short- 1-2 mins is sufficient. in your alcohol changes.
Cultured cells don't have much contrast so try using a reduced osmium fix
(2% osmium tetroxide in 0.1 M cacodylate buffer containing 0.8% potassium
ferricyanide). it gives really nice contrast to membranes and
cytoskeleton. Also try an en bloc UA step before the dehydration.
Your post staining sounds OK.
Good luck
JoAnn Buchanan
Dear Listserver,
}
} I have recently processed Hela cells grown on covertslips by
} conventional chemical fixation( 2.5% formaldehyde plus 2.5% glutaraldehyde
} for 2h and postfixation in 1.5% Osmium in 0.1M sodium cacodylate buffer,
} dehydrated in a series of concentrations of ethanol over a period of 90
} minutes and then infiltrated in Epon-aradite). After sectioning, I stained
} the sections with 2% uranyl acetate in distill water for 10 min and lead
} citrate for 5 min. I could hardly visualize the membrane structrue,
} particularly nuclear membrane, plasma membrane, Golgi apparatus and ER
} membranes. However the other structures were well preserved. I am here
} asking for your advice and greatly appreciate any suggestions!
}
} Thank you very much in advance!
}
} Guofeng Zhang, Ph.D
} Division of Bioengineering & Physical Sciences
} National Institute of Health
} Bethesda, MD 20892
} Tel: 301-451-3856
} Email: zhangguo-at-mail.nih.gov
}

Department of Molecular and Cellular Physiology
Stanford University School of Medicine
Stanford, CA 94305
650-723-5856

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 14:24:13 2004

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On May 3, 2004, at 10:16 AM, Diane.Ciaburri-at-gd-ais.com wrote:

} I'm trying accquire EDS spectra of various posphors and am having
} difficulty. There are peaks that do not seem to match any known
} elements,
} and all of the peaks shift up and down in energy from one spectrum to
} the
} next. I'm wondering if this is a common phenomenon with phosphors, or
} is my
} system out to lunch? All ideas are welcome!
}
Dear Diane,
I assume you're looking at inorganic phosphors, such as CdS, etc., in
which case there should be no problem. Just because it's a phosphor
does not change the interaction with beam electrons that produces
x-rays. There might be contaminants in the mix, but these would be
minor--not ~10%--so there could be some very small peaks, but
everything should match one or more known elements. Have you
calibrated the energy spectrum? The energies should not shift--the
only way that might happen is if the majority of the x-rays were
inelastically scattered. If you take multiple spectra from a single
area (assuming that there is not significant loss of material during
data collection) neither the energies nor the intensities should vary.
I suggest putting in a standard, such as Al evaporated onto a formvar
film on a Cu grid, and taking spectra from locations where both the Al
and Cu signals are strong. The spectra should be consistent, and you
should be able to check the energy calibration and see if the
resolution is OK. To see if the resolution meets spec, put in a grid
with Mn evaporated on formvar and measure the FWHM of the peak.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 15:03:34 2004

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Try changing your fixation protocols. I use the following fixatives
to help with membrane preservation:

"Yellow Fix for EM" (based on Ito, S and Karnovsky J. J Cell. Biol
Abstract 1968)
2.5% glut.
4.0% paraformaldehyde
0.02 % picric acid
in 0.1M sodium cacodylate buffer

(I use 20ml of 0.2M buffer, 10ml of 10% glut, 10 ml of 16% pfa and 2
ml of a saturated sol. of picric acid--I keep a jar of it in my hood,
with the crystals covered with water and draw off as I need it,
adding fresh water when I'm done so that it doesn't explode.)

For a secondary fix I use 1% osmium tetroxide and 1.5% potassium
ferricyanide (aqueous)made up my mixing stock solutions of 2% osmium
and 3% K-ferr 1:1.

Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 15:06:27 2004

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Cool! Well, maybe not for you.

We have an infrared chamber-scope that I have to instruct users to turn off
before they do any EDS. Otherwise, the flood of IR photons overwhelms the
EDS detector and runs it up to 100% dead time. Under less overwhelming
conditions, the photons are still detected and their energy adds on to the
real energy of the x-ray photons and peaks get shifted upscale. Its kind of
fun to watch the effect on our spectrum as we turn the light on and off and
the spectral peaks shift back and forth.

I had never thought about it, but the same effect should be expected when
working with cathodo-luminescent materials. And your phosphors are
definitely luminescent.

I recall that some EDS detectors have their windows coated (with Al, I
think) to avoid just this problem. I don't know if that is something that
can be done very well to an existing detector. I don't suppose you could
interpose another film in front of your detector; it would probably also
absorb your x-rays.

I wonder how others would suggest dealing with this.

Warren

At 12:16 PM 5/3/2004, you wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 15:30:18 2004

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Luci, the Microscopy Today journal, March/April 2003
issue has an article on "The Life and Death of a
Tungsten Hairpin Filament". In it there is described
the different failure modes for a hairpin filament
which may help you.

You should be able to access this article via the
following link:

http://www.microscopy-today.com/TableofContentsPDF.html

Stu Smalinskas, P.E.
Metallurgist
SKF
46815 Port Street
Plymouth, Michigan 48170

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Luci wrote:

Hi

Please help me. I'm really in trouble.
Just burned the second filament after 3 hours.
Previously, I had about 200 h. Now the current is very
unstable.
Before burning, is slowly going down and after that a
quick increase up to 170 uA and bang.
We have a Jeol 1010 (1 year old).

Many thanks,
Luci
_________________________________________
Lucian Barbu-Tudoran
Electron Microscopy Center
Faculty of Biology & Geology
Babes-Bolyai University of Cluj-Napoca
5-7 Clinicilor Str., 3400 Cluj-Napoca, Romania
Tel/Fax: +40 264 598700
{http://hasdeu.ubbcluj.ro/emc/lucian_barbu_tudoran.htm

__________________________________
Do you Yahoo!?
Win a $20,000 Career Makeover at Yahoo! HotJobs
http://hotjobs.sweepstakes.yahoo.com/careermakeover

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 16:24:54 2004

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We would guess the problem may be in your power supply. Your 200+ hours
indicates a good vacuum and clean system. Our customers average 200+ on
rebuilt filaments and slightly less on new filaments due to the special
process used on rebuilt filaments.

Based on your comments, I'd check with Jeol services.

John Arnott

Disclaimer: Ladd Research is a supplier of a wide variety of microscope
supplies and accessories, including new and rebuilt filaments.

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com

----- Original Message -----
} From: "Lucian Barbu (by way of Ask-A-Microscopist)"
{lbarbu-at-hasdeu.ubbcluj.ro}
To: {microscopy-at-ns.microscopy.com}
Sent: Monday, May 03, 2004 9:40 AM

Bill,

Yes, the system was just calibrated last Friday, and I double-checked it
again today which led me to think there must be something funny happening
with the samples. Here's the answer, thanks to a variety of helpful hints I
received. Apparently my detector is sensitive to visible light and the
whole spectrum was being shifted to higher energies by varying amounts
(depending on how much light I was generating). By switching from my thin
window to my berillium window, and blocking the visible light, things make
sense again.

Thanks, Bill and everyone else that responded. You guys are life savers!

Diane Ciaburri

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Monday, May 03, 2004 3:32 PM
To: microscopy-at-msa.microscopy.com

Dear Diane,
If you are using the modern thin-window EDS detectors sold nowadays, you should
know that they are very susceptible to light and that could easily be the source
of your strange signals. The old-style Be-window detectors were not
light-susceptible, so if you can find one you can test the elements above Ne.
For the elements below that, perhaps using a low accelerating voltage ( {5 kV)
will reduce the light emission from the phosphor enough to get a reading on a
thin-window detector.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {Diane.Ciaburri-at-gd-ais.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Monday, May 03, 2004 10:16 AM

Paul and Guofeng
I never though for staining in UA after osmication as a
"postfixation". It's hardly believe to me that UA has something to do with
"fixation". In my point of view UA stained positively nucleic acids and
don't interfere with membranes. When I need reduce the appearance of the
ribosomes in neurone's cytoplasm, I used to remove UA staining after
osmication step from procedure. In my hands, it absolutely does not affect
membranes (I did both: with and without that step). I used Spurr, not
Epon. I also did not see any effect of ethanol on membranes. I think, if
you are using it for 10-15 min each step, it should not affect membrane's
quality, otherwise nearly whole EM is pure artefact (most people still use
ethanol). The basic reason, not to use acetone for dehydratation is
because acetone is very strong denaturing agent (contrary to ethanol), so
acetone will definitely alternate the fine structure. For this reason,
people use acetone in freeze-substitution procedure at low temperature to
reduce denaturing effect of acetone. Returning back to original question,
I would suggest to check is OsO4 was good or not. If there is any
suspicious there, you need to use fresh solution/chemicals. After
osmication the tissue (even in monolayer) should turn brown. Sergey

At 12:36 PM 5/3/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Mon May 3 18:28:33 2004

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Mary & Co.,

I think Diane's issue with phosphorous is visible fluorescence similar to the face of a CRT. After all, to get an image on a TV screen we shoot electrons at phosphorous coated screens and hence it fluoresces in visible light, and likely IR as well. Ideal to make the EDX detector do odd things. Chamberscopes, as Warren indicated, have the same effect.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
Sent: Monday, May 03, 2004 5:53 PM
To: Diane.Ciaburri-at-gd-ais.com
Cc: Microscopy

Dear Diane,
If you are using the modern thin-window EDS detectors sold nowadays, you should
know that they are very susceptible to light and that could easily be the source
of your strange signals. The old-style Be-window detectors were not
light-susceptible, so if you can find one you can test the elements above Ne.
For the elements below that, perhaps using a low accelerating voltage ( {5 kV)
will reduce the light emission from the phosphor enough to get a reading on a
thin-window detector.
Regards,
Mary Mager
Electron Microscopist
Metals and Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {Diane.Ciaburri-at-gd-ais.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Monday, May 03, 2004 10:16 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donaldawbrey-at-hotmail.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, May 3, 2004 at 12:44:21
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Email: donaldawbrey-at-hotmail.com
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] MListserver: EM scopes

Question: Dear MSA netters,

Our department is in the preliminary stages of aquiring a new electron microscope. The one in use is antiquated. I would like to have as many opinions of different scopes and their ancillary systems.

We are looking for a scope to be used for diagnostic services (such as kidney biopsies, tumors, and etc.).

Our requirements are: 120kv, flat bed camera scanner, subliminal printer, image software, dual digital/manual capabilities.

Thank you in advance for any opinions.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon May 3 21:47:58 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ecd10-at-psu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, May 3, 2004 at 14:10:00
---------------------------------------------------------------------------

Email: ecd10-at-psu.edu
Name: Elizabeth Dickey

Organization: Pennsylvania State University

Title-Subject: [Microscopy] [Filtered] MListserver:Postdoc opening at Penn State

Question: POST-DOCTORAL POSITION
in
Electron Microscopy of Nanostructured Electronic Materials
at
The Pennsylvania State University

A postdoctoral position is available in the area of nanostructured electronic materials beginning July 1, 2004. The research project focuses on understanding interface structure and chemistry in heterostructured thin films and nanowires. Aspects of the project will be conducted under the auspices of an NSF-NIRT program on semiconducting nanowires. Through a variety of electron imaging and spectroscopy techniques we aim to quantify atomic structure and chemistry of interfaces in heterostructured materials. Most of the research will be conducted on a JEOL 2010F Field Emission TEM/STEM outfitted with an EDAX energy dispersive x-ray spectrometer (EDS), Gatan Enfina electron energy loss spectrometer (EELS), high-angle annular dark field STEM detector, and acquisition hardware and software for spectrum imaging. The ideal candidate for this position will have experience in HRTEM, STEM, EDS and EELS. The salary will be commensurate with qualifications and experience.

Please forward questions or send applications to:

Professor Elizabeth Dickey
Department of Materials Science and Engineering
The Pennsylvania State University
223 Materials Research Building
University Park, PA 16802
USA

tel: (814) 865-9067
FAX: (814) 865-2326
email: ecd10-at-psu.edu

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From MicroscopyL-request-at-ns.microscopy.com Tue May 4 03:20:46 2004

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Hi all !

does anyone know some manufacturers or distributors of coloďdal silica
also called "syton", for microsectionned dies polishing process ?

thanx in advance...

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 11:03:10 2004

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Dear Sylvain:

South Bay Technology offers 3 types of Colloidal Silica for cross
sectioning of semiconductor materials - as well as other applications.
The products we offer are:

CS1 - Non-crystallizing Colloidal Silica
CS2 - Syton
CS3 - Glanzox

All of these products are available through our local distributor in
France. All of our distrinbutor contact information can be found on our
website. As luck would have it, "Colloidal Silica" is also the featured
product on our website today. You can go to www.southbaytech.com and
find information on the colloidal silica products on the main page.
Alternatively, you can enter "colloidal silica" in the product search
box to bring up all references to our various colloidal silica products.

I hope this helps.

Best regards-

David

sylvain maury wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
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South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

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Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
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From MicroscopyL-request-at-ns.microscopy.com Tue May 4 12:41:00 2004

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The clinical lab I used to work in had a Codonex
di-sub printer which we rarely used. Overall, our
imaging software (Gatan Micrograph ~2+years old) did
not jive with the printer too well - less resolution
with printed image. Not to say its a bad system. It
might have been because our imaging program needed
updating. Case in point, scanned images that were
'tweeked' in Adobe and printed with the Codonex came
out excellent.
Sara Goldston

by way of MicroscopyListserver
{donaldawbrey-at-hotmail.com} wrote:

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The Microscopy ListServer -- Sponsor: The Microscopy
Society of America

Below is the result of your feedback form
(NJZFM-ultra-55). It was submitted by
(donaldawbrey-at-hotmail.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html
on Monday, May 3, 2004 at 12:44:21
---------------------------------------------------------------------------

Email: donaldawbrey-at-hotmail.com
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] MListserver: EM
scopes

Question: Dear MSA netters,

Our department is in the preliminary stages of
aquiring a new electron microscope. The one in use is
antiquated. I would like to have as many opinions of
different scopes and their ancillary systems.

We are looking for a scope to be used for diagnostic
services (such as kidney biopsies, tumors, and etc.).

Our requirements are: 120kv, flat bed camera scanner,
subliminal printer, image software, dual
digital/manual capabilities.

Thank you in advance for any opinions.

---------------------------------------------------------------------------

__________________________________
Do you Yahoo!?
Win a $20,000 Career Makeover at Yahoo! HotJobs
http://hotjobs.sweepstakes.yahoo.com/careermakeover

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 16:31:39 2004

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Dear Listserver,

Many thanks to all of your helpful comments and suggestions on membrane
visualization problems! I think I will get succeed in solving the problems
in near future after taking your advise.

Kind Regards!

Guofeng
}
} Guofeng Zhang, Ph.D
} Division of Bioengineering & Physical Sciences
} National Institute of Health
} Bethesda, MD 20892
} Tel: 301-451-3856
} Email: zhangguo-at-mail.nih.gov
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 17:14:38 2004

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Listers,
I have a researcher wanting to look at seed surface morphology. These
seeds are from dried herbarium sheets. I initially had him simply treat
the seeds with acetone to remove any waxes from the surface and then
O-T-O-T-O them. This was not adequate as we saw what I believe to be
fungal hyphae and spores plus a LOT of debris. Does anybody have a
"tried and true" (and easy!) method of preparing seeds? I was thinking
about doing acetolysis or 10% KOH, which I do with pollen routinely, but

wasn't sure how the seed surface would hold up. Also, I don't think the
person sonicated in acetone. Might that alone be adequate? TIA.

Bill

--
=============================================================
Bill Chissoe III
Electron Microscopist
University of Oklahoma
770 Van Vleet Oval
Norman, Ok. 73019
E-mail: wchiss-at-ou.edu Ph. (405)325-4391
=============================================================

From MicroscopyL-request-at-ns.microscopy.com Tue May 4 20:01:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (cmeyer911-at-yahoo.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 4, 2004 at 19:31:16
---------------------------------------------------------------------------

Email: cmeyer911-at-yahoo.com
Name: Chris Meyer

Organization: Boeing

Title-Subject: [Microscopy] [Filtered] [TEM EELS Gatan 607]

Question: I have an old Gatan Model 607 EELS system that I have never run (I'm new to TEM). It used to be run by a TN-5500 system, that is soon to be replaced with a new EDS system. I do not want to lose EELS capability for future projects. A Gatan representative informed me the 607 system could be run with a Mac with an old operating system.

I'd like to talk (email) to any current or former 607 EELS users that would have ideas on how I could keep this capability for the future. Is my only option to keep the TN-5500 for this purpose alone? I'd appreciate it. Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 02:58:16 2004

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look on the www.struers.com

best regards

chris

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 07:49:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jacqui.ross-at-auckland.ac.nz) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 4, 2004 at 23:18:40
---------------------------------------------------------------------------

Email: jacqui.ross-at-auckland.ac.nz
Name: Jacqui Ross

Organization: The University of Auckland

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: We are about to buy a new inverted fluorescence microscope, probably a Nikon.

Does anyone have any experience/feedback about the Nikon Digital Sight colour camera (DS-5Mc-U1)? We are intending to buy the new cooled one and I would appreciate hearing from anyone who has used one or seen one demonstrated recently.

Cheers,

Jacqui.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 14:48:22 2004

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Listers,

Here is the TABLE OF CONTENTS for the MAY 2004 issue of MICROSCOPY TODAY.

New Subscriptions via http://www.microscopy-today.com only, please.
New subscriptions will close on Tuesday May 11th for this issue.

WE HAVE PURGED NON-MSA MEMBER, NON-NORTH AMERICAN, UNSUBSCRIBED INDIVIDUALS!
SEVERAL HUNDRED NON-QUALIFIED SUBSCRIBERS HAVE BEEN PURGED.

Scanning Wet Specimens
.Stephen W. Carmichael and Wilma L. Lingle, Mayo Clinic

Laboratory Design for High-Performance Electron Microscopy
.M.A. O'Keefe, et al., LBNL; C.J.D. Heatherington, et al., Oxford; B.
.Carragher, et al., Scripps; L.F. Allard, et al., ORNL

New CMEIAS Image Analysis Software for Computer-Assisted Microscopy of
Microorganisms and Their Ecology
.Frank B. Dazzo, Michigan State University

Making Slide Shows in Acrobat
.Jerry Sedgewick, University of Minnesota

Sub-Angstrom Resolution with a Mid-Voltage TEM
.M.A. O'Keefe, C.J.D. Hetherington, E. C. Nelson, LBNL, Berkeley

Viability and Versatility of the Yeast Cell
.Michelle J. Henry-Stanley & Carol L. Wells, Univ. of Minnesota

New Adhesion Mechanism in Giardia: Role of the Ventrolateral Flange in the
Attachment of Trophozoites to Rough and Porous Surfaces
.S.L. Erlandsen, U. Minnesota; A.P. Russo, & J.N. Turner, New York
.Wadsworth Center

Project VISUAL: Facilitating the Connection Between Art and Science
.L.M. Strzegowski & T.P. Russell, U. of Massachusetts, Amherst

Use and Disposal of Uranyl Acetate in the Electron Microscope Laboratory:
Glow in the Dark or Walk in the Park?
.Randy Tindall, University of Missouri

Confocal Microscopy for Diagnostic Cytology
.M.E. Boon, & L.P. Kok, U. Groningen, The Netherlands

Technical Note on the Preparation of Un-decalcified Trabecular Bone for
Examination by TEM
.Jeannette Taylor, Emory Univ. & Iwona Jasiuk, Georgia Inst. of Technology

The Low Voltage SEM Imaging Advantage: A Reminder
.Steven S. Hurban. Endicott Interconnect Technologies, Inc. NY

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:53:09 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (fremingt-at-fhcrc.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 5, 2004 at 11:24:55
---------------------------------------------------------------------------

Email: fremingt-at-fhcrc.org
Name: Franque Remington

Organization: Fred Hutchinson Cancer Research Center

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Many Thanks to all who offered suggestions and techniques for preserving conidia for SEM. They have been very helpful.

Franque Remington

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:53:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwareham-at-utah.gov) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 5, 2004 at 15:08:22
---------------------------------------------------------------------------

Email: bwareham-at-utah.gov
Name: Beverly Wareham

Organization: Utah Veterinary Diagnostic Lab

Title-Subject: [Microscopy] [Filtered] Fixation of animal lung tissue

Question: Hi all,
Does anyone have a protocol for fixing animal lung tissue (sheep) for EM and is willing to share it? I'd really appreciate it.

Thanks,
Beverly Wareham
Utah Veterinary Diagnostic Laboratory
435-797-1799
bwareham-at-utah.gov

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:54:19 2004

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Dear listers,

Sometimes you just gotta share the good news. After trying out my share
of handheld vacuum cleaners for small lab cleanup jobs and finding them
all to be pretty asthmatic, I finally hit paydirt. I found something
called the Euro Pro 700 watt hand vac down at the local Office Depot for
about $30, complete with small hose, attachments and shoulder strap.
Not only does it clean up the plastic fluff that builds up in
ultramicrotomy areas, it would probably suck up the whole microtome if
you turned your back. That's probably why it's also called "The Shark".

No financial interest, just a (finally) happy owner of a tiny vacuum
cleaner that works!

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Wed May 5 16:54:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ananthpb-at-rediffmail.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 5, 2004 at 16:07:20
---------------------------------------------------------------------------

Email: ananthpb-at-rediffmail.com
Name: Ananth Puthucode

Organization: Univ. North Texas

Title-Subject: [Microscopy] [Filtered] electropolisher

Question: Hi all,

I am looking for a used electropolisher for TEM sample preparation. Please let me know if anyone has got one and planning to sell it.

Thanks,
Ananth

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 03:53:57 2004

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hello microscopists !

I have a question for those who work in Failure Analysis of
semiconductors but anyone can answer...

I'm trying to define a methodology to use colloidal silica for polishing
process of microsectionned dies (Si, AsGA), for SEM observations. I'd
like to know the conditions that people commonly use for their sample
preparations with Syton.
Any suggestions are welcome...
Thanx in advance!

and thanx to David Henricks : i just received the documents about
colloidal silica and SEM sample preparation. But the paper about iridium
sputtering was not in the package. You must have forgotten it, but it
doesn't matter. thanx again...

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 07:28:23 2004

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-----

} hi !
}
} ask the company name "logitech" (a division from struers denmark)
} they are have a special equipment for polishing semiconductors !
} email info-at-logitech-us.com or www.logitech.uk.com
}
} best regards
}
} chris huebner
}
} Foundry Research Insitute, Kraków - Poland
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 08:38:24 2004

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Randy

I don't know if anyone else would wish to confirm my fears but I am concerned about the use of any basic vacuum cleaner for clearing up resin dust.

The problem as I see it is:
1. Vacuum cleaners do pump out small particles from their exhaust (unless they have some very fine submicron exhaust filter).
2. It's the fine stuff (below 2 or 3 microns) that remains airborne and worse still is the ideal size for inhalation. It is much more likely to penetrate deeper into the respiratory tract (hence the problem with certain sizes of dust such as asbestos).
3. Resins used for most biological purposes are not completely polymerised at 60 to 80 degrees. They are usually regarded as safe enough to handle but could well be hazardous if inhaled and retained in the lungs for long enough.

If you combine the above facts with, for instance, sawing or grinding resins (particularly epoxies like Spurr's) then you might actually be increasing your exposure to the most hazardous component of the resin dust. Generally I try to avoid sawing and only ever trim blocks with razor blades or glass knives because the pieces are big and even if you could inhale some I doubt they'd ever reach your lungs.

Some of this is assimilated information from years ago, so I can't give you a particular source or reference. I suspect that you could easily check if there is a problem by putting a 'sticky' stub near to the exhaust of your vacuum cleaner and see if it picks up much. I've never tried it because I just simply avoid fine dust now.

Malcolm

Malcolm Haswell
e.m. unit
University of Sunderland
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: "Tindall, Randy D." {TindallR-at-missouri.edu}

The International Metallographic Society is seeking a volunteer to serve as
the Local Chair for the 2005 International Metallographic Contest which will
be held in conjunction with the 38th Annual Convention of the IMS and the
Microscopy and Microanalysis 2005 meeting in Honolulu, Hawaii in July of
2005. Interested individuals from the Honolulu area should contact the
Contest Chair, Jeff Stewart, at jeff-at-metallography.com for additional
information. We would like to have the position filled within the next few
weeks.

Thanks,

Jeff Stewart
International Metallographic Contest Chair
Metallographic Laboratory Manager
Stern-Leach Co.
49 Pearl Street
Attleboro, MA 02703 USA
Phone: 508-222-7400 extension 1329
Fax: 508-699-4030
E-mail: jeff-at-metallography.com

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 08:43:47 2004

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Good points, Malcolm. I forgot to mention that this thing comes with a
HEPA filter. Anyway, most of our resin fluff comes from block trimming
with razor blades and glass knives.

Randy

-----Original Message-----
} From: Malcolm Haswell [mailto:malcolm.haswell-at-sunderland.ac.uk]
Sent: Thursday, May 06, 2004 8:42 AM
To: MSA microscopy listserver
Cc: Tindall, Randy D.

Micromavens,

I'm hoping to find someone with a Gatan model 626
cryostage/cryoholder who wishes to sell it or donate it to a
university. Cryostation is not necessary, we've got that. Anyone out
there?
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 10:12:47 2004

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One of faculty here will be processing lengths of rat femoral artery
for light microscopy and needs to keep track of the distal vs
proximal ends. She tried marking one end with India Ink, but it was
washed out sometime during the dehydration/xylene steps.
Any ideas?
Thanks,
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 10:49:32 2004

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Hi Beverly,

I was on a TEM project many years ago working with sheep and chicken
lungs. Jeff Weidner was the PI on the project. The problem in the
we had was to get the air out of the lungs before we could any of the
specimen prep procedures to work well. To many air bubbles and poor
infiltration.

We ended up use a standard EM procedure with each step done under low vacuum.

Mike

} ------------------------------------------------------------------------------
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--
===================================================================================
Michael Dunlap
office (530) 752-0284
University of California lab (530) 752-5489
Chemical Engineering & Material Science Fax (530) 752-9554
110A Kemper Hall mrdunlap-at-ucdavis.edu
One Shields Ave.
http://www.chms.ucdavis.edu/
Davis CA, 95616
===================================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 11:43:58 2004

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On May 6, 2004, at 9:09 AM, Leona Cohen-Gould wrote:

} One of faculty here will be processing lengths of rat femoral artery
} for light microscopy and needs to keep track of the distal vs proximal
} ends. She tried marking one end with India Ink, but it was washed out
} sometime during the dehydration/xylene steps.
} Any ideas?
}
Dear Lee,
Could one end be cut straight across and the other cut at an angle? I
don't know how readily this could be done or whether it would be easy
to distinguish the ends, but if one cannot determine the shape of the
end, I'd wonder whether other morphology would be reliable.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 13:36:27 2004

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Hi Beverly,
We have the same experience as Mike with both lung, brain (and a few
others) and most plant tissues. Before microwaving, we used the
standard protocols (G, followed by Os, etc.) and did all steps in a low
vacuum. You can use an evaporator using only the rough pump (Good idea
to protect where the vials are set so resin doesn't get on evaporator
plate_, if you don't have another vac chamber such as a vacuum oven.
Now that we microwave most of our tissues, we use the cold plate and
vacuum chamber for hard to penetrate tissues on all steps. It is likely
that the alcohols don't need to be done in the MW however it is faster.

NOTE about pulling the vacuum. One needs to WATCH when pumping the
samples. We pump on the samples and wait for the bubbles to rise. Just
before they get too close to the top, we turn off the vacuum, let the
bubbles settle a bit and start again. Eventually no bubbles appear.
This of course is likely more crucial in the resin steps since resin all
over everything is not nice! After the bubbles have subsided and don't
appear in quantity, we let the vial sit in the vacuum chamber under
vacuum but with the pump off, for the desired time of the step.

When using a microwave with a vacuum chamber it is important to note
WHERE the gauge actually is since if it is directly off the pump, then
when it pulls down to 20mmHg that is only at the pump port, not the
chamber, so that must be taken into consideration. We usually use that
approximate vacuum for the vac chamber on the microwave for most
fixations that are done in the microwave. It is hoped, sincerely hoped,
that eventually the manufacturers will build in a vacuum chamber with a
cold plate in the microwave so it isn't quite so messy to set up.

Good luck,
Judy Murphy

Michael Dunlap wrote:
}
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} Hi Beverly,
}
} I was on a TEM project many years ago working with sheep and chicken
} lungs. Jeff Weidner was the PI on the project. The problem in the
} we had was to get the air out of the lungs before we could any of the
} specimen prep procedures to work well. To many air bubbles and poor
} infiltration.
}
} We ended up use a standard EM procedure with each step done under low vacuum.
}
} Mike
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} } on Wednesday, May 5, 2004 at 15:08:22
} } ---------------------------------------------------------------------------
} }
} } Email: bwareham-at-utah.gov
} } Name: Beverly Wareham
} }
} } Organization: Utah Veterinary Diagnostic Lab
} }
} } Title-Subject: [Microscopy] [Filtered] Fixation of animal lung tissue
} }
} } Question: Hi all,
} } Does anyone have a protocol for fixing animal lung tissue (sheep)
} } for EM and is willing to share it? I'd really appreciate it.
} }
} } Thanks,
} } Beverly Wareham
} } Utah Veterinary Diagnostic Laboratory
} } 435-797-1799
} } bwareham-at-utah.gov
} }
} } ---------------------------------------------------------------------------
}
} --
} ===================================================================================
} Michael Dunlap
} office (530) 752-0284
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} Chemical Engineering & Material Science Fax (530) 752-9554
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Hi Leona:

When you use India Ink it needs to be fixed to the tissue's surface you are
labeling with a picric acid solution such as Bouin's fixative.

Make the ink mark with the opposite end of a swab and then switch to the
cotton tipped end of the swab. Dipp into the Bouin's and dab the area
marked with the India Ink. Blot slightly dry with a Kim Wipe and put back
into formalin. It will be permanently fixed in place and can be processed
and embedded in paraffin.

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Thu May 6 14:53:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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May 6, 2004 at 10:14:58
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Email: sbs38-at-email.byu.edu
Name: Briant Stringham

Organization: BYU

Education: Undergraduate College

Location: Provo, Utah, US

Question: I am collecting protocols for viewing HSV-1 through
negative staining, and I was hoping you could send what you feel is
the best protocol for viewing membrane and capsid integrity. Next, I
need to know the best stain and method for viewing empty or full
capsids.
Thank you for your reply

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Hello MSA folks;

We here at the University of New Brunswick have a Jeol JXA-733
Superprobe that has served us faithfully for many years. Sadly we have
had a catastrophic failure of the oil-cooled objective lens/pole piece
assembly, and so require a replacement. If you have working one and
would be willing to part with it, please contact us.

Thanks for your time,

Steven Cogswell, P.Eng.
UNB Microscopy and Microanalysis Facility
Fredericton, New Brunswick Canada
Phone (506) 453-4887

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You could try OsO4. Its guaranteed to darken on the
specimen and it won't wash out. The only concern is
how useful that end will be once its been treated with
Osmium. I know Osmium is used to fix fatty specimens
in order to give them more contrast. I would use a 1%
or maybe a 2% solution. It usually takes effect
within a few minutes, so you could maybe dip the
distal or promixal portion in the solution. Good
luck.
Sara Goldston
"Bentley, Karen" {Karen_Jensen-at-URMC.Rochester.edu}
wrote:

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Hi Leona:

When you use India Ink it needs to be fixed to the
tissue's surface you are
labeling with a picric acid solution such as Bouin's
fixative.

Make the ink mark with the opposite end of a swab and
then switch to the
cotton tipped end of the swab. Dipp into the Bouin's
and dab the area
marked with the India Ink. Blot slightly dry with a
Kim Wipe and put back
into formalin. It will be permanently fixed in place
and can be processed
and embedded in paraffin.

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

__________________________________
Do you Yahoo!?
Win a $20,000 Career Makeover at Yahoo! HotJobs
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Hi Listers
I am looking for contact information for American Laser. Are they
still out there? How can I contact them?
Thanx
David

____________________

David Elliott Ph.D.

Yale University School of Medicine
Campus Address: TAC S160
333 Cedar Street
PO Box 208022
New Haven, CT 06520-8022

Tel: (203) 785-7572
Fax: (203) 785-6815

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Dear listers

I recently received the parts to a Zeiss Axiotron microscope, which
is no longer supported by the manufacturer. Does anyone have a
manual or schematics for this unit--I hate to waste the box of very
high quality lenses that came with it, and our engineering department
is very interested in getting the unit assembled and working.

Anyone that can help me out with this, please contact me.

thanks in advance

Steve Barlow
--
Dr. Steven Barlow
EM Facility/Biology Dept.
San Diego State University
5500 Campanile Drive
San Diego CA 92182-4614
phone: (619) 594-4523
fax: (619) 594-5676
email: sbarlow-at-sunstroke.sdsu.edu
http://www.sci.sdsu.edu/emfacility

Chairman, Educational Outreach subcommittee
promoting microscopy instruction and increased access to microscopes
Microscopy Society of America
http://www.msa.microscopy.com/

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I'm hoping the microscopy community can help me. I had planned on taking a
course on imaging analysis and photomicrography at McCrone Research but it
was canceled (I was the only student.)

I have a real need to improve my imaging and image measurement skill. I
wish to do particle sizing on images captured via the SEM/TEM/light
microscope.

Does anyone know of short courses and such for the tyro? I would like take
one as soon as possible.

Thanks in advance!!!

Frank Karl
330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Fri May 7 18:15:57 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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7, 2004 at 10:04:31
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Email: e.gagnepain-at-wanadoo.fr
Name: Gagnepain

Organization: ULP of Strasbourg

Education: Graduate College

Location: Strasbourg, France

Question: I have some samples of iron-aluminide (FeAL)and the
thickness is 2 millimeter. How to prepare thin layer of FeAl for an
observation with TEM (Transmission Electron Microscope) without
introduce defaults?

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Below is the result of your feedback form
(NJZFM-ultra-55). It was submitted by
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on Friday, May 7, 2004 at 14:09:42
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Email: cryanez-at-criba.edu.ar
Name: Julia YaŇez

Organization: CONICET

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I need to stain a polymer sample with
RuO4, by oxidation of RuCl3 with
sodium hypochlorite.
I donĄt know the appropiate reactives concentrations.
Could you help me about this procedure?.
Thanks in advance

Julia Y·Ňez

Ing. MarĚa Julia Y·Ňez TE: 54-291-486-1666 int.: 362
Lab.Microscopia ElectrŰnica FAX: 54-291-486-1527
CRIBABB e-mail: cryanez-at-criba.edu.ar
Camino La Carrindanga Km 7
(8000) BahĚa Blanca

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I have never prepared specimens from this material, so I'm not
familiar with its properties.

Is it electrically conductive?

If so, to begin with I would spark errode with a trepanning tool to
get 3 mm dia. discs. Then mechanically grind and polish, preferably
with a dimple grinder, to ~100 um. Finally, electropolish, preferably
with a jet polisher.

Hirsch, Howie, Nicholson, Pashley and Whelan suggest, for Fe-Al
alloys acetic acid (133 cm3), water (7 cm3), chromic acid (25 g) with
a stainless steel cathode and rinses in acetic acid/methanol. Make
sure it remains cool ( {30 C). Voltage in the 25 V to 30 V range.

Possible problems:

1. Different phases may thin at different rates during
electropolishing - you'll need to change the polishing solution.

2. If it is very soft, the mechanical grinding and polishing may
create a deep damage layer - stop mechanical polishing sooner and use
electropolish earlier.

3. If there is stress in the material, thinning may cause a release
of stress and damage.

4. Safety officers

If you can't get electropolishing to work, ion milling should.
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail
will automatically be deleted.
:-)
PS - I'm an employee of JEOL UK.

From MicroscopyL-request-at-ns.microscopy.com Sat May 8 06:25:30 2004

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This humble amateur histologist always used "alcoholic Bouin"
("Duboscq-Brazil Fluid") combined with gentle vacuum applied the way
Judy Murphy describes it, to fix small pieces of rabbit lung...

Try google with "alcoholic bouin" as the search string.

"alcoholic Bouin" (aka:"Duboscq-Brazil Fluid")

Stock Alcoholic Bouin's Solution:
80% ETOH 750.0 ml
formaldehyde 300.0 ml
Picric acid 5.0 gm

Mix solution well, stable 1 year.

Working Solution:
Stock solution 70.0 ml 14.0 ml
Acetic acid 5.0 ml 1.0ml
Add the acetic acid right before use.

Y.

-----Original Message-----
} From: Judy Murphy [mailto:jmurphy-at-deltacollege.org]
Sent: donderdag 6 mei 2004 20:22
To: Michael Dunlap
Cc: Microscopy-at-msa.microscopy.com; bwareham-at-utah.gov

briant

the question really is what is the source of specimen? are you looking
for clinical isolates or at culture material. if culture material, has
it been purified in any way. these things may all affect the
preparation and ultimate quality.

the first issue you have to address is grids. you will need grids with
some form of plastic film, be it collodion, formvar or parlodian. if
you are not set up to make grids, they can be obtained from most EM
supply houses. for short term situations, if you are not going to need
a lot of grids and have no one trained in their preparation, buying them
will be best for your use. you may also wish to carbon coat the grids
to stabilize the film. again, carbon coated plastic coated grids may be
purchased. if cost is a problem, i could probably manage to liberate
50-100 grids.

carbon coated grids introduce several problems, mainly due to the fact
that they are quite hydrophobic. however, they do become more
hydrophilic over time. also, you can treat the grids by glow discharge
(within 2-3 weeks of use) or treat them with alcian blue. usually
clinical material has so much serum or fecal protein present that if you
leave the sample on the grid for several minutes you overcome all
problems of hydrophobicity. we view 2500-3000 clinical samples, and
over 4000 total negative stain preparations/ year. at the risk of being
labeled a reprobate and cretin, we usually do not carbon stabilize the
grids used to examine most samples. the added stability is not enough
benefit for clinical material. if it is a sample of importance we may
use carbon coated grids. if so, we use alcian blue, or old grids.
either way, with our concentration methods, hydrophobicity is not a
problem.

you may wish to consider pretreatment of the sample to stabilize the
virion. we either add glutaraldehyde to a concentration of 0.1%, or
formaldehyde to a concentration of 1-2%. this allows us to neutralize
infectivity, maintain antigenicity and reactivity for IEM, and
stabilizes structure against stresses which may arise during
preparation. the samples need to be vortexed very well immediately to
limit clumping which may be associated with fixative mediated
crosslinking of virions. because of the shorter chain size and mono
aldehyde nature, some argue that formaldehyde is less likely to result
in crosslinking, and is better than glutaraldehyde. personally, we have
never seen any difference between the two.

you do not mention mounting the sample on the grid. i assume you have
some method of preference. if not, please ask, we all have our
favourite methods and are more than willing to tell you them.

as far as staining, most viral electron microscopists have their own
preferences. that does not make any one method 'best', however. we use
several stains routinely, and do a panel 14 different negative stains
whenever we start a new project to confirm the best set of conditions.
that said, the two major staining methods use tungsten or uranyl salts.

the most common tungsten salt is 1.5 to 2% phosphotungstic acid (PTA).
to eqalize the different methods, i have adjusted the concentrations of
stains in my labs to maintain an equal amount of heavy metal atoms
available in the staining solution. therefore, we use 2.5mM PTA. this
works out to be approximately 1.6%. the pH is adjusted to 7.0. the
best method for adjusting pH with this stain is with NaOH. early
studies by Horne and his associates implicated the loss of membrane
integrity with pH adjustment by KOH. if you were working with paramyxo
or myxo, and wanted to release the nucleocapsid, this would be a good
method. for the greater part you do not wish to disrupt the membranes.
with most herpes preparations, you will already see a lot of naked
complete and empty nucleocapsids as it is. we also add 25 micrograms/ml
bacitracin as a surfactant. this helps with stain spreadability and
penetration. other small molecules are available for use. the most
common is probably BSA. again, the addition of fixative will also
stabilize the virions against loss of membranes due to stain
characteristics.

we use two different versions of uranyl stains, uranyl acetate(UA) and
uranyl sulfate (US). both of these must be used at low pH. in fact, if
you try to adjust the pH to around 4.0 you start to get problems keeping
material in solution - especially if your pH meter is not as accurate as
you think. as a rule, we use the material at pH of about 3.5. again,
most protocols call for 2% solutions. adjusting to molar concentrations
and maintaining equivalent heavy metal atoms, we use a 60mM solution.
this represents a 2.5% UA or 2.2% US stain. if you must work with
higher pH, it has been suggested that 1% UA can be adjusted to pH values
as high as 7.0 by the addition of 0.1% ammonium acetate and 0.5% EDTA
(disodium salt). i have not tried this, so i do not know how well it
works. rumour is that it is quite grainy and sublimates badly.

each stain system has its own properties. many feel particles degrade
in PTA but not in UA. PTA has a higher anhydrous density, so you see
more contrast, which could be bad or good. UA tends to be more granular
when imaging, while PTA is low granularity. here the issue is purely
what you think would 'look best'. UA/US tends to sublimate in the beam,
leading to a perceived column contamination problem, while PTA is very
stable, leading some to argue that the column is less contaminated by
vaporizing stain.

the best suggestion - try both PTA and a uranyl stain. i would also
refer you to a recent review: Hazelton, P.R. and Gelderblom, H.R. (2003)
The use of the electron microscope for rapid diagnosis of viral agents
in emergent situations. Emerging Infectious Diseases 9:294-303. it will
give some additional methods and general information. yes, i'm human,
it is one of my articles, but i think it's good, anyway.

hope these thoughts help. let me know if you want specific protocols.
we have them all in electronic file format, albeit WordPerfect files, so
they can be sent easily.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

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From MicroscopyL-request-at-ns.microscopy.com Mon May 10 00:27:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (hunny_pot-at-optusnet.com.au) from http://www.msa.microscopy.com/Ask-A-Microscopist.html on Sunday, May 9, 2004 at 21:45:15
---------------------------------------------------------------------------

Email: hunny_pot-at-optusnet.com.au
Name: Linda

Organization: The University of Sydney

Education: Undergraduate College

Location: Australia

Question: Hello:

I am doing research paper on quanification of shrinkage due to fixation. There are some questions that I like answers to:

1. what are some of the methods used to measure shrinkage?

2. how the effects of foxation can be differentiated from other possible sources of shrinkage?

3. the practices and clincal signifance of quantifying shrinkage due to fixation.

I have been looking around, but I can't find my answers. Could you please help me? Thanks

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Hi

We are looking for a second hand Gatan 666 PEELS, to fit on VG HB5 STEM.
Perheps are there somme which are sleeping in cupboards ! It doesn't
matter if modifications are necessary. Preferently, for administrative
raions, we would prefer a europeen source, but all propositions are
welcome.

Answer directly to my collegue, at
Daniel.Spor-at-ipcms.u-strasbg.fr

Many Thanks.

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 08:04:46 2004

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Hi

What type of silver charged epoxy will be used to make embedding of powder
as standards for EDS microanalysis. If one looks at Epotek's catalog,
there are so much type of epoxys, with very different properties, shelf
live and price. So what is the best compromise. If someone has an advice.

Many thanks

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 08:53:24 2004

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Hi Linda:

A great deal of research was done on these questions in the late
1940's-1960's and you won't find it on the internet. For starters, get a
hold of "Principles of Biological Microtechnique" by John R. Baker,
published in 1958. He discusses various fixatives, their penetration
rates, how they do or do not promote shrinkage (in the fix or in
subsequent processing), etc. I will try to dig up some references to
specific papers later today.

Geoff

by way of Ask-A-Microscopist wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 09:43:36 2004

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"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Julia,

Prepare only the amount of stain that you will use at that moment. For 1
ml of RuO4 stain, use 0.02 g RuCl(subscript: 3 )(superscript: .) nH
(subscript: 2)O [14898-67-0] and 1 ml of NaOCl [7681-52-9].

I recommend that you purchase fresh hypochlorite every few months since the
concentration of hypochlorite in solution does diminish with time. I
discourage using bleach for the same reason, i.e. one is never sure how
long the bottle of bleach has been on the shelf. Keep the RuCl(subscript:
3) hydrate in a nitrogen desiccator when not in use.

The original reference on the use of the in-situ preparation of RuO4 is:
-- Montezinos, D., Well, B.G. and Burns, J.L., J. Polymer Sci.: Polym.
Lett. Ed., 1985, 23, 421.

Another important reference pertains to vapor-staining with RuO4 (using
RuO4 crystals, which are very difficult to find):
-- Sano, H., Usame, T. and Nakagawa, H., Polymer, 1986 27, 1497.

I hybridized the methods of Sano and Montezinos, i.e. using vapor staining
above the in-situ preparation of RuO4, and invariably get outstanding
results:
-- Brown, G. M. and Butler, J. H., Polymer, 1997, 38 (15), 3937.

Although the Montezinos and Sano papers are key, their practicality is
limited. Montezinos recommends staining in the solution using precursors
that are dirt cheap and readily available. Sano convinced me, however,
that solution staining is not a good practice because it produces severe
and uncontrolled oxidation of the outer surface of the sample. Sano's
vapor-staining method is beautiful but the solid RuO4 crystals he uses are
virtually impossible to find in the United States and are very expensive.
I simply combined the two methods and worked out staining durations. Refer
to the appendix of my paper for details including safe use, handling and
disposal as well as sample preparation from beginning to end and staining
durations for some polymer systems.

Happy staining,

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

cryanez-at-criba.edu.ar
(by way of To: microscopy-at-ns.microscopy.com
MicroscopyListserver) cc:
Subject: [Microscopy] viaWWW: stain a polymer

05/07/04 06:38 PM

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Email: cryanez-at-criba.edu.ar
Name: Julia YaŇez

Organization: CONICET

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I need to stain a polymer sample with
RuO4, by oxidation of RuCl3 with
sodium hypochlorite.
I donĄt know the appropiate reactives concentrations.
Could you help me about this procedure?.
Thanks in advance

Julia Y·Ňez

Ing. MarĚa Julia Y·Ňez TE: 54-291-486-1666 int.: 362
Lab.Microscopia ElectrŰnica FAX: 54-291-486-1527
CRIBABB e-mail: cryanez-at-criba.edu.ar
Camino La Carrindanga Km 7
(8000) BahĚa Blanca

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From MicroscopyL-request-at-ns.microscopy.com Mon May 10 09:45:04 2004

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You may be interested in a paper I published a few years ago in which
I measured the size distribution of cells in suspension after
different fixation conditions. Develop. Biol 23:36-61 (1970)

Joel

}
}
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} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (hunny_pot-at-optusnet.com.au) from
} http://www.msa.microscopy.com/Ask-A-Microscopist.html on Sunday, May
} 9, 2004 at 21:45:15
} ----------------------------------------------------------------------
} -----
}
} Email: hunny_pot-at-optusnet.com.au
} Name: Linda
}
} Organization: The University of Sydney
}
} Education: Undergraduate College
}
} Location: Australia
}
} Question: Hello:
}
} I am doing research paper on quanification of shrinkage due to
} fixation. There are some questions that I like answers to:
}
} 1. what are some of the methods used to measure shrinkage?
}
} 2. how the effects of foxation can be differentiated from other
} possible sources of shrinkage?
}
} 3. the practices and clincal signifance of quantifying shrinkage due
} to fixation.
}
} I have been looking around, but I can't find my answers. Could you
} please help me? Thanks
}
} ----------------------------------------------------------------------
} -----
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 09:49:51 2004

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Jacques;

What is the material of interest? You need to say. Obviously it can't be silver but you may want to check to see if you have silver spectrally overlapping the material or element of interest. Is your concern primarily sample charging therefore you want a conductive epoxy?

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: Faerber Jacques [mailto:Jacques.Faerber-at-ipcms.u-strasbg.fr]
Sent: Monday, May 10, 2004 9:09 AM
To: Microscopy Society of America

Hi

What type of silver charged epoxy will be used to make embedding of powder
as standards for EDS microanalysis. If one looks at Epotek's catalog,
there are so much type of epoxys, with very different properties, shelf
live and price. So what is the best compromise. If someone has an advice.

Many thanks

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:06:37 2004

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"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Jacques,

I spent a considerable amount of time working on conductive embedding
media. See my abstract in the 2004 M&M Proceedings.

The problem with virtually all commercial electrically conductive embedding
media that I have seen is that they offer only macroscopic conductivity.
This means that expanses of unfilled, non-conducting and highly charging
epoxy will be found throughout the sample. We need microscopic
conductivity in which the embedding medium is highly conductive and does
not contain non-conductive domains of epoxy. For expoxy-embedding
applications, I recommend compounding (mixing) carbon black filler into the
resin of choice (without catalyst or accelerator) in a mortar and pestle.
Use equal parts by weight of the filler powder and epoxy. At the last
minute before embedding, mix the accelerator into the resin / carbon black
compound as quickly and thoroughly as possible. Embed the sample in this
thick paste.

If well mixed, the embedding medium will not charge at all. Also, since
only carbon and oxygen are present in any appreciable concentration, you
will not have problems with interference lines from metal filler particles,
i.e. silver, etc.

Have fun.

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

Faerber Jacques
{Jacques.Faerber-at-ipcms.u- To: Microscopy Society of America {Microscopy-at-MSA.Microscopy.Com}
strasbg.fr} cc:
Subject: [Microscopy] EDS standards embedding

05/10/04 08:08 AM

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Hi

What type of silver charged epoxy will be used to make embedding of powder
as standards for EDS microanalysis. If one looks at Epotek's catalog,
there are so much type of epoxys, with very different properties, shelf
live and price. So what is the best compromise. If someone has an advice.

Many thanks

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:12:59 2004

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Our standards from Tsousimis came prepared with regular epoxy and a coating
of carbon. We have used the same procedure for our homemade standards. Many
of the standard materials are not conductive anyway, so the conductivity
has to come from a coating. Of course a "conductive" epoxy should not hurt.

I presume you will be not be collecting spectra in variable pressure mode.
The scattering of the beam from the residual atmosphere would produce a
signal from the silver or nickel in your epoxy and would complicate things.

I also advise you to prepare the sample and standards the same. I thought I
was competent at EDS standards and realized fairly recently the difference
that can be caused by different thickness of C coatings (or lack thereof)
between standards and unknowns.

Warren Straszheim

At 08:08 AM 5/10/2004, you wrote:

} Hi
}
} What type of silver charged epoxy will be used to make embedding of powder
} as standards for EDS microanalysis. If one looks at Epotek's catalog,
} there are so much type of epoxys, with very different properties, shelf
} live and price. So what is the best compromise. If someone has an advice.
}
} Many thanks
}
} J. Faerber
} IPCMS-GSI
} (Institut de Physique et Chimie des Matériaux de Strasbourg
} Groupe Surface et Interfaces)
} 23, rue de Loess ; BP43
} 67034 Strasbourg CEDEX 2
} France
}
} Tel 00 33(0)3 88 10 71 01
} Fax 00 33(0)3 88 10 72 48
} E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:28:32 2004

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I want to find a simple TEM protocol for negative staining of microsomal
preparations. Does anyone have suggestions?

Thank you,
Cheri Owen
Cheri Owen, PhD
Dept. Emergency Medicine
Wayne State University
Detroit, Mi 48201

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:56:54 2004

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Ooh, one more question:

The Philips EM400 installations I know of all utilized a Haskris
chiller. We're looking to buy a new chiller and they are considerably
cheaper from Neslab. Would anyone recommend against going with Neslab
for any reason?

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 10:56:54 2004

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Hi folks,

Does anyone know of an archived discussion or a web site anywhere that
describes adapting a C-mount for a digital camera to the old Philips
EM400 TEM? Perhaps by custom machining a cover blank for the 35mm
camera mounting location?

We recently purchased a Pax-it 2.1 Mpixel digital camera to use with a
new inverted metallurgical LM, but after receiving the camera, funding
for the microscope didn't materialize, so we're thinking of using the
Pax-it on our EM400.

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 13:52:13 2004

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Eric -

The only thing I don't particularly care for in our (?8-year-old)
Neslab chiller is the fact that the water reservoir is pretty well sealed
up, like a miniature 45-gallon drum on its side, so you can't see what's
going on in there. The Haskris chillers always used to have a water tank
with a lid, making for much easier service and monitoring of water
condition. Other than that, both types are pretty well just pumps directly
driven by electric motors with some miscellaneous tubing and controls. Both
brands used to use the same pumps (made by Procon of Tennessee), and
probably still do.
Our Neslab has been pretty trouble-free; it's gone through one motor
so far and at least two pumps, but, as they say, your mileage may vary.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Eric Anderson [mailto:andersone1-at-southernct.edu]
Sent: Monday, May 10, 2004 1:03 PM
To: MSA listserver

Ooh, one more question:

The Philips EM400 installations I know of all utilized a Haskris
chiller. We're looking to buy a new chiller and they are considerably
cheaper from Neslab. Would anyone recommend against going with Neslab
for any reason?

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 15:32:29 2004

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We have been using a Neslab chiller since the beginning of time (I can't
find the original records). It runs without much complaint, most of the
time. We have replaced the motor (just an electric motor available from
Grainger's) once, replaced the pump once, and had the old pump rebuilt by
Procon once. We have replaced the shear pin ("nylon coupling")in the pump
head a number of times (maybe as much as once a year), and recharged the
compressor once in the last 6 years.

I've heard that the Haskris is a "better" chiller...but the Neslab seems to
do the job just fine. Their service support--by phone--is wonderful, and
they're in southern NH if you need to send something to them.

I highly recommend having a supply of shear pins available, and definitely
have them teach you how to change them if you never have done this
before--it's a little tricky the first time.

No interest in Neslab other than long experience as a user...

Deborah H. Gaynor, Ph.D.
Scanning Electron Microscopist
Analytical Services, Inc.
PO Box 515
Williston, VT 05495
802-878-5138 x21

-----Original Message-----
} From: Thomas, Frank [mailto:FThomas-at-nrcan.gc.ca]
Sent: Monday, May 10, 2004 2:58 PM
To: 'Eric Anderson'; MSA listserver

Eric -

The only thing I don't particularly care for in our (?8-year-old)
Neslab chiller is the fact that the water reservoir is pretty well sealed
up, like a miniature 45-gallon drum on its side, so you can't see what's
going on in there. The Haskris chillers always used to have a water tank
with a lid, making for much easier service and monitoring of water
condition. Other than that, both types are pretty well just pumps directly
driven by electric motors with some miscellaneous tubing and controls. Both
brands used to use the same pumps (made by Procon of Tennessee), and
probably still do.
Our Neslab has been pretty trouble-free; it's gone through one motor
so far and at least two pumps, but, as they say, your mileage may vary.

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Eric Anderson [mailto:andersone1-at-southernct.edu]
Sent: Monday, May 10, 2004 1:03 PM
To: MSA listserver

Ooh, one more question:

The Philips EM400 installations I know of all utilized a Haskris
chiller. We're looking to buy a new chiller and they are considerably
cheaper from Neslab. Would anyone recommend against going with Neslab
for any reason?

Many thanks for any tips!
Best to all,
Eric Anderson
SCSU Physics Department
501 Crescent Street
New Haven, CT 06515
203-392-6468

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 17:03:35 2004

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Has anyone tried any of the anti-GFP antibodies on the market for
western blotting? Many seem to be cheaper than Clontech for the same
amount but we don't want to buy an untested antibody. Thanks- Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 18:18:11 2004

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What are you trying to look at with your EDS?
What kind of EDS is it?

The "normal" calibration of EDS is done at Al
K alpha (1.486KeV) and Cu K alpha (8.040KeV).
This sets resolution of the EDS according to these
two peaks. The other checks I do are done at C, O and F
and at N & O. And finally, FWMH at Mn.

For these measurements, I use X-Checker and X-Checker Extra.
For C, O and F, I use an Al stub with a Carbon sticky tab
with Teflon tape about 50% covering the stub and the other
50% split between sticky tab and bare Aluminum pin stub.
These readings do not calibrate the system. They produce
resolution figures for ability to resolve light elements.
You can do similar analysis for heavier elements with other
stub configurations.

The rationale for light element work is to see if the
EDS system, over time, drifts in the wrong direction.
Then I would know that something is going bad, either window
problems or EDS system problems. You will see this right
away at low Z.

If you are looking for ISO standards, I'm not sure how
that would work. Cu is Cu and Al is Al. The Cu and Al
peaks are used. If any foreign material was present, it
is simply ignored. The EDAX calibration routine only looks
at the Al and Cu peaks.

gary g.

At 06:08 AM 5/10/2004, you wrote:

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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon May 10 18:27:40 2004

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I have been running my Haskris, on my EM410, virtually continuously,
since November 1982. I have replaced no parts. I have another Haskris
on my 1999 Hitachi S3500-N that has an intermittent algae problem, and
has also needed the starter capacitor on the motor replaced.

Rick A. Harris, exDirector
Microscopy and Imaging Facility
Section of Molecular and Cellular Biology
1241 Life Sciences Addition
University of California
Davis, CA
530 752 2914
http://microscopy.mcb.ucdavis.edu
raharris-at-ucdavis.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 11 02:06:04 2004

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Some precisions, as Peter has asked :

The question comes for a job on thin film of materials such Sr2TiMoO4 and
CoFe2O4 grown by laser ablation. The goal is to control the stochioametric
variation from the films, in comparaison with the target material, which
we have as a powder, or as sintered target. So I need to embed the powder,
or pieces of the sintered bulk, to make a polished surface of
it. I reed in a paper from Geller in the NIST bull. mentionned by someone
on the list about the use of silver charged epoxy. As I use some by the
way for fixing sample for spark machining, I was in question about what
kind could do the job for my standards.

As I have understand the electrical conductivity in such materials will be
done by tunneling effect between the silver grain, through the epoxy. So
it is not so macroscopic. I'll try the methode with carbon black. Seems to
be interesting and much cheaper than all the commercial silver epoxys. And
with carbon, the problem of siver L lignes signal will be avoid.

These standards are used as references for thin films analysis, using
Stratagem thin film software.

Some other suggestions ?
Many thanks.

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

On Mon, 10 May 2004, Tomic, Peter (Peter) wrote:

}
}
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} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
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} -------------------------------------------------------------------------------
}
} Jacques;
}
} What is the material of interest? You need to say. Obviously it can't be silver but you may want to check to see if you have silver spectrally overlapping the material or element of interest. Is your concern primarily sample charging therefore you want a conductive epoxy?
}
} Regards,
}
} Peter Tomic
} Agere Systems
}
} -----Original Message-----
} } From: Faerber Jacques [mailto:Jacques.Faerber-at-ipcms.u-strasbg.fr]
} Sent: Monday, May 10, 2004 9:09 AM
} To: Microscopy Society of America
} Subject: [Microscopy] EDS standards embedding
}
}
}
}
} ------------------------------------------------------------------------------
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} -------------------------------------------------------------------------------
}
}
} Hi
}
} What type of silver charged epoxy will be used to make embedding of powder
} as standards for EDS microanalysis. If one looks at Epotek's catalog,
} there are so much type of epoxys, with very different properties, shelf
} live and price. So what is the best compromise. If someone has an advice.
}
} Many thanks
}
} J. Faerber
} IPCMS-GSI
} (Institut de Physique et Chimie des Matériaux de Strasbourg
} Groupe Surface et Interfaces)
} 23, rue de Loess ; BP43
} 67034 Strasbourg CEDEX 2
} France
}
} Tel 00 33(0)3 88 10 71 01
} Fax 00 33(0)3 88 10 72 48
} E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 11 03:24:48 2004

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Rick

this may be drifting off topic a bit, but we used to have algae problems with our water cooler until I covered the translucent plastic hose with aluminium foil. There doesn't seem to have been a problem for over a year and there is little need to clean out the system these days.

I know that you can get black pressure hoses as an alternative but you can't buy them from your local supermarket for ~ 1 UK pound and fit them in a few minutes while the system is running.

Malcolm

Malcolm Haswell
e.m. unit
University of Sunderland
UK

e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: "Rick A. Harris" {raharris-at-ucdavis.edu}

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mivalmar-at-yahoo.es) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 11, 2004 at 15:10:15
---------------------------------------------------------------------------

Email: mivalmar-at-yahoo.es
Name: Miguel V.Serrano

Organization: C.Haya Hospital

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I want to ask if someone has tryed to do an immunohistochemistry of PPAR alpha (peroxisome proliferator receptor alpha) in rat liver or another tissue ??. Thanks.

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From MicroscopyL-request-at-ns.microscopy.com Tue May 11 15:21:51 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donovanl-at-ufl.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 11, 2004 at 12:50:14
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Email: donovanl-at-ufl.edu
Name: Laura Donovan

Organization: University of Florida College of Veterinary Medicine

Title-Subject: [Microscopy] [Filtered] MListserver:Nikon Labophot 1x objective

Question: I am looking for a 1x objective for a Nikon Labophot, and having a difficult time.
Lab phone: (352)392-4700 ext. 3845
ask for Rose or Laura.

Thank you.

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I'm sorry that this is a bit of a deviation, but, knowing how diverse this list is, somebody
may be able to help:-

I have a Stanton-Redcroft Thermal Analyser, an STA-1600, the company in its last
years was acquired by Polymer Laboratories and then by Rheometrics, and I'm
interested in exploring the possibility of hooking analytical instruments, maybe NDIR or
even mass-spec, to the gas outlet line, to analyse the evolved gases (what was referred
to some time ago, so nicely, by Stanton-Redcroft as "hyphenated techniques").

Does anyone have such a setup?

Presumably one would use a heated PTFE interface tube, but the furnace internal
volume is fairly large, and not necessarily efficiently swept by the 50 ml/min or so of
purge gas, and what I'm wondering about is the time resolution of such EGA in this
instrument.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 04:52:33 2004

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Gary writes ...

} The "normal" calibration of EDS is done at Al
} K alpha (1.486KeV) and Cu K alpha (8.040KeV).
} ...

Out of curiosty, why would a calibration use these
2 peaks rather than CuK and CuL?? Understandably,
the L-line would be a convolution of the L-family,
but I would think the Al K line is in a more difficult
location relative to the slope in the continuum(???)
Is there any preference with respect to EDX window
type? (e.g., Be v UTW)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 05:04:38 2004

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Dear colleagues

We are looking for the RIGHT answers.
Addressing different institutions across the globe appear to be a very difficult.
We have been sent into circles for months without one clear cut answer.

Our EM technician has a HND in Environmental Science. He has been in the EM Unit for just over
a year and is slowly getting the hang of things. We would like to promote him up the ranks.
He has got the right aptitude, has matured and is responsible. Nice to find people like that still.

For him to be promotable, the University require at least a first degree (Senior Technician)
and Masters (Chief Technician). Without going through the rest of the gory details, he need further study. It is the policy of the University of Botswana to send citizens abroad rather than to study locally to enrich the nation academically.

The ranking of preference is 1) South Africa, 2) Australia, 3) USA, 4) UK.

He would prefer to do a EM focused masters. If he can do a pure Electron Microscopy Masters through course and lab work the better. The preference will be in the field of Material Science if he can not do a masters in "electron microscopy".

1) For him to be send by the University for a first degree and a masters consecutively, he must find at least partial sponsorship/bursary.
2) Who must he contact. (Please one name only in your institution, not a string of people!)
3) Can he get Credit for his current qualification?
4) Academic year start, requirements, and duration of study.

We are keeping our fingers crossed.
Thanks

Since my UB mail address is not reliable please send
a copy of all urgent mail to coetzeesh-at-yahoo.co.uk

Mr S. H. Coetzee
Electron Microscope Unit
University of Botswana
Private Bag 0022
Gaborone
Botswana

Phone : +267 355 2462/5222
Mobile : +267 714 55701 (Now active)
Fax : +267 318 5097
e-mail : coetzees-at-mopipi.ub.bw

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 06:52:59 2004

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Hello Ritchie,

FWIW, we have a Leybold quadrapole RGA which we often connect to our vacuum
furnace to monitor evolved gasses. Since the RGA operates at much higher
vacuum than the furnace, the interface is made using conflat flanged s-steel
fittings and a quality leak valve.

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Wednesday, May 12, 2004 1:45 AM
To: Microscopy-at-sparc5.microscopy.com

I'm sorry that this is a bit of a deviation, but, knowing how diverse this
list is, somebody
may be able to help:-

I have a Stanton-Redcroft Thermal Analyser, an STA-1600, the company in its
last
years was acquired by Polymer Laboratories and then by Rheometrics, and I'm
interested in exploring the possibility of hooking analytical instruments,
maybe NDIR or
even mass-spec, to the gas outlet line, to analyse the evolved gases (what
was referred
to some time ago, so nicely, by Stanton-Redcroft as "hyphenated
techniques").

Does anyone have such a setup?

Presumably one would use a heated PTFE interface tube, but the furnace
internal
volume is fairly large, and not necessarily efficiently swept by the 50
ml/min or so of
purge gas, and what I'm wondering about is the time resolution of such EGA
in this
instrument.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext
87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 07:42:46 2004

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shAf,
I've thought that for a long time but have yet to find a software-based
calibration that can use the 2 Cu peaks. Maybe the vendors can speak to
this.

As to Gary's question of why one needs standards, I have a hunch
they're not looking for EDS calibration standards (a piece of Cu tape on
an Al stub works just fine) but quantitative analysis standards for high
quality quant work. Despite the software advances in standardless
analysis, everyone I've talked to who really knows x-ray says that
standardless quant just doesn't have the accuracy or precision of
standards-based analysis.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

michael shaffer wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 08:48:21 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sp-bf-at-physik.upb.de) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 12, 2004 at 05:24:26
---------------------------------------------------------------------------

Email: sp-bf-at-physik.upb.de
Name: Bettina Friedel

Organization: University of Paderborn

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi all!

Our physics group got a Hitachi H-600 a few years ago from biology group. We repaired it and there was no problem. But now the wire from the linkage of the specimen chamber has broken. It jumped out from the guide rolls and now we cannot move the specimen in one direction. "Nissei Sanyo Europe",the Hitachi Service Center here, demands 3500Ä for repair of this silly wire.
I hope anyone can help me!!! Is there a plan (blueprint?) how to thread the wire through the rolls, so that we could repair it ourself, not perfect but in this way, that moving of the specimen would be possible?

Bettina Friedel

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 09:33:30 2004

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I am trying to label the GFP in yeast on either Lowicryl sections or Tokuyashu cryosections. So far, we have had rather poor labeling/high background. I would appreciate any recommendations on a particular commercially available antibody and the fixation protocol.

Also, we would need to label a biotin-tagged protein. We were trying Streptavidin - gold, but to little success. Is there a good anti-biotin antibody (or, even better, anti-biotin/gold conjugate) people have used
for this purpose before?

Any recommendations would be highly appreciated.

Michael Jarnik,
EM Facility
Fox Chase Cancer Center
Philadelphia, PA

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 10:50:57 2004

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Just guessing, but I would suppose the energy calibration is a rather
simplistic algorithm. I am pretty sure that is much easier to work with a
symmetric K peak and pick off the centroid than it is to deconvolute the L
peaks to find the energy of the alpha line.

Presumably the effect of the background slope and curvature is negligible
compared to the peak intensity if all they have to do is get a peak energy.

Warren

At 04:57 AM 5/12/2004, "michael shaffer" wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 12:36:06 2004

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michael

i', sorry, but your second question is not clear to me. are you simply
trying to label your protein with gold, or is this a detection step
where you have already used the antibody to react with its antigen and
now want to see if where the antigen is? also, do you have any antibody
which is not tagged with biotin and that you could use for tagging with
either nanogold or directly onto larger gold labels? finally, could you
do an indirect reaction using gold tagged antibody to the host species
antibody you are using, eg, say the biotin-antibody is an IgG species,
raised in mouse, could you come back with colloidal gold:anti mouse IgG?

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-392

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 12:38:32 2004

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On May 12, 2004, at 2:57 AM, michael shaffer wrote:

} Out of curiosty, why would a calibration use these
} 2 peaks rather than CuK and CuL?? Understandably,
} the L-line would be a convolution of the L-family,
} but I would think the Al K line is in a more difficult
} location relative to the slope in the continuum(???)
} Is there any preference with respect to EDX window
} type? (e.g., Be v UTW)
}
} I've thought that for a long time but have yet to find a
} software-based calibration that can use the 2 Cu peaks. Maybe the
} vendors can speak to this.

Dear Mike and Ken,
Since the Al k-line is at 1.4 keV and the Cu l-line(s) is at ~1 keV,
the Al is more readily separated from the continuum. I don't know of a
difference between Be and UTW calibrations, since it is the response of
the crystal that is being measured, but, perhaps there is an advantage
to using a lower-energy line with the UTW.
The TN2000 had software that could use any two lines. One simply
entered the energies and ran the calibration routine. I guess someone
must have "improved" the system by entering the line energies for us.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 12:54:20 2004

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Sorry, I would try to make it clearer. We need to localize a viral
protein which has been biotin-tagged and expressed in cell culture. I
expected it should be no problem to label it with Streptavidin
conjugate, but it is not that easy, it seems (even according to some
other people). So, as we do not have a good antibody to the viral
protein, I am considering an indirect labeling with anti-biotin
antibody and a secondary conjugate. There are tons of commercially
available anti-biotin antibodies, but certainly not all of them will
work with EM protocols - so I was interested whether somebody has
experience with some of these.

Thanks,

Michael

paul r hazelton wrote:

} michael
}
} i', sorry, but your second question is not clear to me. are you simply
} trying to label your protein with gold, or is this a detection step
} where you have already used the antibody to react with its antigen and
} now want to see if where the antigen is? also, do you have any antibody
} which is not tagged with biotin and that you could use for tagging with
} either nanogold or directly onto larger gold labels? finally, could you
} do an indirect reaction using gold tagged antibody to the host species
} antibody you are using, eg, say the biotin-antibody is an IgG species,
} raised in mouse, could you come back with colloidal gold:anti mouse IgG?
}
} paul
}
} Paul R. Hazelton, PhD
} Electron Microscope Unit
} University of Manitoba
} Department of Medical Microbiology
} 531 Basic Medical Sciences Building
} 730 William Avenue
} Winnipeg, Manitoba, Canada, R3E 0W3
} e-mail: paul_hazelton-at-umanitoba.ca
} Phone:204-789-3313
} Pager:204-931-954
} Cell:204-781-1502
} Fax:204-789-392
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:22:55 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rpowell-at-nanoprobes.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 12, 2004 at 12:22:51
---------------------------------------------------------------------------

Email: rpowell-at-nanoprobes.com
Name: Rick Powell

Organization: Nanoprobes, Incorporated

Title-Subject: [Microscopy] Anti-GFP and anti-biotin Abs for TEM (vendor reply)

Question: Hello Michael:

[Vendor reply...] We (Nanoprobes, Inc,) make an anti-biotin-IgG gold conjugate using our 1.4 nm Nanogold particle; we also offer streptavidin-Nanogold. You don't say why the streptavidin-gold didn't work - if you could let us have some details, we may have some suggestions.

Hope this is useful,

Rick Powell
Nanoprobes, Inc.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:24:42 2004

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In a discussion I had with a service rep for EDAX Inc., the calibration is nothing more than setting the A/D [Analog to digital] converter's scale and offset. It doesn't change anything with respect to the detector itself.

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]
Sent: Wednesday, May 12, 2004 11:57 AM
To: Microscopy-at-msa.microscopy.com

Just guessing, but I would suppose the energy calibration is a rather
simplistic algorithm. I am pretty sure that is much easier to work with a
symmetric K peak and pick off the centroid than it is to deconvolute the L
peaks to find the energy of the alpha line.

Presumably the effect of the background slope and curvature is negligible
compared to the peak intensity if all they have to do is get a peak energy.

Warren

At 04:57 AM 5/12/2004, "michael shaffer" wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:26:36 2004

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Hi Michael,

I've had great results on cryo-sections with a rabbit anti-GFP antibody
from
Molecular Probes: cat# 11122
Works well at dilutions ranging from 1:50-1:200.
Low background.
Hope it works for you.
Best

Marc

On Wednesday, May 12, 2004, at 10:39 AM, Michal Jarnik wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} I am trying to label the GFP in yeast on either Lowicryl sections or
} Tokuyashu cryosections. So far, we have had rather poor labeling/high
} background. I would appreciate any recommendations on a particular
} commercially available antibody and the fixation protocol.
}
} Also, we would need to label a biotin-tagged protein. We were trying
} Streptavidin - gold, but to little success. Is there a good
} anti-biotin antibody (or, even better, anti-biotin/gold conjugate)
} people have used for this purpose before?
} Any recommendations would be highly appreciated.
} Michael Jarnik,
} EM Facility
} Fox Chase Cancer Center
} Philadelphia, PA
}
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 13:32:23 2004

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Fellow Microscopists,

The Microscopy Lab in our Research Center has 3 SEM's, 1 TEM and 1 EMPA
(with a second due in November) in addition to 4 XRD instruments. Our
main function has been as a problem solving facility to our researchers as
well as our field service engineers. Data produced by our lab is usually
issued as reports with images, spectra and graphs as attachments.
Management has directed us to implement a LIMS by the end of the year.
Their requirements include the ability of the researchers and field service
engineers to log samples in from their locations and the tracking of the
sample from the arrival in our lab to the issuance of data. It must also
be able to archive the data as well. For us this means literally hundreds
of images, spectra and reports each month that must be categorized and
saved. The researchers and engineers must also be able to access the data
from their location. This will probably mean a web based system since our
facilities cover the globe.

Has anyone out there been faced with a similar request? Our main hurdle is
convincing management that ours is not a "sample in - number out" type of
lab, and that most LIMS packages out there are designed for that type of
simple operation. If you have implemented such a system, was it an off the
shelf package, a custom designed package or a combination? If you want to
respond to me directly that would be fine. I am not interested in "system
bashing" just some helpful suggestions on how to make management happy
without losing my sanity.

Sharon Goresh
Chemist
sharon.goresh-at-engelhard.com

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 15:04:11 2004

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we like the bethyl labs mouse anti-biotin then follow that with goat
anti-mouse conjugated to gold. it is much better than streptavidin
gold. i am looking for a gfp ab so let me know what works.

At 10:39 AM 5/12/2004 -0400, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 15:26:13 2004

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The Moran Scientific EDS software can use the Cu L and K peaks (or any others the
user chooses) for the peak position calibration. I do this.

It would be a bit more correct not to use L peaks, because, as Shaf said, it's an
unresolved group of lines, so the resolution that gets calculated at the low energy end
isn't quite correct, but unless you're using virtual standards, that doesn't matter.

But hey, even the Al K peak is the Ka1 plus the Ka2 plus the Kb anyway, on an EDS.

cheers

rtch

Date sent: Wed, 12 May 2004 08:48:26 -0400
} From: qualityimages {qualityimages-at-netrax.net}
To: michael shaffer {michael-at-shaffer.net} ,
Microscopy {Microscopy-at-Sparc5.Microscopy.Com}

Dear Michael,
I just checked, and my Quartz XOne system can use any two peaks, including Cu Ka
and Cu La, to calibrate the system. The tradition may be to use Al Ka and Cu La
because those two elements are easy to find in most EM labs and the old
Be-window detectors did not always see Cu La well. Of course, the accuracy of
your calibration will depend on the separation of your peaks and their accurate
location. Ka peaks are sharper than La peaks, so it may improve your calibration
accuracy to use two Ka peaks.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 12, 2004 2:57 AM

Michael,

In response to your question, most, if not all, EDX manufacturers today
including RÖNTEC find it necessary to use only one specified energy line
plus the zero peak. This is because linearity is so high, that a 3-point
calibration (two specified spectral lines + zero peak) for almost all cases
is not beneficial.

Martin Rohde
RÖNTEC GmbH
RÖNTEC USA, Inc.
www.rontec.com

} On May 12, 2004, at 2:57 AM, michael shaffer wrote:

} Out of curiosty, why would a calibration use these
} 2 peaks rather than CuK and CuL?? Understandably,
} the L-line would be a convolution of the L-family,
} but I would think the Al K line is in a more difficult
} location relative to the slope in the continuum(???)
} Is there any preference with respect to EDX window
} type? (e.g., Be v UTW)
} }
} I've thought that for a long time but have yet to find a
} software-based calibration that can use the 2 Cu peaks. Maybe the
} vendors can speak to this.

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 17:04:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Michael,

It's me again.
Actually I have used an anti-biotin that
worked well for immuno-EM.
It's from Rockland, cat # 200-4198.
It's a rabbit antibody, IgG fraction.

I too had problems using streptavidin-gold.
The reason for this, I think, is a lack of stability of
the conjugate. Don't forget that when you purchase
a gold conjugate, it might have sat for months on
a refrigerator shelve and the proteins have either
been degraded or fallen off the gold particles!

In my experience, good sources for antibodies
that work at the EM level are Cappel (bought a
a few years back by ICN - now called MP
Biomedicals), Rockland (to a lesser extent),
and Molecular Probes. I only use protein A
gold for my labelings, and I certainly avoid
gold conjugates from Ted Pella that have not
worked for me even once in the last 5 years!
Good luck

Marc

On Wednesday, May 12, 2004, at 01:59 PM, Michal Jarnik wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Sorry, I would try to make it clearer. We need to localize a viral
} protein which has been biotin-tagged and expressed in cell culture. I
} expected it should be no problem to label it with Streptavidin
} conjugate, but it is not that easy, it seems (even according to some
} other people). So, as we do not have a good antibody to the viral
} protein, I am considering an indirect labeling with anti-biotin
} antibody and a secondary conjugate. There are tons of commercially
} available anti-biotin antibodies, but certainly not all of them will
} work with EM protocols - so I was interested whether somebody has
} experience with some of these.
}
} Thanks,
}
} Michael
}
} paul r hazelton wrote:
}
} } michael
} }
} } i', sorry, but your second question is not clear to me. are you
} } simply
} } trying to label your protein with gold, or is this a detection step
} } where you have already used the antibody to react with its antigen and
} } now want to see if where the antigen is? also, do you have any
} } antibody
} } which is not tagged with biotin and that you could use for tagging
} } with
} } either nanogold or directly onto larger gold labels? finally, could
} } you
} } do an indirect reaction using gold tagged antibody to the host species
} } antibody you are using, eg, say the biotin-antibody is an IgG species,
} } raised in mouse, could you come back with colloidal gold:anti mouse
} } IgG?
} }
} } paul
} }
} } Paul R. Hazelton, PhD
} } Electron Microscope Unit
} } University of Manitoba
} } Department of Medical Microbiology
} } 531 Basic Medical Sciences Building
} } 730 William Avenue
} } Winnipeg, Manitoba, Canada, R3E 0W3
} } e-mail: paul_hazelton-at-umanitoba.ca
} } Phone:204-789-3313
} } Pager:204-931-954
} } Cell:204-781-1502
} } Fax:204-789-392
} }
} }
}
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 17:44:13 2004

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I believe the real object of this is to find two peaks separated far enough in energy to allow the A/D converter to calibrate over a broad range. The broader the less the error. From an electronic point of view, it doesn't matter which peaks are used, just that they have significant separation. The electronics doesn't know the difference. It goes from peak height to a position in energy which corresponds to a voltage which gates a clock. I'm babbling, only electrical engineers worry about these things.

Any EDX vendors care to comment?

Peter

-----Original Message-----
} From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
Sent: Wednesday, May 12, 2004 4:31 PM
To: michael shaffer
Cc: Microscopy

Dear Michael,
I just checked, and my Quartz XOne system can use any two peaks, including Cu Ka
and Cu La, to calibrate the system. The tradition may be to use Al Ka and Cu La
because those two elements are easy to find in most EM labs and the old
Be-window detectors did not always see Cu La well. Of course, the accuracy of
your calibration will depend on the separation of your peaks and their accurate
location. Ka peaks are sharper than La peaks, so it may improve your calibration
accuracy to use two Ka peaks.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 12, 2004 2:57 AM

Dear Peter,
Your age is showing, the electronics are all purely digital, now. No A/D
converter needed. The only reason to use two Ka peaks instead of a Ka and an La
peak are that the Ka peaks are sharper and so the peak centroid is more
precisely located. The software calibration sets the zero point and the
amplifier gain to a fraction of a channel. With the newer, higher-resolution
detectors, more quant precision and lower detection limit is possible, but the
calibration is more critical, since a tiny shift of the peak throws off all the
quant calculations. I find my self calibrating every month where I used to do it
once a year with the old A/D system, but my results are much better.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "Tomic, Peter (Peter)" {ptomic-at-agere.com}
To: "Mary Mager" {mager-at-interchange.ubc.ca} ; "michael shaffer"
{michael-at-shaffer.net}
Cc: "Microscopy" {microscopy-at-MSA.microscopy.com}
Sent: Wednesday, May 12, 2004 3:49 PM

Dear Michael,
I just checked, and my Quartz XOne system can use any two peaks, including Cu Ka
and Cu La, to calibrate the system. The tradition may be to use Al Ka and Cu La
because those two elements are easy to find in most EM labs and the old
Be-window detectors did not always see Cu La well. Of course, the accuracy of
your calibration will depend on the separation of your peaks and their accurate
location. Ka peaks are sharper than La peaks, so it may improve your calibration
accuracy to use two Ka peaks.
Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on occasion.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 12, 2004 2:57 AM

} I find my self calibrating every month where I used to do it once a
} year with the old A/D system, but my results are much better.

Once a month!

Once a year!

I do it once or twice a day.

But that's Virgoans for you. We worry a lot.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 20:07:12 2004

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Hi Bettina,
I have the user's manual for the Hitachi H-600.
I will email you the diagrams.
I remember my boss trying to fix this problem and it almost drove him crazy.

Good luck!

John Brealey
Medical Scientist
Electron Microscopy Unit
The Queen Elizabeth Hospital
IMVS - TQEH Pathology
Woodville, 5011
South Australia
(08) 82226612

Bettina Friedel wrote:

Email: sp-bf-at-physik.upb.de
Name: Bettina Friedel

Organization: University of Paderborn

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi all!

Our physics group got a Hitachi H-600 a few years ago from biology group. We
repaired it and there was no problem. But now the wire from the linkage of
the specimen chamber has broken. It jumped out from the guide rolls and now
we cannot move the specimen in one direction. "Nissei Sanyo Europe",the
Hitachi Service Center here, demands 3500Ä for repair of this silly wire.
I hope anyone can help me!!! Is there a plan (blueprint?) how to thread the
wire through the rolls, so that we could repair it ourself, not perfect but
in this way, that moving of the specimen would be possible?

Bettina Friedel

____________________________

From MicroscopyL-request-at-ns.microscopy.com Wed May 12 22:08:20 2004

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That is nice, but I would like more justification about
why only one point is adequate. I do not buy into this
hypothesis.

EDAX uses Al and Cu peaks. I think that this works very well.
And, it uncovers subtle problems that otherwise would go
un-noticed. I cannot see how a one point calibration
is a calibration at all. Please explain this to me.

The two disparate Al-Cu peaks makes a lot of sense for
calibrating an EDS. In addition to this, I do C, O, F
and Al measurements with one stub. This is a separate
"standard." When the results shift, if they do, I am
concerned. Lately, they have shifted. And I am concerned.
EDAX is on the job. Cool.

The point is to establish a set of standards and
use them frequently. When the results change, contact
the manufacturer. They will not know your situation
unless you tell them.

gary g.

At 02:52 PM 5/12/2004, you wrote:
} Michael,
}
} In response to your question, most, if not all, EDX manufacturers today
} including RÖNTEC find it necessary to use only one specified energy line
} plus the zero peak. This is because linearity is so high, that a 3-point
} calibration (two specified spectral lines + zero peak) for almost all cases
} is not beneficial.
}
} Martin Rohde
} RÖNTEC GmbH
} RÖNTEC USA, Inc.
} www.rontec.com
}
} } On May 12, 2004, at 2:57 AM, michael shaffer wrote:
}
} } Out of curiosty, why would a calibration use these
} } 2 peaks rather than CuK and CuL?? Understandably,
} } the L-line would be a convolution of the L-family,
} } but I would think the Al K line is in a more difficult
} } location relative to the slope in the continuum(???)
} } Is there any preference with respect to EDX window
} } type? (e.g., Be v UTW)
} } }
} } I've thought that for a long time but have yet to find a
} } software-based calibration that can use the 2 Cu peaks. Maybe the
} } vendors can speak to this.

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 02:22:32 2004

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Intersting !

The topic shifted a bit but with interesting points !

About that calibration questions, my few (Euro) cents :

No ADC ? Of coarse, an ADC is still necessary, but just after the
(still analogic) preamp, and no more after the hole ( former analogic)
counting unit.

Two points or more for energy calibration ? First point, the zero.
I suppose that all today sold systems, like that we have, have a dynamic
zero measurement, done on the noise peak. So nothing to do with the zero,
it is continously corrected. I suppose too that the energie range of the
(numerical) MCA is linear. So one (measured) peak in the midlle of the
range, that is between 6 and 12 keV will be good, as said a k line will be
sharper. Fe, Co or Cu... On our first Tracor NS 880, it was the first job
every morning, to play with the the gain and offset trimpot, on two lines.
With 150 eV resolution and a Be window, Al K was better tha Cu L (+ Cu K
for high energy). A good way to put your nerves in condition to welcome
your boss with a smile, when he came with a stupid question !

How often is it necessary to calibrate it ? Depends of the
stability of the system and of the accuracy wanted. But realy, the need of
a new calibration will be easily seen when one look the currently acquired
spectra. Particulary when one work with the same family of coumpound. A
shift in energy, whith a good statistic, if not been quantified, can be
well detected with the eyes ! It's too with the eyes on the spectrum, that
one can apreciated the real presence of a trace element, even when the
soft say that you have 0.000005 % of element Xy (without overlapping, of
coarse) !

And the embeding of my standards ? Nothing more to suggest ? My tests with
the epoxy I have show that it is not fluid enough. So, much bulbes...

Jacques

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 02:36:03 2004

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Resisted the urge to jump in before now, but can't any longer.

Your reasons for use of two K peaks is good, might I also add that K peaks
will also offer better statistics as their count rates will be higher, thus
distinguishing them better from noise and background. Most software these
days allows the use of any two peaks. The choice of calibration peaks
should be made on the materials you normally analyze. There can be
non-linearities in the detector, pre-amplifier and amplifier responses that
could be a problem if you choose peaks that are too widely separated.
Aluminum and copper are commonly used because they fall within the range
of elements commonly analyzed. If, on the other hand, you commonly are
analyzing lanthanide's or actinides, you might want to choose peaks of
higher atomic number.

Problem is that we still have to render the avalanche pulse output from a
silicon detector, that merges millions of electron transfers into a single
pulse who's voltage peak represents energy of the x-ray photon causing it,
to a digital format. That pretty much is the definition of an analog to
digital converter. This function is not abandoned in current designs, only
performed earlier in the electronics. There is still an A/D converter in
the signal chain, it is just faster and controlled by a DSP.

Modern designs, because of increased time resolution of processors and A/D
converters, use digital signal processors (DSP) to provide many of the
functions that were previously done with dedicated electronics. This
trade-off has its own set of problems. Firmware is now responsible for the
identification of peaks, dead time and pulse pile-up and there may be cases
where that firmware could use a little tuning. This trend has resulted in
manufacturer's claims of greater counting rates and resolution but also
results in greater uncertainties as manufacturers strive to meet those
claims. If you are finding that you have to calibrate your EDS system more
frequently that is probably because of those uncertainties.

The recent trend has been to blame the inadequacies of EDS analyses on the
interpretation of the signals from the detectors rather than those signals
themself. In truth, we seem to have, for the moment, stretched the limit
of detector technology and perhaps over-stretched the detection of those
signals. The need for more frequent calibration may well be because the
state of the art in pulse measurement has exceeded the state of the art in
detector technology.

This thread has bifurcated into one that addresses the basic energy
calibration of the detector and electronics and one that addresses the
similar matrix calibrations required for good quantitative analysis. In
regards to that, let me say that these are two very different, yet
interrelated, areas. These are some of the most accurate measurements made
in common laboratory settings and deserve some common understanding. In
one case, we are calibrating our instrumentation to simplistic physical
properties we understand. In the other, we are accommodating our
instruments to complex interactions that we can't completely explain.

EDS calibration involves finding two reliable points that we can use to
establish a linear correction to the corresponding digital values that are
delivered to the computer doing the analysis. While the underlying
assumption is that this is a linear relationship, that's not necessarily
so. That assumption is generally made in the software that then uses this
data to produce results that claim to be quantitative using either
standards based or standardless algorithms.

Similar matrix calibration involves the use of well characterized standards
that are of a range of composition similar to that expected in the unknown
sample to provide a refinement of the simplistic linear corrections
mentioned above. These standards and corrections allow us to improve our
quantitative estimations by narrowing the range of linear corrections used.
In reality, the interelement interactions in any particular sample can not
be completely derived from the actions of their individual components at
the present time.

This is still an empirical science, like it or not. As such, we have to
continually accommodate our instrumentation to the task rather than to an
ideal. Those accommodations will continue to be a problem and a limitation
to the results we derive.

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174

phone (630) 513-7093 fax (630) 513-7092 http://www.sem.com

On Wednesday, May 12, 2004 6:09 PM, Mary Mager
[SMTP:mager-at-interchange.ubc.ca] wrote:
}
}
}
------------------------------------------------------------------------
------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
} Dear Peter,
} Your age is showing, the electronics are all purely digital, now. No A/D
} converter needed. The only reason to use two Ka peaks instead of a Ka and
an La
} peak are that the Ka peaks are sharper and so the peak centroid is more
} precisely located. The software calibration sets the zero point and the
} amplifier gain to a fraction of a channel. With the newer,
higher-resolution
} detectors, more quant precision and lower detection limit is possible,
but the
} calibration is more critical, since a tiny shift of the peak throws off
all the
} quant calculations. I find my self calibrating every month where I used
to do it
} once a year with the old A/D system, but my results are much better.
} Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on
occasion.
} Regards,
} Mary Mager
} Electron Microscopist
} Department of Materials Engineering
} University of British Columbia
} 6350 Stores Road
} Vancouver, B.C. V6T 1Z4
} CANADA
} tel: 604-822-5648
} e-mail: mager-at-interchange.ubc.ca
}
} ----- Original Message -----
} } From: "Tomic, Peter (Peter)" {ptomic-at-agere.com}
} To: "Mary Mager" {mager-at-interchange.ubc.ca} ; "michael shaffer"
} {michael-at-shaffer.net}
} Cc: "Microscopy" {microscopy-at-MSA.microscopy.com}
} Sent: Wednesday, May 12, 2004 3:49 PM
} Subject: [Microscopy] RE: Re: RE: Re: EDS standards embedding
}
}
} I believe the real object of this is to find two peaks separated far
enough in
} energy to allow the A/D converter to calibrate over a broad range. The
broader
} the less the error. From an electronic point of view, it doesn't matter
which
} peaks are used, just that they have significant separation. The
electronics
} doesn't know the difference. It goes from peak height to a position in
energy
} which corresponds to a voltage which gates a clock. I'm babbling, only
} electrical engineers worry about these things.
}
} Any EDX vendors care to comment?
}
} Peter
}
} -----Original Message-----
} } From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
} Sent: Wednesday, May 12, 2004 4:31 PM
} To: michael shaffer
} Cc: Microscopy
} Subject: [Microscopy] Re: RE: Re: EDS standards embedding
}
}
}
}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
} Dear Michael,
} I just checked, and my Quartz XOne system can use any two peaks,
including Cu Ka
} and Cu La, to calibrate the system. The tradition may be to use Al Ka and
Cu La
} because those two elements are easy to find in most EM labs and the old
} Be-window detectors did not always see Cu La well. Of course, the
accuracy of
} your calibration will depend on the separation of your peaks and their
accurate
} location. Ka peaks are sharper than La peaks, so it may improve your
calibration
} accuracy to use two Ka peaks.
} Disclaimer: I act as a EDS consultant to Quartz Imaging Corp. on
occasion.
} Regards,
} Mary Mager
} Electron Microscopist
} Department of Materials Engineering
} University of British Columbia
} 6350 Stores Road
} Vancouver, B.C. V6T 1Z4
} CANADA
} tel: 604-822-5648
} e-mail: mager-at-interchange.ubc.ca
}
} ----- Original Message -----
} } From: "michael shaffer" {michael-at-shaffer.net}
} To: "Gary Gaugler" {gary-at-gaugler.com}
} Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
} Sent: Wednesday, May 12, 2004 2:57 AM
} Subject: [Microscopy] RE: Re: EDS standards embedding
}
}
} }
} }
} }
------------------------------------------------------------------------
------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
------------------------------------------------------------------------
------
} -
} }
} } Gary writes ...
} }
} } } The "normal" calibration of EDS is done at Al
} } } K alpha (1.486KeV) and Cu K alpha (8.040KeV).
} } } ...
} }
} } Out of curiosty, why would a calibration use these
} } 2 peaks rather than CuK and CuL?? Understandably,
} } the L-line would be a convolution of the L-family,
} } but I would think the Al K line is in a more difficult
} } location relative to the slope in the continuum(???)
} } Is there any preference with respect to EDX window
} } type? (e.g., Be v UTW)
} }
} } cheerios ... shAf :o)
} } Avalon Peninsula, Newfoundland
} } www.micro-investigations.com (in progress)
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 02:47:11 2004

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Hi,

Most of us at some moment have to deal with the capture and storage of
image sequences, either as part of a video-experiment or when doing a
video time-lapse. Until 3 years ago, I did my video-microscopy on a
Silicon Graphics based system. The nice features of SGI were that we
could do multiple videostreams in parallel, which allowed us to do
multiposition time-lapse experiments.

However, three years ago I changed to another Unix-platform (Linux) and
to my unpleasant surprise, it was not so trivial anymore to keep
multiple video-streams in the air during an experiment and there were
some other caveats too.

In the end I decided that the only thing I needed was a simple way to
concatenate individual frames into a filestream, as for me the most
important issue is to put the frames where I can find them afterwards
for analysis, not so much for looking a them over anetwork at high
speed. The format should be simple, no overhead and frame-oriented, so
even mixing frames of different types should be possible. Another thing
I wanted to have, was that it should be possble to store 3D-frame
movie-sequences. Lossy compression schemes are not so beneficial for
image anlsysis aftwerwards, as they manipulate the frame content which
causes artefacts in the analysis.

The drawback of this frame-oriented approach is that some lossy
compression techniques, which require multiple frame comparison, are not
possible.

I would like to know if there are other people, doing video microscopy
who are also interested in this approach, maybe we could create a simple
software-library (ANSI C) which we can link with software we use, so we
can have a video-system designed and optimized for video-microscopy
(analysis oriented instead of visualization-oriented) ?

Regards,

Peter Van Osta

Director Imaging
MAIA SCIENTIFIC (formerly Union Biometrica NV)
Cipalstraat 3
B-2440 Geel
Belgium
Tel.: +32-(0)14 570 620
Fax.: +32-(0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 03:08:48 2004

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Sharon,
it is possible to spend a lot of money on these systems. However, I
have yet to find one which offers significantly more than can be done with
MSExcel spreadsheets.

MSExcel spreadsheets on a server can be used in a 'shared' format, where
many people can open the same file without that irritating 'This file is
being used by...' error. In the system we have here, the files can only be
written to by a member of the analysis group, but read by anyone. People
have to come here to give us a sample anyway, so this is not a problem.
Each sample gets a line in the spreadsheet with the usual fields (date,
name, analysis needed etc.). When someone is working on a job, they put
their initials in the box for that analysis type; when the job is done, a
date goes in the box instead. The spreadsheet is updated every time someone
saves it. Each column has an 'Autofilter' at the top which means they can
be searched for any of the fields.
This 'master' spreadsheet contains hyperlinks to the electronic log books
for each microscope or technique (also shared MSExcel spreadsheets). These
are updated as the analysis happens, and here each image has a line giving
sample, analysis details, operator, customer, etc.. Each line in these
'technique' spreadsheets has a hyperlink to the data file. Again, each
column has an 'Autofilter' at the top which means they can be searched for
any of the fields.

As a user, it is easy to operate (that 'fill down' feature of Excel allows
you to copy the provious line and change one box without having to make 10
entries for each image). The only discipline needed is to keep saving the
files frequently (autosaving doesn't work, if two computers try to save at
the same time they can lock up). Our customers seem to be happy too - they
know the status of their job and can find the data without having to hassle
us. We rely on the standard software on each user's PC to be able to open
the images.

I'm not sure how this could be implemented on a web-based system, but for a
server it works very well. We keep track of about 4000 samples a year - and
all the data files they generate - with this system, and it usually only
takes a few minutes to find old data even from a vague description. I have
yet another spreadsheet which allows me to count how many jobs have been
done, are left to do, etc., for each analysis type. The nice thing about
spreadsheets is that they are totally 'customizable', so you only keep track
of what you think is important.

I'd be happy to send you an example of the files if you like. As a 'free'
solution it is hard to beat!

Cheers

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com
All incoming mail is filtered for spam. If you do not receive a reply from
me, do not assume I have received your mail.

-----Original Message-----
} From: Sharon_Goresh-at-engelhard.com [mailto:Sharon_Goresh-at-engelhard.com]
Sent: 12 May 2004 19:20
To: Microscopy-at-MSA.Microscopy.Com

Fellow Microscopists,

The Microscopy Lab in our Research Center has 3 SEM's, 1 TEM and 1 EMPA
(with a second due in November) in addition to 4 XRD instruments. Our
main function has been as a problem solving facility to our researchers as
well as our field service engineers. Data produced by our lab is usually
issued as reports with images, spectra and graphs as attachments.
Management has directed us to implement a LIMS by the end of the year.
Their requirements include the ability of the researchers and field service
engineers to log samples in from their locations and the tracking of the
sample from the arrival in our lab to the issuance of data. It must also
be able to archive the data as well. For us this means literally hundreds
of images, spectra and reports each month that must be categorized and
saved. The researchers and engineers must also be able to access the data
from their location. This will probably mean a web based system since our
facilities cover the globe.

Has anyone out there been faced with a similar request? Our main hurdle is
convincing management that ours is not a "sample in - number out" type of
lab, and that most LIMS packages out there are designed for that type of
simple operation. If you have implemented such a system, was it an off the
shelf package, a custom designed package or a combination? If you want to
respond to me directly that would be fine. I am not interested in "system
bashing" just some helpful suggestions on how to make management happy
without losing my sanity.

Sharon Goresh
Chemist
sharon.goresh-at-engelhard.com

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From MicroscopyL-request-at-ns.microscopy.com Thu May 13 05:16:19 2004

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Dear Michael,

A two-step detection method is indeed a good option to visualize your
biotinylated viral protein. Compared to the 2-step method the advantage
of a 1-step immunodetection method, as you initially suggested, will be
improved resolution. Your labeling density decreases however. As you
know labeling density is inversely related to the gold particle size.

Improved resolution combined with high sensitivity can be obtained when
using gold conjugates prepared with Ultra-Small gold particles. For
your application we would recommend Goat anti Biotin Ultra-Small. See
e.g. Müller-Höcker et al., (1998), Histochem. and Cell Biol. 109(2),
119-125.

When the protein of interest is located on the outside of the virus, in
other words the biotin is accessible for the antibodies, another option
may be the use of a pre-embedding labeling procedure. The use of
Ultra-Small gold conjugates is a prerequisite to successfully combine
appropriate labeling densities with a decent morphology. See e.g.
Decossas et al, (2003) J. of Comp. Neurology 462(3), 302-314 for
details on this technique.

Hope this is of help
Kind regards,
Peter

------------------------------------------
Michael Jarnik wrote:

Sorry, I would try to make it clearer. We need to localize a viral
protein which has been biotin-tagged and expressed in cell culture. I
expected it should be no problem to label it with Streptavidin
conjugate, but it is not that easy, it seems (even according to some
other people). So, as we do not have a good antibody to the viral
protein, I am considering an indirect labeling with anti-biotin
antibody and a secondary conjugate. There are tons of commercially
available anti-biotin antibodies, but certainly not all of them will
work with EM protocols - so I was interested whether somebody has
experience with some of these.

Thanks,

Michael

-----------
Peter van de Plas
Aurion
Costerweg 5
6702 AA Wageningen
The Netherlands
Phone: +31 317 497676
Fax: +31 317 415955

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 06:55:04 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Michael,

A two-step detection method is indeed a good option to visualize your
biotinylated viral protein. Compared to the 2-step method the advantage
of a 1-step immunodetection method, as you initially suggested, will be
improved resolution. Your labeling density decreases however. As you
know labeling density is inversely related to the gold particle size.

Improved resolution combined with high sensitivity can be obtained when
using gold conjugates prepared with Ultra-Small gold particles. For
your application we would recommend Goat anti Biotin Ultra-Small. See
e.g. Müller-Höcker et al., (1998), Histochem. and Cell Biol. 109(2),
119-125.

When the protein of interest is located on the outside of the virus, in
other words the biotin is accessible for the antibodies, another option
may be the use of a pre-embedding labeling procedure. The use of
Ultra-Small gold conjugates is a prerequisite to successfully combine
appropriate labeling densities with a decent morphology. See e.g.
Decossas et al, (2003) J. of Comp. Neurology 462(3), 302-314 for
details on this technique.

Hope this is of help
Kind regards,
Peter

------------------------------------------
Michael Jarnik wrote:

Sorry, I would try to make it clearer. We need to localize a viral
protein which has been biotin-tagged and expressed in cell culture. I
expected it should be no problem to label it with Streptavidin
conjugate, but it is not that easy, it seems (even according to some
other people). So, as we do not have a good antibody to the viral
protein, I am considering an indirect labeling with anti-biotin
antibody and a secondary conjugate. There are tons of commercially
available anti-biotin antibodies, but certainly not all of them will
work with EM protocols - so I was interested whether somebody has
experience with some of these.

Thanks,

Michael

-----------
Peter van de Plas
Aurion
Costerweg 5
6702 AA Wageningen
The Netherlands
Phone: +31 317 497676
Fax: +31 317 415955

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 09:29:14 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rosscac-at-aol.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, May 13, 2004 at 07:52:40
---------------------------------------------------------------------------

Email: rosscac-at-aol.com
Name: Connie Cummings

Title-Subject: [Microscopy] [Filtered] Print processors

Question: I am interested in purchasing a print processor and was
wondering if anyone out there is using or has used either a Fujimoto
Roller Transport print processor CP51 or a JOBO printlab 3504 print
processor. I was looking for some feedback on these units on there
durablility and functionalitiy or any other tidbits! You can respond
back via email to me at rosscac-at-aol.com or at
connie.a.cummings-at-gsk.com.
Thanks in advance.
Connie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:01:17 2004

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Hi fellow microscopists,

A post doc is trying to detect GFP being expressed in plant leaves. She is
fixing leaves in formaldehyde and doing a standard paraffin embedding. Her
question is if GFP going to survive xylene treatments for paraffin
infiltration. She plans to section the paraffin embedded blocks and look
for GFP using fluorescence microscopy.

If anyone has an answer please reply back to me.

Thanks in advance.

Soumitra

*************************************************************
Soumitra Ghoshroy
College Associate Professor, Biology
Director, Electron Microscopy Lab
Box 3EML
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office), 646-3283 (lab)
Fax: 505-646-3282
e-mail:sghoshro-at-nmsu.edu
http://www.cs.nmsu.edu/~biology/Faculty%20&%20Staff/Ghoshroy/Ghoshroy.htm
http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:16:44 2004

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hi all!

a simple question :

Does anyone have ever used graphite for sputtering or coating a SEM
sample ?

maybe a question from a dummy boy :-) , doesn't it?

thanx for answers...

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:35:04 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all,
Lazy me recommended pre-coated SuperFrostPlus slides to Anne Dunn a
post-doc working on antlions but the gut goo doesn't always survive her
processing protocol (see her message below).

So the question is - What is the preferred slide coating method?
Gelatin vs poly-L-lysine...or something else?

advice and recipes would be greatly appreciated.
thanks,
Beth

} Hi Beth,
}
} I am finding that when I use the superfrost plus slides for
} my cryosections that often if there is material inside the
} gut that it will wash away as I am fixing and dehydrating
} my sections before hybridization (and I am not seeing any
} bacteria in the gut area after hybridization). I have no idea
} whether it is just something that is going to happen with
} a fluid-feeding insect, or if it is the superfrost slides not
} being sticky enough. I don't seem to be having a
} problem with the tissue itself sticking.
}
} I was looking up ways to coat slides and found there is
} the gelatin method and the poly-L-lysine method.
} Unfortunately I am not finding any info that tells me if one
} is better than the other. Do you have an opinion? I was
} wondering if it is a case of one coating being better for
} certain applications than another?
}
} I was going to go ahead and dissect out a gut or two, fix
} and hybridize them, trying to see if I can find any
} bacteria-like objects in the gut smooshate...to let me
} know if the loss of the material in the gut is an issue or
} not, but wanted to start thinking/plotting if I need to coat
} some slides.

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 10:52:50 2004

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I'm looking for a shield to exclude air movement around the stage of my
Ultracut. I remember years ago having one for my Reichert OM-U3 but I
don't believe I got one for my Ultracut a few years ago. I've checked a
couple of the vendors and found nothing. I could find nothing at the
Leica site either. Does anyone have a source for these or will I have
to make my own?

Rick A. Harris, exDirector
Microscopy and Imaging Facility
Section of Molecular and Cellular Biology
1241 Life Sciences Addition
University of California
Davis, CA
530 752 2914
http://microscopy.mcb.ucdavis.edu
raharris-at-ucdavis.edu

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 11:41:29 2004

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Hello Sharon,

Richard is of course right -- you can spend a fortune on LIMS systems and
for most users it may be overkill. On the other hand, the Excel sheets that
Richard mentions may be too limited.

A third option, somewhat in the middle, could be to use software that
supports or can read the images and other data from your software and keep
track of those in an archive or database. That way you can search for
keyfields, you deal with the same software for all applications, and you can
distribute the images easily. Our software analySIS includes such a
database. We also have a web frontend for this database so you can deal with
the global issues you mentioned.

Please take a look at our website or contact me directly if you wolud like
to get more information.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Richard Beanland [mailto:richard.beanland-at-bookham.com]
Sent: Thursday, May 13, 2004 02:14
To: 'Sharon_Goresh-at-engelhard.com'
Cc: 'Microscopy-at-MSA.Microscopy.Com'

Sharon,
it is possible to spend a lot of money on these systems. However, I
have yet to find one which offers significantly more than can be done with
MSExcel spreadsheets.

MSExcel spreadsheets on a server can be used in a 'shared' format, where
many people can open the same file without that irritating 'This file is
being used by...' error. In the system we have here, the files can only be
written to by a member of the analysis group, but read by anyone. People
have to come here to give us a sample anyway, so this is not a problem.
Each sample gets a line in the spreadsheet with the usual fields (date,
name, analysis needed etc.). When someone is working on a job, they put
their initials in the box for that analysis type; when the job is done, a
date goes in the box instead. The spreadsheet is updated every time someone
saves it. Each column has an 'Autofilter' at the top which means they can
be searched for any of the fields.
This 'master' spreadsheet contains hyperlinks to the electronic log books
for each microscope or technique (also shared MSExcel spreadsheets). These
are updated as the analysis happens, and here each image has a line giving
sample, analysis details, operator, customer, etc.. Each line in these
'technique' spreadsheets has a hyperlink to the data file. Again, each
column has an 'Autofilter' at the top which means they can be searched for
any of the fields.

As a user, it is easy to operate (that 'fill down' feature of Excel allows
you to copy the provious line and change one box without having to make 10
entries for each image). The only discipline needed is to keep saving the
files frequently (autosaving doesn't work, if two computers try to save at
the same time they can lock up). Our customers seem to be happy too - they
know the status of their job and can find the data without having to hassle
us. We rely on the standard software on each user's PC to be able to open
the images.

I'm not sure how this could be implemented on a web-based system, but for a
server it works very well. We keep track of about 4000 samples a year - and
all the data files they generate - with this system, and it usually only
takes a few minutes to find old data even from a vague description. I have
yet another spreadsheet which allows me to count how many jobs have been
done, are left to do, etc., for each analysis type. The nice thing about
spreadsheets is that they are totally 'customizable', so you only keep track
of what you think is important.

I'd be happy to send you an example of the files if you like. As a 'free'
solution it is hard to beat!

Cheers

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com
All incoming mail is filtered for spam. If you do not receive a reply from
me, do not assume I have received your mail.

-----Original Message-----
} From: Sharon_Goresh-at-engelhard.com [mailto:Sharon_Goresh-at-engelhard.com]
Sent: 12 May 2004 19:20
To: Microscopy-at-MSA.Microscopy.Com

Fellow Microscopists,

The Microscopy Lab in our Research Center has 3 SEM's, 1 TEM and 1 EMPA
(with a second due in November) in addition to 4 XRD instruments. Our
main function has been as a problem solving facility to our researchers as
well as our field service engineers. Data produced by our lab is usually
issued as reports with images, spectra and graphs as attachments.
Management has directed us to implement a LIMS by the end of the year.
Their requirements include the ability of the researchers and field service
engineers to log samples in from their locations and the tracking of the
sample from the arrival in our lab to the issuance of data. It must also
be able to archive the data as well. For us this means literally hundreds
of images, spectra and reports each month that must be categorized and
saved. The researchers and engineers must also be able to access the data
from their location. This will probably mean a web based system since our
facilities cover the globe.

Has anyone out there been faced with a similar request? Our main hurdle is
convincing management that ours is not a "sample in - number out" type of
lab, and that most LIMS packages out there are designed for that type of
simple operation. If you have implemented such a system, was it an off the
shelf package, a custom designed package or a combination? If you want to
respond to me directly that would be fine. I am not interested in "system
bashing" just some helpful suggestions on how to make management happy
without losing my sanity.

Sharon Goresh
Chemist
sharon.goresh-at-engelhard.com

=======================================================================
This e-mail is intended for the person it is addressed to only. The
information contained in it may be confidential and/or protected by
law. If you are not the intended recipient of this message, you must
not make any use of this information, or copy or show it to any
person. Please contact us immediately to tell us that you have
received this e-mail, and return the original to us. Any use,
forwarding, printing or copying of this message is strictly prohibited.
No part of this message can be considered a request for goods or
services.
=======================================================================
Any questions about Bookham's E-Mail service should be directed to
postmaster-at-bookham.com.

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 12:27:22 2004

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Hi Beth,

We use silane to coat our slides, it is the standard for the histology labs in the pathology dept.

Silane = 3-aminopropyl-triethoxy-silane

Protocol:

Silane 20 ml
Actenoe 2000 ml

Dip precleaned slides in Silane solution for 2 minutes
Drain and wash in distilled water 2 times
Drain and dry at 60 degrees C for 1 hour
Store away from light and moisture.

Our sildes last for many months (6+), we make huge batches at a time.

I hope this helps you out of your sticky situation!

Paula :-)

Paula Sicurello
George Washington Univ. Medical Center
Electron Microscope Lab
Washington, DC 20037
202-994-2930 phone
202-994-2518 fax

} } } Beth Richardson {beth-at-plantbio.uga.edu} 05/13/04 11:38AM } } }

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hi all,
Lazy me recommended pre-coated SuperFrostPlus slides to Anne Dunn a
post-doc working on antlions but the gut goo doesn't always survive her
processing protocol (see her message below).

So the question is - What is the preferred slide coating method?
Gelatin vs poly-L-lysine...or something else?

advice and recipes would be greatly appreciated.
thanks,
Beth

} Hi Beth,
}
} I am finding that when I use the superfrost plus slides for
} my cryosections that often if there is material inside the
} gut that it will wash away as I am fixing and dehydrating
} my sections before hybridization (and I am not seeing any
} bacteria in the gut area after hybridization). I have no idea
} whether it is just something that is going to happen with
} a fluid-feeding insect, or if it is the superfrost slides not
} being sticky enough. I don't seem to be having a
} problem with the tissue itself sticking.
}
} I was looking up ways to coat slides and found there is
} the gelatin method and the poly-L-lysine method.
} Unfortunately I am not finding any info that tells me if one
} is better than the other. Do you have an opinion? I was
} wondering if it is a case of one coating being better for
} certain applications than another?
}
} I was going to go ahead and dissect out a gut or two, fix
} and hybridize them, trying to see if I can find any
} bacteria-like objects in the gut smooshate...to let me
} know if the loss of the material in the gut is an issue or
} not, but wanted to start thinking/plotting if I need to coat
} some slides.

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 13:19:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I am going to buy scanner for TEM negatives and considering two models:
Microtek ArtixScan 1800f and Epson Expression 1680 Pro. Any advise and
comments are very welcome.

Thank you in advance,

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 13:39:06 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,

I am looking for a replacement glass spacer for a Polaron E5100 series
II 'Cool' Sputter Coater. The external diameter etched on metal collar
base is 165.1 m/m. The internal diameter of the metal collar is 5.75".
The height of the glass spacer is 3 and 3/16". I have been working with
EBS to locate a replacement collar but would like to know if there are
any other sources I could contact.

Thank you in advance for your help

aruna

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 15:30:40 2004

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Dear Sylvain,
I use graphite, evaporated in a high-vacuum evaporator, to make SEM samples
conductive when I want to do EDS analysis. I use gold/palladium for SEM imaging
without analysis, but carbon coating to minimize any interference of the coating
with the EDS analysis.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "sylvain maury" {sylvain.maury-at-thalesgroup.com}
To: "Microscopy community" {microscopy-at-msa.microscopy.com}
Sent: Thursday, May 13, 2004 8:22 AM

} I'm looking for a shield to exclude air movement around the stage of my
} Ultracut. I remember years ago having one for my Reichert OM-U3 but I
} don't believe I got one for my Ultracut a few years ago. I've checked a
} couple of the vendors and found nothing. I could find nothing at the
} Leica site either. Does anyone have a source for these or will I have
} to make my own?
}
} Rick A. Harris, exDirector
} Microscopy and Imaging Facility
} Section of Molecular and Cellular Biology
} 1241 Life Sciences Addition
} University of California
} Davis, CA
} 530 752 2914
} http://microscopy.mcb.ucdavis.edu
} raharris-at-ucdavis.edu

Rick -

Make a hole in the bottom of a plastic veggie bag from your
supermarket & rubber-band it around the binocular objective. Ugly,
but it works better than a rigid plastic box.

Caroline
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 16:09:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Short and sweet: about a year ago we bought a Microtek ArtixScan 2500f (firewire); a little different from the 1800f but I don't know how much. Anyway, we like it. Great dynamic range and reasonable software (we scan into a G4 Mac running OSX).

cheers, John

********
John S. Vetrano
Sr. Research Scientist
Materials Structure and Performance Group
Pacific Northwest National Laboratory
MSIN P8-16
P.O. Box 999
Richland, WA 99352
Phone: (509)372-0724 Fax: (509)376-6308
Email: mailto:john.vetrano-at-pnl.gov

} ----------
} From: Dusevich, Vladimir
} Sent: Thursday, May 13, 2004 11:25 AM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy]
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I am going to buy scanner for TEM negatives and considering two models:
} Microtek ArtixScan 1800f and Epson Expression 1680 Pro. Any advise and
} comments are very welcome.
}
} Thank you in advance,
}
} Vladimir
}
} Vladimir M. Dusevich, Ph.D.
} Electron Microscope Lab Manager
} 3127 School of Dentistry
} 650 E. 25th Street
} Kansas City, MO 64108-2784
}
} Phone: (816) 235-2072
} Fax: (816) 235-5524
} Web: http://www.umkc.edu/dentistry/microscopy
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 16:33:19 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,
I would like to have an evaluation of the Denton Desk III TSC sputter
coater from those who are using or have used this instrument for preparation
of samples for FESEM imaging. Please direct your response to me rather than
to the list.

Many thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 18:42:36 2004

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I don't use C. I use Au/Pd and Pt. C is
too messy.

Depending on what you are looking at, either
image- or EDS/WDS-wise, your options may vary.
For EDS, I just ignore the small Au/Pd peaks.
The coating is only 40-60A and is typically
only seen as piled up Au with Al, Si and W.
With my specimens, Pd is by itself.

I suppose that if you were looking at P or Zr
specimens, Au/Pd or Pt would be a problem. Perhaps
the ultimate coating is Os. Someday, I would love
to try one of these coaters. It ought to be
great for EBSD.

But let us know what type of work you are trying
to do. That may make a big difference in coating
strategies.

gary g.

At 08:22 AM 5/13/2004, you wrote:

} hi all!
}
} a simple question :
}
} Does anyone have ever used graphite for sputtering or coating a SEM
} sample ?
}
} maybe a question from a dummy boy :-) , doesn't it?
}
} thanx for answers...
}
} Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Thu May 13 20:43:29 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I don't use C. I use Au/Pd and Pt. C is
too messy.

Depending on what you are looking at, either
image- or EDS/WDS-wise, your options may vary.
For EDS, I just ignore the small Au/Pd peaks.
The coating is only 40-60A and is typically
only seen as piled up Au with Al, Si and W.
With my specimens, Pd is by itself.

I suppose that if you were looking at P or Zr
specimens, Au/Pd or Pt would be a problem. Perhaps
the ultimate coating is Os. Someday, I would love
to try one of these coaters. It ought to be
great for EBSD.

But let us know what type of work you are trying
to do. That may make a big difference in coating
strategies.

gary g.

At 08:22 AM 5/13/2004, you wrote:

} hi all!
}
} a simple question :
}
} Does anyone have ever used graphite for sputtering or coating a SEM
} sample ?
}
} maybe a question from a dummy boy :-) , doesn't it?
}
} thanx for answers...
}
} Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 08:16:15 2004

Contents Retrieved from Microscopy Listserver Archives
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I have an earlier model of the Epson (the 1600 Pro) and I"ve been
happy with it.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 09:44:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Someone recently posed the same question on ListServer. We have an Epson
Perfection 3200 Photo and love it. There is no holder for the standard 3 1/4 X
4 negatives, but I just put them directly on the glass and they come out fine.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Dusevich, Vladimir [mailto:DusevichV-at-umkc.edu]
Sent: Thursday, May 13, 2004 2:26 PM
To: microscopy-at-msa.microscopy.com

I am going to buy scanner for TEM negatives and considering two models:
Microtek ArtixScan 1800f and Epson Expression 1680 Pro. Any advise and
comments are very welcome.

Thank you in advance,

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 15:04:09 2004

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Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Fri May 14 16:30:39 2004

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What is the cross sectional construction like?
Is the die passivated? If it is, use MIL-STD-883 for
GLIT. If there is metal underneath the passivation,
and the passivation has voids, GLIT will show it
up big time. GLIT is glassivation layer integrity test.

gary g.

At 01:10 PM 5/14/2004, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Fri May 14 17:47:07 2004

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Dear Pavel: my first thought is, don't coat the device. Find an
accelerating voltage/tilt angle combination that will prevent of
minimize charging. Next thought, coat with something besides gold. But
I've done a lot of cracked devices and have never had any problems
telling the cracks from the original surface. Unless they are huge
cracks, the gold won't get in them to confuse the issue. Are these
surface cracks or cracks going down into the surface?

AtcSEM wrote:

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--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Sat May 15 00:47:25 2004

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------------------------------------------------------------------------
------------------------------------------------------------------------
------------------------
PRINCIPLES OF FLUORESCENCE TECHNIQUES COURSE 2004.

LAMBS, Department of Physics, University of Genoa, June 14-16, 2004.

The use and application of fluorescence techniques is increasing daily
both in the academia and in industry. The Principles of Fluorescence
Techniques course will outline the basic concepts of fluorescence
techniques and the successful utilization of the currently available
commercial instrumentation.

The course is designed for students who utilize fluorescence
instrumentation and techniques, as well as for researchers
and industrial scientists who intend to deepen their knowledge of
fluorescence techniques. The theoretical lectures delivered by key
scientists in the field are complemented by the direct utilization of
steady state and lifetime fluorescence instrumentation provided by
leading companies.

It is recommended that participants have at least a bachelor's degree
in the life science, physical sciences or engineering before attending
this course. Topics addressed in this course include:

Basic Definitions and Principles of Fluorescence
Fluorescence Polarization
Time- resolved Fluorescence
Instrumentation

Data Manipulation and Data Analysis
Fiber Optic Sensors
Confocal Fluorescence Microscopy
Lifetime Imaging
Fluorescence Correlation Spectroscopy
Multiphoton excitation microscopy and spectroscopy
Quantum dots

The Principles of Fluorescence Techniques course will be held at:

Laboratory for Advanced Microscopy, Bioimaging and Spectroscopy
Diaspro lab, Research Center MICROSCOBIO
Department of Physics, University of Genoa
via Dodecaneso, 33
16146 Genova, Italy

Details: www.lambs.it; diaspro-at-fisica.unige.it

The number of participants to the Principles of Fluorescence Techniques
Course

is limited to 40 people. PLEASE RESERVE YOUR PARTICIPATION AS SOON AS
POSSIBLE SENDING AN E-MAIL TO: coordinator-at-fluorescence-foundation.org.

Details : www.fluorescence-foundation.org
------------------------------------------------------------------------
------------------------------------------------------------------------
------------------

------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun May 16 13:24:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (zr zrzhang_xrli-at-ybb.ne.jp) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Saturday, May 15, 2004 at 21:16:24
---------------------------------------------------------------------------

Email: zr zrzhang_xrli-at-ybb.ne.jp
Name: Zheng-Rong Zhang

Organization: Yokohama National University

Education: Graduate College

Location: Yokohama, Japan

Question: Dear Microscopist,

I need to prepare TEM samples from Ag and Ag-Pd(10pct) alloy sheets. May you suggest me any electrolytes for twin-jet electropolishing and the corresponding conditions? No toxic chemicals would be used.

Thank you in advance!

With best regards

Zheng-Rong Zhang

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jtrynak-at-SciGenium.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 12, 2004 at 18:22:09
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Email: jtrynak-at-SciGenium.com
Name: JT Rynak

Organization: SciGenium

Title-Subject: [Microscopy] [Filtered] Opening - New England Regional - Imaging Sales

Question: New England Regional - Imaging Sales

5+ years experience selling imaging / visualization capital equipment into Research Market space. Ideal person will have a rolodex of PI and Lead Vivo research scientists. BS/MS is Biology or Zoology

If you have any further questions feel free to contact me at 617-661-1067 or via email at jtrynak-at-scigenium.com

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From MicroscopyL-request-at-ns.microscopy.com Sun May 16 18:53:06 2004

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Pavel;

Having looked at more fractures in silicon and GaAs devices than I care to remember, it's not generally a problem finding them and as often with optical means as with EM.

If you would kindly provide the list with more specifics about your samples and the nature of these "cracks?" That is, are they along crystal planes or fractures that travel at random angles with respect to the surface? Fractures, or cleaves perpendicular to the die surface, are difficult to detect with EM but apparent with visible light microscopy. How separated are both sides of the crack and why do you need to see into them? Sounds like you only need to identify whether they exist or not. How long are the cracks?

I have plenty of EM's I'd be happy to send you images of samples that have fractured for various reasons, and there are multiple root causes of this failure mechanism. I'm sure if you provide a little more detail you'll get plenty of good suggestions on how to image your samples.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Friday, May 14, 2004 4:10 PM
To: MicroscopyListServer (MicroscopyListServer)

Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Sun May 16 19:26:15 2004

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Any course that will promote even the correct spelling of
fluorescence has to be a good thing.

Maybe someone will run one on how to spell 'JEOL' someday.

:)

cheers

rtch

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 00:12:47 2004

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Hello listers,

We are in the process of justifying, to the University, a proposal to
purchase an ESEM. In prepapring the business case I am including the
ten year financials for both FEG and Tungtsen filament machines. Given
that we have to break even in that time, including covering our
depreciation, the Tungsten instrument is easier to justify in a purely
financial sense.

From a scientific and operational viewpoint, though, I was hoping some
of you could provide opinions on the relative merits of Tungsten or FEG.
Our current conventional SEM is a Philips XL-30 S-FEG so we already know
of the costs associated with the emitter.

The range of samples we will be required to put in our ESEM will be
anything you oculd possibly imagine from the Faculties of Engineering,
Science and Medicine. Samples will inlcude food materials (big dairy
industry in New Zealand), polymers, conducting polymers, mammalian
tissue, bacteria, fruit and veg, fish and chips, superconductors,
ceramic coatings and bees knees. We will definitely need a hot-stage.

If you would like to contact me off list with your opinions please feel
free.

Kind regards
Bryony James
Research Centre for Surface and Materials Science
Univetrsity of Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 07:57:52 2004

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Thank you all for the responses that I have received.

Just to clarify:
We had multiple field failures of the chips. The SEM examination
revealed some sort of coating on the fracture surfaces, which I believe is
the urethane coating. The transition from the side wall to the fracture
surface, on some of the chips, suggests that the chips could have had a
small cracks prior urethane coating.

Now, I am looking at the "Virgin" chips for any evidence of cracking
at the side wall and diaphragm transition, but my problem is that the Gold
coating does not coat the area well enough for me to resolve the crack. Due
to lack of coating that area is charging and I see only a black line.
I have coated it at least 3 times and rotate the chips to insure good
coatings in those areas, but it was not enough.

After SEM examination I would also like to cross section the chip to check
for the evidence of pre-cracks, but I am afraid to introduce the cracks
myself. Could you help me with a proper preparation procedure of the cross
sections? We have metallography lab. equipment and nothing special to
prepare the chip cross sections.

I have uploaded some more photos of the fracture surfaces of the failed
chips and Virgin chip that I am trying to image now.
http://www.atclabs.com/images/temp/MicrList_files/frame.htm

Sorry, it might be a little slow at showing the images due to their size.

Thanks for your help again,

Pavel

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]

What is the cross sectional construction like?
Is the die passivated? If it is, use MIL-STD-883 for
GLIT. If there is metal underneath the passivation,
and the passivation has voids, GLIT will show it
up big time. GLIT is glassivation layer integrity test.

gary g.

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]

Do you get charging at the crack due to a gap in the coating?
Otherwise,you should be able to see the break.

-----Original Message-----
} From: Jim Quinn [mailto:jquinn-at-www.matscieng.sunysb.edu]
Pavel

Your image is very low mag, so it is difficult to judge anything.

I suggest that you use a sacrificial chip and coat
it with about 10nm of gold. If your coater does not
rotate the sample, then you should manually rotate
the sample at 45 degrees atleast twice. This is
will help the gold to get into the perpendicular
surfaces.

Next use a Robinson BS detector. 10 or 15kV is sufficient.

Once you image the cracks, then you can go about
trying to image without the gold. Variable pressure
and voltage will reduce charging in uncoated samples.

JQ

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Pavel;

Having looked at more fractures in silicon and GaAs devices than I
care to remember, it's not generally a problem finding them and as
often with optical means as with EM.

If you would kindly provide the list with more specifics about your
samples and the nature of these "cracks?" That is, are they along
crystal planes or fractures that travel at random angles with respect to
the surface? Fractures, or cleaves perpendicular to the die surface, are
difficult to detect with EM but apparent with visible light microscopy.
How separated are both sides of the crack and why do you need to see into
them? Sounds like you only need to identify whether they exist or not.
How long are the cracks?

I have plenty of EM's I'd be happy to send you images of samples
that have fractured for various reasons, and there are multiple root
causes of this failure mechanism. I'm sure if you provide a little more
detail you'll get plenty of good suggestions on how to image your
samples.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Friday, May 14, 2004 4:10 PM
To: MicroscopyListServer (MicroscopyListServer)

Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 09:11:57 2004

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Thank you so much for all of your advice. I received a large number of
great suggestions and almost everyone suggested using anti GFP antibody
and we are certainly going to go that route.

Thanks again and this is truly a great resource.

Best wishes,

Soumitra

*************************************************************
Soumitra Ghoshroy
College Associate Professor, Biology
Director, Electron Microscopy Lab
Box 3EML
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office), 646-3283 (lab)
Fax: 505-646-3282
e-mail:sghoshro-at-nmsu.edu
http://www.cs.nmsu.edu/~biology/Faculty%20&%20Staff/Ghoshroy/Ghoshroy.htm
http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 11:36:59 2004

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I think I can offer a few ideas and questions.

1) Can you say "stress concentration"? My academic background is in
Engineering Science and Mechanics. It looks like you have some very sharp
corners where the diaphragm meets the substrate. That is trouble waiting to
happen. I cannot tell if there is any pre-crack there. There might be hints
of one in slide 43. Either way, that geometry is going to lead to problems.
The stresses will be highest at the edges of the diaphragm. I think you
would prefer a gradual change in geometry there to avoid any concentration
and to help reinforce the edges. I don't know the fabrication process, and
it might be hard to implement, but it might be worth investigating.

Slides 38 and 42 show some jagged surfaces. I guess those are the edges of
the substrate and the diaphragm is on the bottom. If so, the nose of the
jaggie jutting out further into the opening will be a point of stress
concentration.

You may also want to consider round openings in the substrate. The corners
of the square holes don't help and might hurt. The highest stresses should
be in the middle of the edges.

2) You haven't said how prematurely these chips failed. Are they subjected
to a cyclic load? What fraction of their design load were they subjected
to? There may be hints of fatigue failure (slide 34?), but it seems to be
rather short cycle fatigue if it is fatigue at all. I have seen glass break
with such fractures in overload.

3) Slides 37, 40 and 41 show dark corners. I think that is the normal
appearance for an interior corner in secondary mode. An exterior corner
tends to show up bright in SE mode.

4) I can't quite tell where many of the photos were taken (e.g., slides 13
and 39). I usually use a three-fold step in magnification to easily follow
from one view to another. Also, the progressions 10, 30, 100, 300 or 15,
50, 150, 500 are easy to remember and to standardize on.

5) Did you copy these images into Powerpoint to make this presentation? My
computer took quite a while to load each slide, and I have a fast
connection. We routinely record our SEM images at 1024-pixels across and
store the files as JPGs. (Keep reading for the rationale.) Those files are
maybe 300 KB in size. If I use the Insert, Image, From_file function to add
the image to my document, it retains the JPG compression and gray nature
and requires only 300 KB. But, if I open those files in an imaging program
and copy them over they expand. The computer has the image rendered as a
bitmap in full color, the image gets copied with no compression and it now
consumes 2400 kB (1024x768 pixels times 3-bytes-per-pixel). That 8-fold
difference in size is noticeable. I know more and more users have broadband
connections; however these order-of-magnitude expansions start to add up. {g}

Hope this helps.

Warren

At 08:06 AM 5/17/2004, you wrote:

} Thank you all for the responses that I have received.
}
} Just to clarify:
} We had multiple field failures of the chips. The SEM
} examination
} revealed some sort of coating on the fracture surfaces, which I believe is
} the urethane coating. The transition from the side wall to the fracture
} surface, on some of the chips, suggests that the chips could have had a
} small cracks prior urethane coating.
}
} Now, I am looking at the "Virgin" chips for any evidence of cracking
} at the side wall and diaphragm transition, but my problem is that the Gold
} coating does not coat the area well enough for me to resolve the crack. Due
} to lack of coating that area is charging and I see only a black line.
} I have coated it at least 3 times and rotate the chips to insure good
} coatings in those areas, but it was not enough.
}
} After SEM examination I would also like to cross section the chip to check
} for the evidence of pre-cracks, but I am afraid to introduce the cracks
} myself. Could you help me with a proper preparation procedure of the cross
} sections? We have metallography lab. equipment and nothing special to
} prepare the chip cross sections.
}
} I have uploaded some more photos of the fracture surfaces of the failed
} chips and Virgin chip that I am trying to image now.
} http://www.atclabs.com/images/temp/MicrList_files/frame.htm
}
} Sorry, it might be a little slow at showing the images due to their size.
}
} Thanks for your help again,
}
} Pavel

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 11:44:19 2004

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We look mostly at hydrated biological samples. We have a
tungsten gun XL30 ESEM TMP. For looking at bacteria and
cells a FEGESEM would be superior in terms of reduced
damage and improved resolution. I find it hard to get
medium/high resolution with wet biological samples. I feel
FEGESEM would make this a lot easier.

Dave

On Mon, 17 May 2004 17:21:33 +1200 Bryony James
{b.james-at-auckland.ac.nz} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hello listers,
}
} We are in the process of justifying, to the University, a proposal to
} purchase an ESEM. In prepapring the business case I am including the
} ten year financials for both FEG and Tungtsen filament machines. Given
} that we have to break even in that time, including covering our
} depreciation, the Tungsten instrument is easier to justify in a purely
} financial sense.
}
} From a scientific and operational viewpoint, though, I was hoping some
} of you could provide opinions on the relative merits of Tungsten or FEG.
} Our current conventional SEM is a Philips XL-30 S-FEG so we already know
} of the costs associated with the emitter.
}
} The range of samples we will be required to put in our ESEM will be
} anything you oculd possibly imagine from the Faculties of Engineering,
} Science and Medicine. Samples will inlcude food materials (big dairy
} industry in New Zealand), polymers, conducting polymers, mammalian
} tissue, bacteria, fruit and veg, fish and chips, superconductors,
} ceramic coatings and bees knees. We will definitely need a hot-stage.
}
} If you would like to contact me off list with your opinions please feel
} free.
}
} Kind regards
} Bryony James
} Research Centre for Surface and Materials Science
} Univetrsity of Auckland
} New Zealand
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 13:37:31 2004

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We are an independent commercial lab serving general industry. Unless
directed by a court order or we suspect misuse of our findings, all
information is strictly confidential to our client.

We have a situation with a small project we just completed. We detected the
presence of a toxic compound in product. While not the intended use, it is
conceivable that this product could be put into one's mouth which would
present a health concern.

Upon discovery of this compound, I called our client immediately and found
out that they submitted competitors' products. Our client is certainly
aware of this now, but they are not in a position to disclose to their
competitors that they were analyzing their products. Given that these
products are not intended to have oral contact, I doubt that the FDA has
any applicable regulations regarding the composition.

Any thoughts?

Alan Stone
ASTON Metallurgical Services

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Mon May 17 16:10:25 2004

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Dear Bryony,
The combined FE and ESED instruments are very pricey, expensive to maintain and,
since you already have a FE, perhaps a bit redundant. We have a two-year-old
tungsten variable-pressure and it is a popular workhorse that is in constant
use. It can do high resolution or ESED but not both at the same time. If you
need both at the same time, then you need FE-ESED. BTW, the thing we would most
like to have is a cold stage, to look at hydrated samples without having to go
to higher pressures.
Good luck.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Bryony James" {b.james-at-auckland.ac.nz}
To: {Microscopy-at-msa.microscopy.com}
Sent: Sunday, May 16, 2004 10:21 PM

Alan;

It sounds like you need legal advice and not scientific advice. You should consult with your corporate counsel on this issue.

Competitor analysis is done all the time and I don't see any issues with that. What you do with the data afterwards may be another matter and open to litigation so see the attorney.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: Alan Stone [mailto:as-at-astonmet.com]
Sent: Monday, May 17, 2004 2:47 PM
To: Microscopy-at-MSA.Microscopy.Com

We are an independent commercial lab serving general industry. Unless
directed by a court order or we suspect misuse of our findings, all
information is strictly confidential to our client.

We have a situation with a small project we just completed. We detected the
presence of a toxic compound in product. While not the intended use, it is
conceivable that this product could be put into one's mouth which would
present a health concern.

Upon discovery of this compound, I called our client immediately and found
out that they submitted competitors' products. Our client is certainly
aware of this now, but they are not in a position to disclose to their
competitors that they were analyzing their products. Given that these
products are not intended to have oral contact, I doubt that the FDA has
any applicable regulations regarding the composition.

Any thoughts?

Alan Stone
ASTON Metallurgical Services

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 07:02:20 2004

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Pavel;

If you really need a x-section without the issues with mechanical polishing, try using an FIB [Focused Ion Beam].

Peter

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Monday, May 17, 2004 9:07 AM
To: MicroscopyListServer (MicroscopyListServer)

Thank you all for the responses that I have received.

Just to clarify:
We had multiple field failures of the chips. The SEM examination
revealed some sort of coating on the fracture surfaces, which I believe is
the urethane coating. The transition from the side wall to the fracture
surface, on some of the chips, suggests that the chips could have had a
small cracks prior urethane coating.

Now, I am looking at the "Virgin" chips for any evidence of cracking
at the side wall and diaphragm transition, but my problem is that the Gold
coating does not coat the area well enough for me to resolve the crack. Due
to lack of coating that area is charging and I see only a black line.
I have coated it at least 3 times and rotate the chips to insure good
coatings in those areas, but it was not enough.

After SEM examination I would also like to cross section the chip to check
for the evidence of pre-cracks, but I am afraid to introduce the cracks
myself. Could you help me with a proper preparation procedure of the cross
sections? We have metallography lab. equipment and nothing special to
prepare the chip cross sections.

I have uploaded some more photos of the fracture surfaces of the failed
chips and Virgin chip that I am trying to image now.
http://www.atclabs.com/images/temp/MicrList_files/frame.htm

Sorry, it might be a little slow at showing the images due to their size.

Thanks for your help again,

Pavel

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]

What is the cross sectional construction like?
Is the die passivated? If it is, use MIL-STD-883 for
GLIT. If there is metal underneath the passivation,
and the passivation has voids, GLIT will show it
up big time. GLIT is glassivation layer integrity test.

gary g.

-----Original Message-----
} From: Warren E Straszheim [mailto:wesaia-at-iastate.edu]

Do you get charging at the crack due to a gap in the coating?
Otherwise,you should be able to see the break.

-----Original Message-----
} From: Jim Quinn [mailto:jquinn-at-www.matscieng.sunysb.edu]
Pavel

Your image is very low mag, so it is difficult to judge anything.

I suggest that you use a sacrificial chip and coat
it with about 10nm of gold. If your coater does not
rotate the sample, then you should manually rotate
the sample at 45 degrees atleast twice. This is
will help the gold to get into the perpendicular
surfaces.

Next use a Robinson BS detector. 10 or 15kV is sufficient.

Once you image the cracks, then you can go about
trying to image without the gold. Variable pressure
and voltage will reduce charging in uncoated samples.

JQ

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Pavel;

Having looked at more fractures in silicon and GaAs devices than I
care to remember, it's not generally a problem finding them and as
often with optical means as with EM.

If you would kindly provide the list with more specifics about your
samples and the nature of these "cracks?" That is, are they along
crystal planes or fractures that travel at random angles with respect to
the surface? Fractures, or cleaves perpendicular to the die surface, are
difficult to detect with EM but apparent with visible light microscopy.
How separated are both sides of the crack and why do you need to see into
them? Sounds like you only need to identify whether they exist or not.
How long are the cracks?

I have plenty of EM's I'd be happy to send you images of samples
that have fractured for various reasons, and there are multiple root
causes of this failure mechanism. I'm sure if you provide a little more
detail you'll get plenty of good suggestions on how to image your
samples.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: AtcSEM [mailto:atcsem-at-sbcglobal.net]
Sent: Friday, May 14, 2004 4:10 PM
To: MicroscopyListServer (MicroscopyListServer)

Dear microscopy experts I need your expertise.

We are evaluation transducer chips and suspecting that the chips have
pre-cracks forming between the side wall and the diaphragm. The problem: if
we do have a some sort of crack forming the gold coating, that I coat chips
for analysis, does not get inside the crack, so it's hard to prove if there
is any cracks or not. Do you have any suggestions how to show if there is
any cracks.

The arrows in the picture show the location of possible cracks.
http://www.atclabs.com/images/%231.jpg

Thanks,
Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 07:15:34 2004

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Hello,
We want to image, by SEM, the surface of a HfO2 layer deposited on Si.
Is there a method to reveal the structure of the layer ?
for instance chemical etching or others....
We have tried on the as grown layer but we can see nothing, the image is
very smooth. By means of X-ray diffraction we know that
we have very small crystals, just a few nanometers. Now we wonder wether
there are larger structures than the crystals. We expect
something like polycrystalline grains...
Thank you for your help
Regards

--
Claude GRATTEPAIN / Bernard SERVET

THALES R & T France Tel : (+33 1) 69.33.91.13
Domaine de Corbeville Fax : (+33 1) 69.33.07.40

91404 Orsay Cedex, France mailto:claude.grattepain-at-thalesgroup.com
_____________________________________________________________________

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intended
recipient, please notify us immediately, send this message back to us
and
destroy it. You are hereby notified that any review, dissemination,
distribution, copying or otherwise use of this e-mail/fax is strictly
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From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:17:11 2004

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Dear All

We would like to get a centrifuge to separate viruses. What are you using in your TEM laboratory?
Suggestions and hints will be helpful.
Thanks

Since my UB mail address is not reliable please send
a copy of all urgent mail to

coetzeesh-at-yahoo.co.uk

Mr S. H. Coetzee
Electron Microscope Unit
University of Botswana
Private Bag 0022
Gaborone
Botswana
Phone : +267 355 2462/5222
Mobile : +267 714 55701 (Now active)
Fax : +267 318 5097
e-mail : coetzees-at-mopipi.ub.bw

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:46:08 2004

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Hello Listers,

I wanted to see if anyone has had any experience scanning negatives with the Canon Canoscan 9900F.
I have a low end Canoscan that I use for documents and the occasional photograph, which has given me
very good results, but is not set up for negatives. I have seen the recent posts about the Epson scanner,
but I am trying to keep it under a $1000 so that I do not have to treat it as a capital purchase. I have tried
for the last two years to get a Coolscan 8000 on the capital budget with no luck, and do not see any scanner
above $1000 as an option right now.

Thanks,
Steve

Steven Lee
Chief Technologists
Electron Microscopy Laboratory
Baylor University Medical Center
3500 Gaston Ave
Dallas, TX 750246
Ph: 214.820.3302
Fx: 214.820.4110
Em: stevenle-at-baylorhealth.edu

This e-mail, facsimile, or letter and any files or attachments transmitted with it contains information that is confidential and privileged. This information is intended only for the use of the individual(s) and entity(ies) to whom it is addressed. If you are the intended recipient, further disclosures are prohibited without proper authorization. If you are not the intended recipient, any disclosure, copying, printing, or use of this information is strictly prohibited and possibly a violation of federal or state law and regulations. If you have received this information in error, please notify Baylor Health Care System immediately at 1-866-402-1661 or via e-mail at privacy-at-baylorhealth.edu. Baylor Health Care System, its subsidiaries, and affiliates hereby claim all applicable privileges related to this information.

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:47:42 2004

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In my experience medium/high magnifications for wet
specimens are limited mostly by specimens themselves and not by a
type of emitter. While I can get a nice picture of gold on carbon
at x100k, for most of my "real life" specimens magnification is
limited by x20k (or less).

Vladimir

} We look mostly at hydrated biological samples. We have a
} tungsten gun XL30 ESEM TMP. For looking at bacteria and
} cells a FEGESEM would be superior in terms of reduced
} damage and improved resolution. I find it hard to get
} medium/high resolution with wet biological samples. I feel
} FEGESEM would make this a lot easier.
}
} Dave
}
} On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} {b.james-at-auckland.ac.nz} wrote:
}
} }
} }
} }
} ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} -----------------
} }
} } Hello listers,
} }
} } We are in the process of justifying, to the University, a
} proposal to
} } purchase an ESEM. In prepapring the business case I am
} including the
} } ten year financials for both FEG and Tungtsen filament
} machines. Given
} } that we have to break even in that time, including covering our
} } depreciation, the Tungsten instrument is easier to justify
} in a purely
} } financial sense.
} }
} } From a scientific and operational viewpoint, though, I was hoping
} } some
} } of you could provide opinions on the relative merits of
} Tungsten or FEG.
} } Our current conventional SEM is a Philips XL-30 S-FEG so we
} already know
} } of the costs associated with the emitter.
} }
} } The range of samples we will be required to put in our ESEM will be
} } anything you oculd possibly imagine from the Faculties of
} Engineering,
} } Science and Medicine. Samples will inlcude food materials
} (big dairy
} } industry in New Zealand), polymers, conducting polymers, mammalian
} } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } ceramic coatings and bees knees. We will definitely need a
} hot-stage.
} }
} } If you would like to contact me off list with your opinions please
} } feel
} } free.
} }
} } Kind regards
} } Bryony James
} } Research Centre for Surface and Materials Science
} } Univetrsity of Auckland
} } New Zealand
} }
} }
} }
} } This incoming email to UWE has been independently scanned
} for viruses
} } and any virus detected has been removed using McAfee anti-virus
} } software
} }
}
} ----------------------------------------
} Patton, David
} Email: David.Patton-at-uwe.ac.uk
} "University of the West of England"
}
}
}
} This email has been independently scanned for viruses and any
} virus detected has been removed using McAfee anti-virus software
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 08:51:20 2004

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Try EBSD. It will tell if you have grains
or if the layer is amorphous.

gary g.

At 05:24 AM 5/18/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 09:16:24 2004

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Depressing isn't it? I usually give up with cultured
cells and look at them after drying with HMDS and gold
coating. Have you (or anyone out there) ever taken/seen a
good picture of a hydrated cultured cell at x20,000 or
higher?

Dave

On Tue, 18 May 2004 08:55:19 -0500 "Dusevich, Vladimir"
{DusevichV-at-umkc.edu} wrote:

} In my experience medium/high magnifications for wet
} specimens are limited mostly by specimens themselves and not by a
} type of emitter. While I can get a nice picture of gold on carbon
} at x100k, for most of my "real life" specimens magnification is
} limited by x20k (or less).
}
} Vladimir
}
} } We look mostly at hydrated biological samples. We have a
} } tungsten gun XL30 ESEM TMP. For looking at bacteria and
} } cells a FEGESEM would be superior in terms of reduced
} } damage and improved resolution. I find it hard to get
} } medium/high resolution with wet biological samples. I feel
} } FEGESEM would make this a lot easier.
} }
} } Dave
} }
} } On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} } {b.james-at-auckland.ac.nz} wrote:
} }
} } }
} } }
} } }
} } ----------------------------------------------------------------------
} } } --------
} } } The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America
} } } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } --------------------------------------------------------------
} } -----------------
} } }
} } } Hello listers,
} } }
} } } We are in the process of justifying, to the University, a
} } proposal to
} } } purchase an ESEM. In prepapring the business case I am
} } including the
} } } ten year financials for both FEG and Tungtsen filament
} } machines. Given
} } } that we have to break even in that time, including covering our
} } } depreciation, the Tungsten instrument is easier to justify
} } in a purely
} } } financial sense.
} } }
} } } From a scientific and operational viewpoint, though, I was hoping
} } } some
} } } of you could provide opinions on the relative merits of
} } Tungsten or FEG.
} } } Our current conventional SEM is a Philips XL-30 S-FEG so we
} } already know
} } } of the costs associated with the emitter.
} } }
} } } The range of samples we will be required to put in our ESEM will be
} } } anything you oculd possibly imagine from the Faculties of
} } Engineering,
} } } Science and Medicine. Samples will inlcude food materials
} } (big dairy
} } } industry in New Zealand), polymers, conducting polymers, mammalian
} } } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } } ceramic coatings and bees knees. We will definitely need a
} } hot-stage.
} } }
} } } If you would like to contact me off list with your opinions please
} } } feel
} } } free.
} } }
} } } Kind regards
} } } Bryony James
} } } Research Centre for Surface and Materials Science
} } } Univetrsity of Auckland
} } } New Zealand
} } }
} } }
} } }
} } } This incoming email to UWE has been independently scanned
} } for viruses
} } } and any virus detected has been removed using McAfee anti-virus
} } } software
} } }
} }
} } ----------------------------------------
} } Patton, David
} } Email: David.Patton-at-uwe.ac.uk
} } "University of the West of England"
} }
} }
} }
} } This email has been independently scanned for viruses and any
} } virus detected has been removed using McAfee anti-virus software
} }
} }
} }
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 10:42:01 2004

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When choosing a scanner for negatives, an important parameter is the Dmax
(which is a log value so relatively small differences can be
significant). The Dmax needed for negs is a lot more than for most printed
images or documents.

At 08:55 AM 5/18/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 11:16:44 2004

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I agree that resolution is more dependent on sample than microscope. What a
microscope is capable of doing with an "ideal" sample often does not relate
to the real world of biological samples which are anything but ideal!

To get really good resolution you need to use higher kV values. These same
values will result in the primary electrons penetrating too far into the low
density biological sample resulting in substantial loss of signal in general
and se1 & se2's in particular. Resulting image will be low resolution and
often of much lesser quality than the same sample taken at a lower
magnification.

The problem of kV can be partially overcome by using a more coherent
beam with greater beam density, i.e. Field Emission. FE allows one to work
at lower kV values resulting in a se yield that is still adequate while
minimizing sample damage. Resulting images are likely to be higher
resolution (sharper with more detail) than comparable images at similar kVs
from a tungsten instrument.

However, there is a point where you go from useful magnification to
"empty " magnification regardless of the gun type. This is sample dependent
and must be determined accordingly. So it is unlikely that you will get any
additional information from a bacteria sample at 100k than at say 50K.
However you will most likely get a much sharper image at 20k with FE than
you could with a W filament.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 5/18/04 8:55 AM, "Dusevich, Vladimir" {DusevichV-at-umkc.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--}
-
}
} In my experience medium/high magnifications for wet
} specimens are limited mostly by specimens themselves and not by a
} type of emitter. While I can get a nice picture of gold on carbon
} at x100k, for most of my "real life" specimens magnification is
} limited by x20k (or less).
}
} Vladimir
}
} } We look mostly at hydrated biological samples. We have a
} } tungsten gun XL30 ESEM TMP. For looking at bacteria and
} } cells a FEGESEM would be superior in terms of reduced
} } damage and improved resolution. I find it hard to get
} } medium/high resolution with wet biological samples. I feel
} } FEGESEM would make this a lot easier.
} }
} } Dave
} }
} } On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} } {b.james-at-auckland.ac.nz} wrote:
} }
} } }
} } }
} } }
} } ----------------------------------------------------------------------
} } } --------
} } } The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America
} } } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } --------------------------------------------------------------
} } -----------------
} } }
} } } Hello listers,
} } }
} } } We are in the process of justifying, to the University, a
} } proposal to
} } } purchase an ESEM. In prepapring the business case I am
} } including the
} } } ten year financials for both FEG and Tungtsen filament
} } machines. Given
} } } that we have to break even in that time, including covering our
} } } depreciation, the Tungsten instrument is easier to justify
} } in a purely
} } } financial sense.
} } }
} } } From a scientific and operational viewpoint, though, I was hoping
} } } some
} } } of you could provide opinions on the relative merits of
} } Tungsten or FEG.
} } } Our current conventional SEM is a Philips XL-30 S-FEG so we
} } already know
} } } of the costs associated with the emitter.
} } }
} } } The range of samples we will be required to put in our ESEM will be
} } } anything you oculd possibly imagine from the Faculties of
} } Engineering,
} } } Science and Medicine. Samples will inlcude food materials
} } (big dairy
} } } industry in New Zealand), polymers, conducting polymers, mammalian
} } } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } } ceramic coatings and bees knees. We will definitely need a
} } hot-stage.
} } }
} } } If you would like to contact me off list with your opinions please
} } } feel
} } } free.
} } }
} } } Kind regards
} } } Bryony James
} } } Research Centre for Surface and Materials Science
} } } Univetrsity of Auckland
} } } New Zealand
} } }
} } }
} } }
} } } This incoming email to UWE has been independently scanned
} } for viruses
} } } and any virus detected has been removed using McAfee anti-virus
} } } software
} } }
} }
} } ----------------------------------------
} } Patton, David
} } Email: David.Patton-at-uwe.ac.uk
} } "University of the West of England"
} }
} }
} }
} } This email has been independently scanned for viruses and any
} } virus detected has been removed using McAfee anti-virus software
} }
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 18 11:19:50 2004

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I haven't tried the scanners you mentioned but you may want to check out this April 2004 review article in PCWorld online:

http://www.pcworld.com/reviews/article/0,aid,115075,00.asp

Gene P. Young
Sr. Analytical Technologist
Analytical Sciences, Polymer Characterization

The Dow Chemical Company
2301 N. Brazosport Blvd., B-1470
Freeport, Texas 77541-3257
Fax: (979) 238-0095

*(979) 238-1579 * gpyoung-at-dow.com

****************************************
Original message:

Hello Listers,

I wanted to see if anyone has had any experience scanning negatives with the Canon Canoscan 9900F.
I have a low end Canoscan that I use for documents and the occasional photograph, which has given me very good results, but is not set up for negatives. I have seen the recent posts about the Epson scanner, but I am trying to keep it under a $1000 so that I do not have to treat it as a capital purchase. I have tried for the last two years to get a Coolscan 8000 on the capital budget with no luck, and do not see any scanner above $1000 as an option right now.

Thanks,
Steve

Steven Lee
Chief Technologists
Electron Microscopy Laboratory
Baylor University Medical Center
3500 Gaston Ave
Dallas, TX 750246
Ph: 214.820.3302
Fx: 214.820.4110
Em: stevenle-at-baylorhealth.edu

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 02:44:19 2004

Contents Retrieved from Microscopy Listserver Archives
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}
} IbPRIA'2005
}
} 2nd Iberian Conference on Pattern Recognition and Image Analysis
}
} June 7-9, 2005 - Estoril, Portugal
}
} http://ibpria2005.isr.ist.utl.pt
}
}
} =================
} ABOUT IbPRIA'2005
} =================
} IbPRIA'2005 is the second edition of the Iberian Conference on Pattern
} Recognition and Image Analysis and will be held in Estoril (Portugal)
} in June 7-9, 2005.
}
} IbPRIA is an international event co-organised every two years, by the
} Spanish and Portuguese Associations for Pattern Recognition (AERFAI
} and APRP). Its mission is to bring together researchers from all over
} the world working in Pattern Recognition and in all areas of Video,
} Image and Signal Processing. Participants will have the opportunity to
} meet colleagues working in these areas, to attend oral sessions and to
} exchange ideas during poster sessions.
}
} IbPRIA'2005 is sponsored by IAPR-International Association for Pattern
} Recognition and the conference proceedings are planned to be published
} by Springer in LNCS series.
}
} ======
} TOPICS
} ======
} The topics of the conference include, but are not limited to:
}
} - Pattern Recognition
} - Image Analysis
} - Computer Vision
} - Multimedia Systems
} - Statistical & Structural Pattern Recognition
} - Neural Networks
} - Bioinformatics
} - Image Coding and Processing
} - Shape and Texture Analysis
} - Biomedical Pattern Analysis
} - Information Systems
} - Speech Recognition
} - Natural Language Analysis
} - Document Processing
} - Robotics
} - Remote Sensing
} - Industrial Applications of Pattern Recognition
} - Special Hardware Architectures
}
} =================
} PROGRAM COMMITTEE
} =================
} Jake Aggarwal, University of Texas, USA
} José Benedi, Polyt. University of Valencia, Spain
} Isabelle Bloch, ENST, France
} Hervé Bourlard, EPFL, Switzerland
} Patrick Bouthemy, IRISA, France
} Horst Bunke, University of Bern, Switzerland
} Aurélio Campilho, University of Porto, Portugal
} Gilles Celeux, Université Paris-Sud, France
} Luigi Cordella, University of Napoles, Italy
} Alberto Del Bimbo, University of Firenze, Italy
} Hervé Delinguette, INRIA, France
} Rachid Deriche, INRIA, France
} José Dias, Instituto Superior Técnico, Portugal
} Robert Duin, University of Delft, The Netherlands
} Mário Figueiredo, Instituto Superior Técnico, Portugal
} Ana Fred, Instituto Superior Técnico, Portugal
} Andrew Gee, University of Cambridge, UK
} Mohamed Kamel, University of Waterloo, Canada
} Aggelos Katsaggelos, Northwestern University, USA
} Joseph Kittler, University of Surrey, UK
} Seong-Whan Lee, University of Korea, Korea
} Ana Mendonça, University of Porto, Portugal
} Hermann Ney, University of Aachen, Germany
} Wiro Niessen, University of Utrecht, The Netherlands
} Maria Petrou, University of Surrey, UK
} Armando Pinho, University of Aveiro, Portugal
} Ioannis Pitas, University of Tessaloniki, Greece
} Filiberto Pla, University Jaume I, Spain
} Richard Prager, University of Cambridge, UK
} José Principe, University of Florida, USA
} Ian Reid, University of Oxford, UK
} Gabriella Sanniti di Baja, Istituto di Cibernética, Italy
} Beatriz Santos, University of Aveiro, Portugal
} Jose Santos-Victor, Inst. Superior Técnico, Portugal
} Joan Serrat, Aut. University of Barcelona, Spain
} Yoshiaki Shirai, Osaka University, Japan
} Pierre Soille, Joint Research Centre, Italy
} Karl Tombre, LORIA, France
} M. Ines Torres, Univ. of the Basque Country, Spain
} Emmanuele Trucco, Heriot-Watt University, UK
} Alessandro Verri, University of Genova, Italy
} Max Viergever, University of Utrecht, The Netherlands
} Joachim Weickert, Saarland University, Germany
}
} ======
} CHAIRS
} ======
} GENERAL CO-CHAIRS:
} Jorge S. Marques (Instituto Superior Técnico, Portugal)
} Nicolás Pérez de la Blanca (University of Granada, Spain)
}
} LOCAL CHAIR:
} Pedro Pina (Instituto Superior Técnico, Portugal)
}
} ====================
} ORGANISING COMMITTEE
} ====================
} Joăo Sanches, Joăo Paulo Costeira, Teresa Barata, Vitorino Ramos,
} José Saraiva, Michele Mengucci, Fernando Soares
}
}
} ===================================
} PAPER SUBMISSION AND REVIEW PROCESS
} ===================================
} Papers should describe original and unpublished work on the topics of
} the conference. Prospective authors should prepare a full paper,
} written in english, not exceeding 8 pages and must submit it
} electronically.
}
} All manuscripts will be blind-reviewed by at least two members of the
} program committee. Accepted papers are intended to appear in the
} Springer LNCS series which will be distributed to all participants at
} the Conference.
}
} Submission implies that at least one of the authors has to register
} and to present the communication at the conference if the paper is
} accepted.
}
} ===============
} IMPORTANT DATES
} ===============
} Submission of papers : Noverber 12, 2004
} Notification of acceptance: January 7, 2005
} Camera-ready : January 30, 2005
} Early registration : April 7, 2005
} Conference : June 7-9, 2005
}
} =====
} VENUE
} =====
} The conference will take place in Estoril, a beautiful village located
} at about 20 km of Lisbon centre.
}
} The conference will be held at a four star hotel (Hotel Eden), that
} disposes of adequate facilities for workshops and conferences.
}
} The international airport of Lisbon is about 40 minutes from the
} venue. There is a direct bus-shuttle from/to the airport to the Hotel
} every hour. Alternatively, participants can also easily reach the
} venue by train, car or taxi.
}
} ========
} CONTACTS
} ========
} IbPRIA'2005 Secretariat
} CVRM / Geo-Systems Centre
} Instituto Superior Técnico
} Av. Rovisco Pais
} 1049-001 Lisboa
} PORTUGAL
}
} URL : http://ibpria2005.isr.ist.utl.pt
} e-mail: ibpria2005-at-isr.ist.utl.pt
} Tel : +351-218417438
} Fax : +351-218417442
}

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 10:22:00 2004

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Fellow Listmembers,

Members in the Greater Orlando, Florida area are cordially invited to attend
a two day mini-workshop on "Cryomicrotomy and Cryoultramicrotomy for Materials
Sciences."

When:
Tuesday, June 8 and Wednesday, June 9, 2004, 9:00am-4:00pm

Where:
Room 101, Materials Characterization Facility
Advanced Materials Processing & Analysis Center
University of Central Florida
12443 Research Parkway
Orlando, FL 32826

What:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryomicrotomy and cryoultramicrotomy, including toolmaking (wire loops
and hair probes), glass knife making, evaluation of glass knives, care and
cleaning of diamond knives and operation of the cryomicrotome and
cryoultramicrotome.

Background:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing" at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

Important Info:
There is no charge for this workshop.
Meals and refreshments will be served!
Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryosectioning hands-on
sessions on the second day.

Contacts:
To RSVP and to reserve a spot for the hands-on sessions, please contact
either Ms. Kim Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} ,
800.552.2262) or Ms. Nancy Crouch at ICMAS, Inc. ( {nancy-at-icmas.com} , 865.984.8058)

Sponsors and Organizers:
University of Central Florida
Advanced Materials Processing & Analysis Center
Materials Characterization Facility
RMC Products Group, Boeckeler Instruments, Inc.

Hope to see you there!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 10:32:23 2004

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For ESEM in wet mode low voltage beam is not suitable,
even at 5 kV noise level is too high.

Vladimir

} I agree that resolution is more dependent on sample than
} microscope. What a microscope is capable of doing with an
} "ideal" sample often does not relate to the real world of
} biological samples which are anything but ideal!
}
} To get really good resolution you need to use higher kV
} values. These same values will result in the primary
} electrons penetrating too far into the low density biological
} sample resulting in substantial loss of signal in general and
} se1 & se2's in particular. Resulting image will be low
} resolution and often of much lesser quality than the same
} sample taken at a lower magnification.
}
} The problem of kV can be partially overcome by using a
} more coherent beam with greater beam density, i.e. Field
} Emission. FE allows one to work at lower kV values resulting
} in a se yield that is still adequate while minimizing sample
} damage. Resulting images are likely to be higher resolution
} (sharper with more detail) than comparable images at similar
} kVs from a tungsten instrument.
}
} However, there is a point where you go from useful
} magnification to "empty " magnification regardless of the gun
} type. This is sample dependent and must be determined
} accordingly. So it is unlikely that you will get any
} additional information from a bacteria sample at 100k than at
} say 50K. However you will most likely get a much sharper
} image at 20k with FE than you could with a W filament.
}
} Debby
}
}
}
} Debby Sherman, Manager Phone: 765-494-6666
} Life Science Microscopy Facility FAX: 765-494-5896
} Purdue University E-mail: dsherman-at-purdue.edu
} S-052 Whistler Building
} 170 S. University Street
} West Lafayette, IN 47907 http://www3.agriculture.purdue.edu/microscopy
}
}
} On 5/18/04 8:55 AM, "Dusevich, Vladimir" {DusevichV-at-umkc.edu} wrote:
}
} }
} }
} }
} ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} --------------
} --}
} -
} }
} } In my experience medium/high magnifications for wet specimens are
} } limited mostly by specimens themselves and not by a type of
} emitter.
} } While I can get a nice picture of gold on carbon at x100k,
} for most of
} } my "real life" specimens magnification is limited by x20k (or less).
} }
} } Vladimir
} }
} } } We look mostly at hydrated biological samples. We have a tungsten
} } } gun XL30 ESEM TMP. For looking at bacteria and cells a
} FEGESEM would
} } } be superior in terms of reduced damage and improved resolution. I
} } } find it hard to get medium/high resolution with wet biological
} } } samples. I feel FEGESEM would make this a lot easier.
} } }
} } } Dave
} } }
} } } On Mon, 17 May 2004 17:21:33 +1200 Bryony James
} } } {b.james-at-auckland.ac.nz} wrote:
} } }
} } } }
} } } }
} } } }
} } }
} ---------------------------------------------------------------------
} } } -
} } } } --------
} } } } The Microscopy ListServer -- Sponsor: The Microscopy
} } } Society of America
} } } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } } On-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } }
} } } --------------------------------------------------------------
} } } -----------------
} } } }
} } } } Hello listers,
} } } }
} } } } We are in the process of justifying, to the University, a
} } } proposal to
} } } } purchase an ESEM. In prepapring the business case I am
} } } including the
} } } } ten year financials for both FEG and Tungtsen filament
} } } machines. Given
} } } } that we have to break even in that time, including covering our
} } } } depreciation, the Tungsten instrument is easier to justify
} } } in a purely
} } } } financial sense.
} } } }
} } } } From a scientific and operational viewpoint, though, I
} was hoping
} } } } some of you could provide opinions on the relative merits of
} } } Tungsten or FEG.
} } } } Our current conventional SEM is a Philips XL-30 S-FEG so we
} } } already know
} } } } of the costs associated with the emitter.
} } } }
} } } } The range of samples we will be required to put in our
} ESEM will be
} } } } anything you oculd possibly imagine from the Faculties of
} } } Engineering,
} } } } Science and Medicine. Samples will inlcude food materials
} } } (big dairy
} } } } industry in New Zealand), polymers, conducting polymers,
} mammalian
} } } } tissue, bacteria, fruit and veg, fish and chips, superconductors,
} } } } ceramic coatings and bees knees. We will definitely need a
} } } hot-stage.
} } } }
} } } } If you would like to contact me off list with your
} opinions please
} } } } feel free.
} } } }
} } } } Kind regards
} } } } Bryony James
} } } } Research Centre for Surface and Materials Science Univetrsity of
} } } } Auckland New Zealand
} } } }
} } } }
} } } }
} } } } This incoming email to UWE has been independently scanned
} } } for viruses
} } } } and any virus detected has been removed using McAfee anti-virus
} } } } software
} } } }
} } }
} } } ----------------------------------------
} } } Patton, David
} } } Email: David.Patton-at-uwe.ac.uk
} } } "University of the West of England"
} } }
} } }
} } }
} } } This email has been independently scanned for viruses and
} any virus
} } } detected has been removed using McAfee anti-virus software
} } }
} } }
} } }
} }
} }
} }
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 14:24:44 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Fellow Listmembers,

Members in the Greater Madison, Wisconsin area are cordially invited to
attend a two day mini-workshop on "Cryoultramicrotomy for Materials Sciences."

When:
Wednesday, June 2 and Thursday, June 3, 2004, 9:00am-4:00pm

Where:
Room 374, Truax Building
Madison Area Technical College
3550 Anderson Street
Madison, WI 53704

(Gated lot near Truax Bldg. has audio to Parking Department. Mention this
Workshop for entrance to parking lot. Enter left side of building, take main
elevator to third floor)

What:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair probes),
glass knife making, evaluation of glass knives, care and cleaning of diamond
knives and operation of the cryomicrotome and cryoultramicrotome.

Background:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing" at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

Important Info:
There is no charge for this workshop.
Meals and refreshments will be served!
Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryosectioning hands-on
sessions on the second day.

Contacts:
To RSVP and to reserve a spot for the hands-on sessions, please contact
either Kim Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262)
or Michael Kostrna at Madison Area Technical College
( {mkostrna-at-matcmadison.edu} , 608.246.6762).

Sponsors and Organizers:
Madison Area Technical College
(Electron Microscopy)
RMC Products Group, Boeckeler Instruments, Inc.
Doug D'Arcy, Midwest Regional Representative

See you in Madison!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 17:00:14 2004

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Hello Fellow List Members,

Iąd appreciate your collective wisdom and experiences for a project Iąm
starting. I need to create high resolution (250 Mb minimum) photo files of
current microprocessor die faces (pentium 4 type) to show the circuitry and
traces with as much detail as possible. Iąd like to do this using my Nikon
Optiphot and a yet to be purchased motorized positionable stage with
automation software to include my Fuji S2 still camera (34 Mb sized files
per image) with image stitching as an added option. I have extensive
experience in Photoshop and would use that to stitch the images if the
automation software package doesnąt include that. The stage travel only
needs to be about 3" (75mm) in the X and Y dimensions.

Iąve been reading about some of the software programs available to help
accomplish this. Iąve come across Image-Pro Plus with the Scope-Pro plugin
and the software program Metamorph in my Google searches. I donąt need
extensive filtering or analysis functions in the software, just the ability
to create multiple, tileable images in a repeatable manner.

What economical software and hardware (such as the MultiScan-4 Low Cost
Scanning Stage for example) do you have experience with in similar projects?

Do any of you have an older version of Image Pro Plus or similar software
program that is sitting abandoned and alone on a shelf that needs a new
home? How about a used basic scanning stage thatąs collecting dust?

Any and all advice would be appreciated. You can email me off-list if thatąs
easier.

Thanks,
Doug Baldwin
Baldwin Hi-Tech Photography
dougbaldwin-at-mindspring.com

From MicroscopyL-request-at-ns.microscopy.com Wed May 19 19:03:05 2004

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The P4 BGA devices are like PPC G3, G4 and G5
products and are flip chip BGAs. Between the
inverted die and the multi layer ceramic package
is a thin layer of silicone. Through this layer
are many (700+) solder vias between the die and
package. Once the silicone is removed (and assuming
that you get the die off), the top layer greatly
masks the underlying 5-8 layers (depending on part
timeframe of manufacture) since it is used for interface
to the ceramic package.

This top-most layer must be removed to begin to
get at the actual interconnect layers. Once removed,
the underlying layers can be exposed by plasma
depassivation. Or, you can try wet etching.

These types of processors are face down rather than
face up. This is because they are too hot compared
to earlier CPUs.

The other factor is that you do not need high rez
image segments to make a high rez final image. To get
any reasonable image detail, you will likely need to
shoot at 500X or 1000X. At these mags, your field of
view is somewhere around 300u (guessing). For a 0.5cm
die, you will likely take 1,000 images (guessing again).
You can do the math. The point is that for a final high
rez image, it is made up of many low rez image segments.
The other problem you will face at high mag is the problem
of low DOF. The solution is to shoot with a SEM at high
tilt angle and dynamic focus. Then colorize the image.

If you need motorized and programmed stage movement,
Prior E103 is a good candidate and Soft Imaging analySIS
Opti is a good driving software product. Neither of
these items are free.

Anyway, I have found that it is not worth the effort.
But of course, YMMV.

gary g.

At 03:07 PM 5/19/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 04:11:37 2004

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Doug

given the complexity of what you are doing, would it not be possible to try another method. If the die faces are flat and of the right size, why not just use a very high resolution flat bed scanner and do the whole thing in one go.

I'm sure that HP, Epson, Canon all do better than 3000dpi (optical resolution. It might certainly be worth investigating if camera photography involves a horrendous amount of image stitching (especially given the edge distortion in even the best camera). The only problems may be the reflective light quality of the scanner or how much depth of field there would be in a scanner image if the die has lots of depth to its layers.

My apologies if I've missed some technical point.

Malc

Malcolm Haswell
e.m. unit
University of Sunderland
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Doug Baldwin {dougbaldwin-at-mindspring.com}

My thanks to everyone who replied to my legal/ethics query. After my
client became a bit more educated regarding the health risk we discovered
and checked with their counsel, they will do the right thing. The twist
here was that they were analyzing competitors' products which are made
overseas, so there are issues of diplomacy.

Alan Stone

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 09:52:22 2004

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Hi All,

I wish to set up a logging system to record instrument use.
Ideally it would log date and time users start and
finish work on a particular project on each of our
instruments so that we can assess use of our facility.

At present users fill in a log book when they use an
instrument. It is easy to get general data (25 sessions to
the page gives an idea of instrument use but not user). I
don't want to waste time transcribing the data from the 20
instrument log books into a computer. Neither do I want to
spend a lot of money on each machine to gather the
information, however, most machines already have a PC
attached running the instrument or some ancillary equipment
and these are all networked.

What systems are being used at other sites? Any suggestions
of inexpensive systems that would work on two sites 6 miles
apart?

Regards,
Ron

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 15:49:26 2004

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Hello Everyone
We have a Nonotech Semprep2 sputter coater which is so old the
company no longer exists. The glass cylinder has now got one more
gouge in it and it will have to lose at least 3 cm to grind it out.
Does anyone have any experience with where to buy a new glass
cylinder?

Many thanks
Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 17:26:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mocherla-at-eng.fsu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, May 20, 2004 at 10:43:53
---------------------------------------------------------------------------

Email: mocherla-at-eng.fsu.edu
Name: supriya

Organization: FSU

Title-Subject: [Microscopy] [Filtered] Liposome Grids

Question: Dear authors,

I really appreciate this group for their support in my work.

I observed that for negative staining, carbon coated Formvar grid was used mostly. I would like to know if there is any significance in using this particlular grid or Can I use Carbon support film on Copper or Gold grid.

Thanks!!

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 19:24:44 2004

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On May 20, 2004, at 3:35 PM, by way of MicroscopyListserver wrote:

} Title-Subject: [Microscopy] [Filtered] Liposome Grids
}
} Question: Dear authors,
}
} I really appreciate this group for their support in my work.
}
} I observed that for negative staining, carbon coated Formvar grid was
} used mostly. I would like to know if there is any significance in
} using this particlular grid or Can I use Carbon support film on Copper
} or Gold grid.
}
Dear Supriya,
The grids most often used for negative staining are copper grids on
which there is a layer of formvar and usually an additional layer of
carbon. These are often referred to as carbon-formvar grids or
carbon-coated formvar grids. It is much easier to use a carbon-formvar
support film than to use just a carbon film for support. The resulting
film is much stronger than plain carbon, and does not degrade the
images of negatively stained preps. The web sites of several of the EM
supply companies describe their carbon-formvar grids.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 20:04:13 2004

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Malcolm,

Interestingly, I had the same thought and tried this technique. I stopped by
one of the area's premier graphics arts service bureaus with an 8000+ dpi
flat bed scanner. We put the open faced CPU chip on the glass and proceeded
to scan it. It was awful. The main problem was that the light source on the
scanner was off-axis to the scanning array. This renders the face of the
chip dark and worthless.

Photos of microprocessors benefit from coaxial lighting since the metal
parts and traces reflect the light straight back to the lens and light
source. Lighting that's even slightly off-axis shows a marked drop off in
detail and reflectivity of the die faces.

The high dpi flat bed scanners are set up for flat artwork such as paintings
and drawings where side lighting is fine for rendering all the detail but
not for reflective metal parts.

Doug

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Doug
}
} given the complexity of what you are doing, would it not be possible to try
} another method. If the die faces are flat and of the right size, why not just
} use a very high resolution flat bed scanner and do the whole thing in one go.
}
} I'm sure that HP, Epson, Canon all do better than 3000dpi (optical resolution.
} It might certainly be worth investigating if camera photography involves a
} horrendous amount of image stitching (especially given the edge distortion in
} even the best camera). The only problems may be the reflective light quality
} of the scanner or how much depth of field there would be in a scanner image if
} the die has lots of depth to its layers.
}
} My apologies if I've missed some technical point.
}
} Malc
}
} Malcolm Haswell
} e.m. unit
} University of Sunderland
} UK
} e-mail: malcolm.haswell-at-sunderland.ac.uk
}
}
}
}
} ----- Original Message -----
} } From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} Date: Wednesday, May 19, 2004 11:07 pm
} Subject: [Microscopy] Hi-Res Microprocessor Photos
}
} }
} }
} } -------------------------------------------------------------------
} } -----------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } AmericaTo Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } -------------------------------------------------------------------
} } ----
} }
} } Hello Fellow List Members,
} }
} } IŹd appreciate your collective wisdom and experiences for a
} } project IŹm
} } starting. I need to create high resolution (250 Mb minimum) photo
} } files of
} } current microprocessor die faces (pentium 4 type) to show the
} } circuitry and
} } traces with as much detail as possible. IŹd like to do this using
} } my Nikon
} } Optiphot and a yet to be purchased motorized positionable stage with
} } automation software to include my Fuji S2 still camera (34 Mb
} } sized files
} } per image) with image stitching as an added option. I have extensive
} } experience in Photoshop and would use that to stitch the images if the
} } automation software package doesnŹt include that. The stage travel
} } onlyneeds to be about 3" (75mm) in the X and Y dimensions.
} }
} } IŹve been reading about some of the software programs available to
} } helpaccomplish this. IŹve come across Image-Pro Plus with the
} } Scope-Pro plugin
} } and the software program Metamorph in my Google searches. I donŹt need
} } extensive filtering or analysis functions in the software, just
} } the ability
} } to create multiple, tileable images in a repeatable manner.
} }
} } What economical software and hardware (such as the MultiScan-4 Low
} } CostScanning Stage for example) do you have experience with in
} } similar projects?
} }
} } Do any of you have an older version of Image Pro Plus or similar
} } softwareprogram that is sitting abandoned and alone on a shelf
} } that needs a new
} } home? How about a used basic scanning stage thatŹs collecting dust?
} }
} } Any and all advice would be appreciated. You can email me off-list
} } if thatŹs
} } easier.
} }
} } Thanks,
} } Doug Baldwin
} } Baldwin Hi-Tech Photography
} } dougbaldwin-at-mindspring.com
} }
} }
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 22:16:30 2004

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There is a photographer here in Oz who produces absolutely brilliant images
by scanning objects on a flat-bed scanner. They are very high resolution,
look as good as the images of leaves, flowers, insects (even very shiny
ones) we get using a good digital camera - Olympus DP70 or ProgRes or
similar, on a dissecting microscope. He's developed some ways of using the
scanner to get such great images. Name is Stuart Owen Fox, go here
http://www.smartstate.qld.gov.au/images/icase4g_2.jpg for an example.
cheers,
Rosemary

} From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} Date: Thu, 20 May 2004 18:10:14 -0700
} To: {microscopy-at-msa.microscopy.com}
} Cc: Malcolm Haswell {malcolm.haswell-at-sunderland.ac.uk}
} Subject: [Microscopy] Re: Hi-Res Microprocessor Photos
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Malcolm,
}
} Interestingly, I had the same thought and tried this technique. I stopped by
} one of the area's premier graphics arts service bureaus with an 8000+ dpi
} flat bed scanner. We put the open faced CPU chip on the glass and proceeded
} to scan it. It was awful. The main problem was that the light source on the
} scanner was off-axis to the scanning array. This renders the face of the
} chip dark and worthless.
}
} Photos of microprocessors benefit from coaxial lighting since the metal
} parts and traces reflect the light straight back to the lens and light
} source. Lighting that's even slightly off-axis shows a marked drop off in
} detail and reflectivity of the die faces.
}
} The high dpi flat bed scanners are set up for flat artwork such as paintings
} and drawings where side lighting is fine for rendering all the detail but
} not for reflective metal parts.
}
} Doug
}
}
} }
} }
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ----------------------------------------------------------------------------
} --} -
} }
} } Doug
} }
} } given the complexity of what you are doing, would it not be possible to try
} } another method. If the die faces are flat and of the right size, why not just
} } use a very high resolution flat bed scanner and do the whole thing in one go.
} }
} } I'm sure that HP, Epson, Canon all do better than 3000dpi (optical
} } resolution.
} } It might certainly be worth investigating if camera photography involves a
} } horrendous amount of image stitching (especially given the edge distortion in
} } even the best camera). The only problems may be the reflective light quality
} } of the scanner or how much depth of field there would be in a scanner image
} } if
} } the die has lots of depth to its layers.
} }
} } My apologies if I've missed some technical point.
} }
} } Malc
} }
} } Malcolm Haswell
} } e.m. unit
} } University of Sunderland
} } UK
} } e-mail: malcolm.haswell-at-sunderland.ac.uk
} }
} }
} }
} }
} } ----- Original Message -----
} } } From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} } Date: Wednesday, May 19, 2004 11:07 pm
} } Subject: [Microscopy] Hi-Res Microprocessor Photos
} }
} } }
} } }
} } } -------------------------------------------------------------------
} } } -----------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } AmericaTo Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } } -------------------------------------------------------------------
} } } ----
} } }
} } } Hello Fellow List Members,
} } }
} } } IŹd appreciate your collective wisdom and experiences for a
} } } project IŹm
} } } starting. I need to create high resolution (250 Mb minimum) photo
} } } files of
} } } current microprocessor die faces (pentium 4 type) to show the
} } } circuitry and
} } } traces with as much detail as possible. IŹd like to do this using
} } } my Nikon
} } } Optiphot and a yet to be purchased motorized positionable stage with
} } } automation software to include my Fuji S2 still camera (34 Mb
} } } sized files
} } } per image) with image stitching as an added option. I have extensive
} } } experience in Photoshop and would use that to stitch the images if the
} } } automation software package doesnŹt include that. The stage travel
} } } onlyneeds to be about 3" (75mm) in the X and Y dimensions.
} } }
} } } IŹve been reading about some of the software programs available to
} } } helpaccomplish this. IŹve come across Image-Pro Plus with the
} } } Scope-Pro plugin
} } } and the software program Metamorph in my Google searches. I donŹt need
} } } extensive filtering or analysis functions in the software, just
} } } the ability
} } } to create multiple, tileable images in a repeatable manner.
} } }
} } } What economical software and hardware (such as the MultiScan-4 Low
} } } CostScanning Stage for example) do you have experience with in
} } } similar projects?
} } }
} } } Do any of you have an older version of Image Pro Plus or similar
} } } softwareprogram that is sitting abandoned and alone on a shelf
} } } that needs a new
} } } home? How about a used basic scanning stage thatŹs collecting dust?
} } }
} } } Any and all advice would be appreciated. You can email me off-list
} } } if thatŹs
} } } easier.
} } }
} } } Thanks,
} } } Doug Baldwin
} } } Baldwin Hi-Tech Photography
} } } dougbaldwin-at-mindspring.com
} } }
} } }
} } }
} } }
} }
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu May 20 23:52:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi all

Can anyone suggest a good text or reference for helping to identify
asbestos bodies in lung using an SEM, and using EDS.

Many thanks

Regards

Allan

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 00:26:15 2004

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Dear Elaine

A good glassblower can sort it.
Either by producing another or taking the gouge out.
I have done that in the past on a VERY OLD Edwards. Definitely cheaper than the scientific company's. The quality of the work was good and the new dome is still in operation after 6 years.

-----Original Message-----
} From: Elaine Humphrey [mailto:ech-at-interchange.ubc.ca]
Sent: Thursday, May 20, 2004 10:59 PM
To: microscopy-at-msa.microscopy.com

Hello Everyone
We have a Nonotech Semprep2 sputter coater which is so old the
company no longer exists. The glass cylinder has now got one more
gouge in it and it will have to lose at least 3 cm to grind it out.
Does anyone have any experience with where to buy a new glass
cylinder?

Many thanks
Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 03:55:22 2004

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Dear Doug,

Regarding stitching images, we have successfully stitched micrographs using
PanaVue ImageAssembler (www.panavue.com) as it works with flat perspective.
Have not tried to stitch very large numbers of images though.

With regards
Thor

Dr Thor Bostrom
Analytical EM Facility; and
School of Physical and Chemical Sciences,
Queensland University of Technology (QUT)
Brisbane, QLD 4001, Australia

----------Original
message-------------------------------------------------------

Hi all!

does anybody know how is the phase in AFM software Nanoscope III for
Dimension 2100 defined? Could the bright regions in the phase image be
assigned to the depressions, if we are working in the attractive force
regime? Thank's a lot for any hint.

Best regards!

--
__________________________________________________

Đenan Konjhodzic
Max-Planck-Institut für Kohlenforschung
Kaiser-Wilhelm-Platz 1
D-45470 Mülheim an der Ruhr

Phone: +49-208-306 2449
Fax: +49-208-306 2995
Mobile: +49-179-94 98 435
e-mail: denan-at-mpi-muelheim.mpg.de
___________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 06:54:26 2004

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Hi Allan,

I seriously doubt there is one as to unambiguously identify fibrous
asbestos is the job of TEM and (not or) an EDS on TEM.

****************************************
Chaoying Ni, PhD
The W.M. Keck Electron Microscope Facility
Facility location: 022 Spencer Laboratory
Mailing address:
201 duPont Hall
Dept of Matls Sci & Eng
University of Delaware
Newark, DE 19716
(302) 831-8354 (O); -2318(L); -4545(Fax)
http://eml.masc.udel.edu
*****************************************

On Fri, 21 May 2004, Allan Mitchell wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi all
}
} Can anyone suggest a good text or reference for helping to identify
} asbestos bodies in lung using an SEM, and using EDS.
}
} Many thanks
}
} Regards
}
} Allan
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 07:57:16 2004

Contents Retrieved from Microscopy Listserver Archives
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I have some cells in solution. Is there some general technique to preserve
them so that I can put some down on a carbon membrane coated TEM grid
without them shriveling up? Can anyone refer me to a good reference on TEM
sample prep of cells?

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 08:09:47 2004

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Allan,

The Mineralogical Society of America has a series of books on
mineralogical and geochemical topics. Volume 28 is titled "Health
Effects of Mineral Dusts" and covers a wide range of topics, from basic
asbestos mineralogy to cellular and molecular mechanisms for disease.
I'm not sure if it specifically deals with identifying asbestos bodies
in lung tissue specificaly but it should have some references, and there
should be useful information to help with EDS identification. It's
available at the MSA (the other MSA) website at
www.minsocam.org/MSA/RIM/ for a very reasonable price for the amount of
information contained ($32 US).

Best Regards,
Bryan Bandli

Allan Mitchell wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hi all
}
} Can anyone suggest a good text or reference for helping to identify
} asbestos bodies in lung using an SEM, and using EDS.
}
} Many thanks
}
} Regards
}
} Allan
}
}

--
-----------------------------------------------------------------------------------------------------------------------------------------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Fri May 21 10:48:40 2004

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I had a request recently to perform EDS on a presumed crysotile
crystal/shard that had been located with TEM on a grid. We have an
Oxford INCA system on our FEI Quanta 400, so I resurrected an old grid
holder from a salvaged RCA EMU4, mounted the grid in holder in the ESEM,
located the offending grid square and performed a point and ID on the
crystal in question.

As Chaoying suggests, this would not be in concert with NIOSH 7402
(TEM)
http://www.cdc.gov/niosh/nmam/pdfs/7402.pdf, or NIOSH 9000 (XRD)
http://www.cdc.gov/niosh/nmam/pdfs/7402.pdf, identifications of
asbestos, to give quick examples.

Other sources and possibilities for your problem(?):
SEM+:
http://sup.ultrakohl.com/News-nov/mesoth.htm

EBSD:

http://www.asbestostemlabs.com/staff.htm

SEM/EBSD
http://www.dxcicdd.com/01/pdf/D-075.pdf

I don't believe that EBSD/SEM has been approved for asbestos:

http://hyperphysics.phy-astr.gsu.edu/hbase/minerals/asbestos.html

But that doesn't mean that SEM can't be used in simple identifications
of morphology and composition. The real problem is to find it, if you
are looking in tissue. Mapping for the relevant elements should work,
but for very small crystals, you will be working at or above the 'good
result' window for EDS and mapping when you want to identify and image
at high mag.

Hope some of this helps,

Fred

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: Allan Mitchell [mailto:allan.mitchell-at-stonebow.otago.ac.nz]
Sent: Friday, May 21, 2004 1:01 AM
To: microscopy-at-msa.microscopy.com

Hi all

Can anyone suggest a good text or reference for helping to identify
asbestos bodies in lung using an SEM, and using EDS.

Many thanks

Regards

Allan

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 11:05:04 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Do you want to just look at them whole, in a HVEM? No
embedding/sectioning? What do you want to see?

On Fri, 21 May 2004, Larsen, Michael (Research) wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I have some cells in solution. Is there some general technique to preserve
} them so that I can put some down on a carbon membrane coated TEM grid
} without them shriveling up? Can anyone refer me to a good reference on TEM
} sample prep of cells?
}
}

|--------------------------------------------------|
Tamara Howard
Department of Cell Biology and Physiology
University of New Mexico - Health Sciences Center
Albuquerque, NM 87131
thoward-at-unm.edu
|--------------------------------------------------|

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 11:51:52 2004

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Today's microprocessors have micron scale metal lines. You would require submicron resolution to distinguish the lines. A flat bed scanner that would resolve micron scale lines would need at least 25,000 DPI resolution just to detect the lines.

John Mardinly
Intel

-----Original Message-----
} From: Rosemary White [mailto:Rosemary.White-at-csiro.au]
Sent: Thursday, May 20, 2004 8:24 PM
To: Doug Baldwin; microscopy-at-msa.microscopy.com
Cc: Malcolm Haswell

There is a photographer here in Oz who produces absolutely brilliant images
by scanning objects on a flat-bed scanner. They are very high resolution,
look as good as the images of leaves, flowers, insects (even very shiny
ones) we get using a good digital camera - Olympus DP70 or ProgRes or
similar, on a dissecting microscope. He's developed some ways of using the
scanner to get such great images. Name is Stuart Owen Fox, go here
http://www.smartstate.qld.gov.au/images/icase4g_2.jpg for an example.
cheers,
Rosemary

} From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} Date: Thu, 20 May 2004 18:10:14 -0700
} To: {microscopy-at-msa.microscopy.com}
} Cc: Malcolm Haswell {malcolm.haswell-at-sunderland.ac.uk}
} Subject: [Microscopy] Re: Hi-Res Microprocessor Photos
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Malcolm,
}
} Interestingly, I had the same thought and tried this technique. I stopped by
} one of the area's premier graphics arts service bureaus with an 8000+ dpi
} flat bed scanner. We put the open faced CPU chip on the glass and proceeded
} to scan it. It was awful. The main problem was that the light source on the
} scanner was off-axis to the scanning array. This renders the face of the
} chip dark and worthless.
}
} Photos of microprocessors benefit from coaxial lighting since the metal
} parts and traces reflect the light straight back to the lens and light
} source. Lighting that's even slightly off-axis shows a marked drop off in
} detail and reflectivity of the die faces.
}
} The high dpi flat bed scanners are set up for flat artwork such as paintings
} and drawings where side lighting is fine for rendering all the detail but
} not for reflective metal parts.
}
} Doug
}
}
} }
} }
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ----------------------------------------------------------------------------
} --} -
} }
} } Doug
} }
} } given the complexity of what you are doing, would it not be possible to try
} } another method. If the die faces are flat and of the right size, why not just
} } use a very high resolution flat bed scanner and do the whole thing in one go.
} }
} } I'm sure that HP, Epson, Canon all do better than 3000dpi (optical
} } resolution.
} } It might certainly be worth investigating if camera photography involves a
} } horrendous amount of image stitching (especially given the edge distortion in
} } even the best camera). The only problems may be the reflective light quality
} } of the scanner or how much depth of field there would be in a scanner image
} } if
} } the die has lots of depth to its layers.
} }
} } My apologies if I've missed some technical point.
} }
} } Malc
} }
} } Malcolm Haswell
} } e.m. unit
} } University of Sunderland
} } UK
} } e-mail: malcolm.haswell-at-sunderland.ac.uk
} }
} }
} }
} }
} } ----- Original Message -----
} } } From: Doug Baldwin {dougbaldwin-at-mindspring.com}
} } Date: Wednesday, May 19, 2004 11:07 pm
} } Subject: [Microscopy] Hi-Res Microprocessor Photos
} }
} } }
} } }
} } } -------------------------------------------------------------------
} } } -----------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } AmericaTo Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } } -------------------------------------------------------------------
} } } ----
} } }
} } } Hello Fellow List Members,
} } }
} } } IŹd appreciate your collective wisdom and experiences for a
} } } project IŹm
} } } starting. I need to create high resolution (250 Mb minimum) photo
} } } files of
} } } current microprocessor die faces (pentium 4 type) to show the
} } } circuitry and
} } } traces with as much detail as possible. IŹd like to do this using
} } } my Nikon
} } } Optiphot and a yet to be purchased motorized positionable stage with
} } } automation software to include my Fuji S2 still camera (34 Mb
} } } sized files
} } } per image) with image stitching as an added option. I have extensive
} } } experience in Photoshop and would use that to stitch the images if the
} } } automation software package doesnŹt include that. The stage travel
} } } onlyneeds to be about 3" (75mm) in the X and Y dimensions.
} } }
} } } IŹve been reading about some of the software programs available to
} } } helpaccomplish this. IŹve come across Image-Pro Plus with the
} } } Scope-Pro plugin
} } } and the software program Metamorph in my Google searches. I donŹt need
} } } extensive filtering or analysis functions in the software, just
} } } the ability
} } } to create multiple, tileable images in a repeatable manner.
} } }
} } } What economical software and hardware (such as the MultiScan-4 Low
} } } CostScanning Stage for example) do you have experience with in
} } } similar projects?
} } }
} } } Do any of you have an older version of Image Pro Plus or similar
} } } softwareprogram that is sitting abandoned and alone on a shelf
} } } that needs a new
} } } home? How about a used basic scanning stage thatŹs collecting dust?
} } }
} } } Any and all advice would be appreciated. You can email me off-list
} } } if thatŹs
} } } easier.
} } }
} } } Thanks,
} } } Doug Baldwin
} } } Baldwin Hi-Tech Photography
} } } dougbaldwin-at-mindspring.com
} } }
} } }
} } }
} } }
} }
} }
} }
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 14:17:27 2004

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Listers,

I'll try again. Does anyone have a Gatan model 626-300 cryoholder to
sell or donate to a university?
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 14:21:00 2004

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We would like to buy or trade in:
epi-fluorescence lamp housing and slider for Diaphot (inverted Nikon)
new or refurbished.

Vendors welcome!

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 14:48:08 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Doug,

Image-Pro Plus is a very good image analysis software with
extensive capabilities. But there is a another product from
Media Cybernetics which is "Image-Pro Discovery". This
is the smaller version of Image-Pro Plus and therefore
cheaper. It allows you to capture X-Y automatically in
combination with Scope-Pro. The software gives you the
possibility to select the order how you want to capture
the images and it stitches them automatically.
You also could capture Z-stacks automatically either by
moving the microscope stage or with a motorized objective
(Piezo) which gives you very precise results.

However if you want to work with an automatic x-y stage you
should work with a camera which is integrated in the
capturing software because then the software also captures
the images, then the stage moves on, the image is captured and so
on. With your Fuji camera you have to do the capturing
manually which is very cumbersome. You should use a digital
CCD camera which is connected to your computer and shows you
the live image on the computer monitor.

Please let me know if you have further questions.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

DB} ------------------------------------------------------------------------------
DB} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
DB} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
DB} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
DB} -------------------------------------------------------------------------------

DB} Hello Fellow List Members,

DB} Iąd appreciate your collective wisdom and experiences for a project Iąm
DB} starting. I need to create high resolution (250 Mb minimum) photo files of
DB} current microprocessor die faces (pentium 4 type) to show the circuitry and
DB} traces with as much detail as possible. Iąd like to do this using my Nikon
DB} Optiphot and a yet to be purchased motorized positionable stage with
DB} automation software to include my Fuji S2 still camera (34 Mb sized files
DB} per image) with image stitching as an added option. I have extensive
DB} experience in Photoshop and would use that to stitch the images if the
DB} automation software package doesnąt include that. The stage travel only
DB} needs to be about 3" (75mm) in the X and Y dimensions.

DB} Iąve been reading about some of the software programs available to help
DB} accomplish this. Iąve come across Image-Pro Plus with the Scope-Pro plugin
DB} and the software program Metamorph in my Google searches. I donąt need
DB} extensive filtering or analysis functions in the software, just the ability
DB} to create multiple, tileable images in a repeatable manner.

DB} What economical software and hardware (such as the MultiScan-4 Low Cost
DB} Scanning Stage for example) do you have experience with in similar projects?

DB} Do any of you have an older version of Image Pro Plus or similar software
DB} program that is sitting abandoned and alone on a shelf that needs a new
DB} home? How about a used basic scanning stage thatąs collecting dust?

DB} Any and all advice would be appreciated. You can email me off-list if thatąs
DB} easier.

DB} Thanks,
DB} Doug Baldwin
DB} Baldwin Hi-Tech Photography
DB} dougbaldwin-at-mindspring.com

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 15:19:40 2004

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Bill
I disagree with you: carbon coated Formvar film do degrade the image in
your words versus just carbon. Formvar film is quite thick in compare with
"plain carbon", so it "adsorbs" more electrons and therefore "degrade the
image"... Another problem with Formvar and other plastic support films is
that they change their properties under the beam which cause the image
drift... So, in my point of view, it's just wrong statement that carbon
coated Formvar film "does not degrade the images of negatively stained
preps". It's quite opposite: pure thin carbon film is very stable under
the beam, much thinner than any plastic film and therefore provides best
possible (for biological samples) support material in terms of stability
and "transparency" (to the electrons) for negative staining. Carbon coated
plastic support films are popular just because it's much easier to produce
in the Lab (and not necessary the best choice). In my Lab we routinely use
1.4-1.8 nm thick "pure" carbon support films over "holey" film. You may
not use such thin film for huge objects like whole cell, but it works great
for macromolecules of any sort. "Carbon over holey film" grids are
available thorough major EM suppliers. Interestingly, I never used carbon
coated Formvar films. I used to use carbon coating on cellulose-derivative
films like Parlodion (because it drifted so much without carbon) and I used
"naked" Formvar film because it's more stable under the beam than other
variety of films. Formvar film looks much "darker" in the scope than
Parlodion, so I prefer to use carbon coated Parlodion film if I could not
use "normal carbon": very contaminated samples with a lot of aggregates,
cells etc. Someone may need to try "naked" Parlodion (or similar) because
good hydrophilic properties of cellulose-deviated films if Formvar of
carbon is too hydrophobic to them (at the huge price of film instability in
the beam). I don't like glow-discharge, personally: I would rather use
poly-lysine coating. Have a great weekend, Sergey

At 05:39 PM 5/20/2004 -0700, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Fri May 21 16:18:31 2004

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Hi listers
I have a problem I am hoping that someone out there can help me with.
7 years ago our lab jointly bought a Photometrix SenSys PVCAM with
another lab. The labs are splitting up. We need to determine the
current value of the camera so that one lab can pay the other lab. Can
anybody point me to this data?
Thanx
David

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 17:29:47 2004

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Hi -

We have been using the Epson Perfection 3200 scanner for 8x10 cm TEM
negatives for about a year now, and find it excellent. The
resolution (3200 dpi optical) is almost as good as the 4000 dpi on
the Nikon 8000 etc., and we successfully scanned some very dense
(accidentally overexposed) negatives when our TEM's exposure meter
went on the fritz. We mount the negatives in the standard 4x5"
negative carrier. (The Nikon negative holder doesn't fit 8x10 cm
negatives without modification, or cutting the negatives down to
size.) The 3200 was listed at $299 on the Epson website the last
time I looked.

Cheers,
Tom Kosel

Original message:

Hello Listers,

I wanted to see if anyone has had any experience scanning negatives
with the Canon Canoscan 9900F.
I have a low end Canoscan that I use for documents and the occasional
photograph, which has given me
very good results, but is not set up for negatives. I have seen the
recent posts about the Epson scanner,
but I am trying to keep it under a $1000 so that I do not have to
treat it as a capital purchase. I have tried
for the last two years to get a Coolscan 8000 on the capital budget
with no luck, and do not see any scanner
above $1000 as an option right now.

Thanks,
Steve

Steven Lee
Chief Technologists
Electron Microscopy Laboratory
Baylor University Medical Center
3500 Gaston Ave
Dallas, TX 750246
Ph: 214.820.3302
Fx: 214.820.4110
Em: stevenle-at-baylorhealth.edu
--
*********************************
Thomas H. Kosel
Department of Electrical Engineering
University of Notre Dame
Notre Dame, IN 46556
(574) 631-5642 (201 Cushing)
(574) 631-4393 FAX
kosel-at-nd.edu
*********************************

From MicroscopyL-request-at-ns.microscopy.com Fri May 21 19:08:23 2004

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Hi,

I want to find some papers or books which introduce the determination of
the direction of dislocation lines by TEM.

Thank you very much,

Regards,

Nina

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 02:05:24 2004

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"Electron Microscopy of Thin Crystals"
Hirsch, Howie, Nicholson, Pashley & Whelan
Pub: Robert E. Krieger
ISBN: 0-88275-376-2

"Transmission Electron Microscopy of Materials"
Thomas & Goringe
Pub: John Wiley & Sons
ISBN: 0-471-12244-0

"Defect Analysis in Electron Microscopy"
Loretto & Smallman
Pub: Chapman & Hall
ISBN: 0-470-54760-X

The latter, in particular, is quite detailed about dislocation
analysis with specific instructions. It also gives details of
weak-beam methods, which give much higher resolution images of
dislocations, very useful if you have closely packed dislocations.

Unfortunately, I suspect all are no longer in print.
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail
will automatically be deleted.
:-)

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 04:58:19 2004

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Dear microscopist experts,

When I read literatures, I have been all the time
confused by the resolution definition in transmission
electron microscopy. Could you please kindly help?

For a FEG-HRTEM, what is the "line resolution" as
opposed to the "information resolution"? What is the
difference between each other?

How could I achieve the "line resolution" and the
"information resolution" in TEM experiments? And, how
can I resolve (identify, or "see") the "line
resolution" and the "information resolution"
respectively from a state-of-the-art HREM image?

Thank you for your time. Wish you a nice weekend,

-Juha

__________________________________
Do you Yahoo!?
Yahoo! Domains – Claim yours for only $14.70/year
http://smallbusiness.promotions.yahoo.com/offer

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 09:13:06 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (antuni-at-aol.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, May 21, 2004 at 16:19:26
---------------------------------------------------------------------------

Email: antuni-at-aol.com
Name: Anthony Ribaudo

Organization: Consultant

Title-Subject: [Microscopy] [Filtered] Identifying Asbestos Using ptical Microscopy

Question: Can one identify asbestos only utilizing optical microscopy without the aid of electron diffraction/TEM ?

Anthony Ribaudo

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 09:14:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (christian_b_a-at-hotmail.com) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Friday, May 21, 2004 at 09:07:25
---------------------------------------------------------------------------

Email: christian_b_a-at-hotmail.com
Name: christian albano

Organization: Neuropsychiatric Research Institute

Education: Graduate College

Location: Fargo, ND, USA

Question: Does using the Fluoview Olympus LSCM for non-floresence degrade the equipment lifetime?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 11:52:37 2004

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Warning: Non scientific answer:

I remember an edition of "This Old House" or one of those types of shows
where they took some shingle samples to a lab for testing.

The lab used polarized microscopy to do at least an "initial" screening
and determine that the shingles "most likely" contained asbestos.

The "would do some additional testing" to verify (it was, and the house
needed to have a tent built around it, etc., etc.). I assume the
additional testing was something along the lines of TEM, etc.

The conclusion I drew was that if you had materials that you were
expecting asbestos, this (polarized examination) was a good screening
tool. If the fibers didn't change from one specific color to another as
the analyzer was rotated, you didn't have asbestos. If they did, you
probably have asbestos, but there are other fibers that may do the same
thing.

These were also fibers, not dust, and I don't know if that would affect
the results or not.

Sorry if this wasn't useful.

John R.

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
Sent: Saturday, May 22, 2004 9:23 AM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (antuni-at-aol.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday,
May 21, 2004 at 16:19:26
------------------------------------------------------------------------
---

Email: antuni-at-aol.com
Name: Anthony Ribaudo

Organization: Consultant

Title-Subject: [Microscopy] [Filtered] Identifying Asbestos Using ptical
Microscopy

Question: Can one identify asbestos only utilizing optical microscopy
without the aid of electron diffraction/TEM ?

Anthony Ribaudo

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Sat May 22 16:00:20 2004

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Only one of the forms of asbestos is harmful to humans. Chrysotile
and then only if it is inhaled and the particle size is such it
lodges in the lung so it can form a site for cancer to get a start.
Chrysotile is only a small percentage of asbestos and the particle
size must fall in the 5 to 15 micron range to stay in the lungs.

These conditions are almost only found in asbestos worker and miners
and not in the general public. In the case of high exposure to
asbestos cigarette smoking is also a very large contributor to the
cancer caused by asbestos.

Had the asbestos studies been allowed to be fully peer reviewed
before legislation was passed we would probably still be using
asbestos in many applications today with more protection for
asbestos workers and minors and restrictions on some products such
as asbestos powder and asbestos cloth. Unfortunately the legislators
won't review thier laws once they are passed and the western world
is spending needless billions of dollars in asbestos abatement in
every old building that is renovated.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Chiphead" {chiphead-at-sbcglobal.net}

:
: Warning: Non scientific answer:
:
: I remember an edition of "This Old House" or one of those types of
shows
: where they took some shingle samples to a lab for testing.
:
: The lab used polarized microscopy to do at least an "initial"
screening
: and determine that the shingles "most likely" contained asbestos.
:
: The "would do some additional testing" to verify (it was, and the
house
: needed to have a tent built around it, etc., etc.). I assume the
: additional testing was something along the lines of TEM, etc.
:
: The conclusion I drew was that if you had materials that you were
: expecting asbestos, this (polarized examination) was a good
screening
: tool. If the fibers didn't change from one specific color to
another as
: the analyzer was rotated, you didn't have asbestos. If they did,
you
: probably have asbestos, but there are other fibers that may do the
same
: thing.
:
: These were also fibers, not dust, and I don't know if that would
affect
: the results or not.
:
: Sorry if this wasn't useful.
:
: John R.
:
: -----Original Message-----
: } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
: Sent: Saturday, May 22, 2004 9:23 AM
: To: microscopy-at-ns.microscopy.com
: Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
: Microscopy
:
:
:
: ------------------------------------------------------------------
------
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: The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
: To Subscribe/Unsubscribe --
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:
: Below is the result of your feedback form (NJZFM-ultra-55). It
was
: submitted by (antuni-at-aol.com) from
: http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday,
: May 21, 2004 at 16:19:26
: ------------------------------------------------------------------
------
: ---
:
: Email: antuni-at-aol.com
: Name: Anthony Ribaudo
:
: Organization: Consultant
:
: Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
Using ptical
: Microscopy
:
: Question: Can one identify asbestos only utilizing optical
microscopy
: without the aid of electron diffraction/TEM ?
:
:
: Anthony Ribaudo
:
:
:
: ------------------------------------------------------------------
------
: ---
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 09:31:26 2004

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This is off the topic of identifying asbestos, but thought I should comment
that just yesterday there was a program on the radio (streaming audio
available at http://www.abc.net.au/rn/talks/bbing/, transcript available by
Thursday) about new cases of asbestosis and mesothelioma showing up. The
young people (20s and 30s) now getting this lived in high asbestos areas as
kids, were children of builders (and builders themselves) who demolished or
renovated fibro houses, etc. Perhaps just an Australian problem....
Rosemary

} From: "Gordon Couger" {gcouger-at-provalue.net}
} Date: Sat, 22 May 2004 16:09:06 -0500
} To: "Chiphead" {chiphead-at-sbcglobal.net} , "'by way of MicroscopyListserver'"
} {antuni-at-aol.com} , {microscopy-at-ns.microscopy.com}
} Subject: [Microscopy] Re: RE: viaWWW: Identifying Asbestos Using ptical
} Microscopy
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Only one of the forms of asbestos is harmful to humans. Chrysotile
} and then only if it is inhaled and the particle size is such it
} lodges in the lung so it can form a site for cancer to get a start.
} Chrysotile is only a small percentage of asbestos and the particle
} size must fall in the 5 to 15 micron range to stay in the lungs.
}
} These conditions are almost only found in asbestos worker and miners
} and not in the general public. In the case of high exposure to
} asbestos cigarette smoking is also a very large contributor to the
} cancer caused by asbestos.
}
} Had the asbestos studies been allowed to be fully peer reviewed
} before legislation was passed we would probably still be using
} asbestos in many applications today with more protection for
} asbestos workers and minors and restrictions on some products such
} as asbestos powder and asbestos cloth. Unfortunately the legislators
} won't review thier laws once they are passed and the western world
} is spending needless billions of dollars in asbestos abatement in
} every old building that is renovated.
}
} Gordon
} Gordon Couger gcc-at-couger.com
}
} I collect links on information related to light microscopes.
} http://www.couger.com/microscope/links/gclinks.html
} Please forward any links or information you think might be useful to
} others.
} Microscope Manual at www.science-info.org
}
} } From: "Chiphead" {chiphead-at-sbcglobal.net}
}
} :
} : Warning: Non scientific answer:
} :
} : I remember an edition of "This Old House" or one of those types of
} shows
} : where they took some shingle samples to a lab for testing.
} :
} : The lab used polarized microscopy to do at least an "initial"
} screening
} : and determine that the shingles "most likely" contained asbestos.
} :
} : The "would do some additional testing" to verify (it was, and the
} house
} : needed to have a tent built around it, etc., etc.). I assume the
} : additional testing was something along the lines of TEM, etc.
} :
} : The conclusion I drew was that if you had materials that you were
} : expecting asbestos, this (polarized examination) was a good
} screening
} : tool. If the fibers didn't change from one specific color to
} another as
} : the analyzer was rotated, you didn't have asbestos. If they did,
} you
} : probably have asbestos, but there are other fibers that may do the
} same
} : thing.
} :
} : These were also fibers, not dust, and I don't know if that would
} affect
} : the results or not.
} :
} : Sorry if this wasn't useful.
} :
} : John R.
} :
} : -----Original Message-----
} : } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
} : Sent: Saturday, May 22, 2004 9:23 AM
} : To: microscopy-at-ns.microscopy.com
} : Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
} : Microscopy
} :
} :
} :
} : ------------------------------------------------------------------
} ------
} : ------
} : The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} : To Subscribe/Unsubscribe --
} : http://www.msa.microscopy.com/MicroscopyListserver
} : On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} : ------------------------------------------------------------------
} ------
} : -------
} :
} : Below is the result of your feedback form (NJZFM-ultra-55). It
} was
} : submitted by (antuni-at-aol.com) from
} : http://microscopy.com/MicroscopyListserver/MLFormMail.html on
} Friday,
} : May 21, 2004 at 16:19:26
} : ------------------------------------------------------------------
} ------
} : ---
} :
} : Email: antuni-at-aol.com
} : Name: Anthony Ribaudo
} :
} : Organization: Consultant
} :
} : Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
} Using ptical
} : Microscopy
} :
} : Question: Can one identify asbestos only utilizing optical
} microscopy
} : without the aid of electron diffraction/TEM ?
} :
} :
} : Anthony Ribaudo
} :
} :
} :
} : ------------------------------------------------------------------
} ------
} : ---
} :
} :
} :
} :
} :
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 09:50:34 2004

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Listers,

Sorry, I forgot to state that the cryoholder we're looking for would
be for a Hitachi S-900 in-lens FESEM, which uses a Hitachi TEM holder.

Phil
--
Philip Oshel
Supervisor, AMFSC and BBPIC microscopy facilities
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 11:14:18 2004

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Gordon,

It is hard to believe other forms of asbestos: amosite asbestos(grunerite), actinolite-tremolite asbestos, anthophyllite (asbestos)and crocidolite asbestos(riebeckite) are not harmful. Have any studies been done on this? Chrysotile asbestos makes up to +90% of all asbestos in North America. (please correct if somebody has published figures on this).

Asbestos has been linked to mesothelioma and, also, asbestos is the cause of asbestosis(also harmful to humans). Isn't it?

I agree. If asbestos studies had been fully reviewed we would still using asbestos it has unique chemical and physical properties, especially for a mineral. The politicians used asbestos as a political football first scaring the public then passing legislation covering asbestos in schools, AHERA. Yes many problems have occurred as a result of this. The regulation should be reviewed and changed(if if hasn't already been).

Yes, asbestos can be identified by polarized light microscopy, not OLM or PCM. Using dispersion staining techniques to determine refractive indices, a properly prepared asbestos fiber can be identified, by PLM. Other measured properties: pleochroism, sign of elongation, and angle of extinction plus physical characteristic further aid the PLM analyst in the proper identification. Preparation of the fiber and proper training of the analyst are the critical factors here. Binder/matrix effects may hinder the analysis, for example chrysotile in vinyl floor tile.

Where are all the McCrone(ies) on this? Maybe this subject has been hashed out in the past. If so pardon me for the repeated redundancy.

Regards,

Timothy J. Bard, Scientist
Scanning Electron Microscopy
OSRAM SYLVANIA
Towanda, PA

U

-----Original Message-----
} From: Gordon Couger [mailto:gcouger-at-provalue.net]
Sent: Saturday, May 22, 2004 5:09 PM
To: Chiphead; 'by way of MicroscopyListserver';
microscopy-at-ns.microscopy.com

Only one of the forms of asbestos is harmful to humans. Chrysotile
and then only if it is inhaled and the particle size is such it
lodges in the lung so it can form a site for cancer to get a start.
Chrysotile is only a small percentage of asbestos and the particle
size must fall in the 5 to 15 micron range to stay in the lungs.

These conditions are almost only found in asbestos worker and miners
and not in the general public. In the case of high exposure to
asbestos cigarette smoking is also a very large contributor to the
cancer caused by asbestos.

Had the asbestos studies been allowed to be fully peer reviewed
before legislation was passed we would probably still be using
asbestos in many applications today with more protection for
asbestos workers and minors and restrictions on some products such
as asbestos powder and asbestos cloth. Unfortunately the legislators
won't review their laws once they are passed and the western world
is spending needless billions of dollars in asbestos abatement in
every old building that is renovated.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Chiphead" {chiphead-at-sbcglobal.net}

:
: Warning: Non scientific answer:
:
: I remember an edition of "This Old House" or one of those types of
shows
: where they took some shingle samples to a lab for testing.
:
: The lab used polarized microscopy to do at least an "initial"
screening
: and determine that the shingles "most likely" contained asbestos.
:
: The "would do some additional testing" to verify (it was, and the
house
: needed to have a tent built around it, etc., etc.). I assume the
: additional testing was something along the lines of TEM, etc.
:
: The conclusion I drew was that if you had materials that you were
: expecting asbestos, this (polarized examination) was a good
screening
: tool. If the fibers didn't change from one specific color to
another as
: the analyzer was rotated, you didn't have asbestos. If they did,
you
: probably have asbestos, but there are other fibers that may do the
same
: thing.
:
: These were also fibers, not dust, and I don't know if that would
affect
: the results or not.
:
: Sorry if this wasn't useful.
:
: John R.
:
: -----Original Message-----
: } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
: Sent: Saturday, May 22, 2004 9:23 AM
: To: microscopy-at-ns.microscopy.com
: Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
: Microscopy
:
:
:
: ------------------------------------------------------------------
------
: ------
: The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
: To Subscribe/Unsubscribe --
: http://www.msa.microscopy.com/MicroscopyListserver
: On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
: ------------------------------------------------------------------
------
: -------
:
: Below is the result of your feedback form (NJZFM-ultra-55). It
was
: submitted by (antuni-at-aol.com) from
: http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday,
: May 21, 2004 at 16:19:26
: ------------------------------------------------------------------
------
: ---
:
: Email: antuni-at-aol.com
: Name: Anthony Ribaudo
:
: Organization: Consultant
:
: Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
Using ptical
: Microscopy
:
: Question: Can one identify asbestos only utilizing optical
microscopy
: without the aid of electron diffraction/TEM ?
:
:
: Anthony Ribaudo
:
:
:
: ------------------------------------------------------------------
------
: ---
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 12:48:22 2004

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I have a student in my lab who wants to do immunohist on mouse skin. He
is looking at RPA. His current protocol for RPA is on cells. He was
able to get skin from mice treated with BPDE, he fixed the small strips
of skin in 4% paraformaldehyde in Dulbecco's PBS. He fixed it for 20-24
hours, then put it in 70% ethanol followed by routine paraffin
embedding.
Was the fixation time too long? I always fixed for 4-6 hours tops.
Will this affect his immunohist?
Thanks for any help or advice on this.

Stacey Andringa

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 12:52:09 2004

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I work in Cincinnati and we are experiencing our 17 year cicada
invasion. I have never worked with insects and I am interested in
fixing some for light microscopy. What fixative would work on them and
how do I fix them - remove wings, pierce abdomen, etc.? This is for fun
as much as education.
Thanks for your help.

Stacey Andringa

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 12:53:49 2004

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On May 22, 2004, at 3:07 AM, Juha Dapper wrote:

} For a FEG-HRTEM, what is the "line resolution" as
} opposed to the "information resolution"? What is the
} difference between each other?
}
} How could I achieve the "line resolution" and the
} "information resolution" in TEM experiments? And, how
} can I resolve (identify, or "see") the "line
} resolution" and the "information resolution"
} respectively from a state-of-the-art HREM image?
}
Dear Juha,
The line resolution is the closest distance between two edges that can
be resolved, and it can be pretty confusing. A better measure is point
resolution, which can be determined from the first zero of the contrast
transfer function at Shertzer focus. The information limit is the
farthest extent of the Thon rings that can be achieved. To determine
the point resolution, put a thin amorphous carbon specimen in the
scope, adjust the height to eucentric height, make sure the scope is
aligned as well as possible, go to a sufficiently high magnification so
that the spatial frequency of the expected point resolution is larger
than two--or better three--pixels (on a CCD, the actual elements, on
film, the grain separation or resolution of a scanner), then take an
image. Determine the power spectrum by taking the FFT of the
image--easy on a CCD; on film, scan with a high-resolution scanner,
then take the FFT. The spatial frequency of the first zero is the
point resolution of the image. The better the scope is adjusted and
the better the area of the specimen, the closer you will come to the
true resolution of the scope. The information limit is best seen by
shifting the image during the exposure. This produces Young's fringes
in the power spectrum, which makes the extent of the Thon rings easier
to see. The service engineers who set up our scopes used a switch
attached to a shift coil to do this test. In order to achieve the best
resolution and information transfer possible, make sure your scope is
as well aligned as possible. If your specimen is too thick, or
otherwise unsuitable, you may not achieve the specified performance, so
don't blame the equipment in this case. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 13:59:59 2004

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OK, you sucked me in to asbestos and so here goes...........

Almost all of the minerals in existence were identified and
characterized by PLM at one time. Not all of these mineral were done as
well as the rest but still PLM is a powerful tool in the hands of an
experienced and trained microscopist. All of the legally defined asbestos
can be identified by PLM. Dispersion staining is a very useful tool for
this purpose. Vinyl tile, mortar, ceiling tiles, fluffy insulation, wall
plaster, and black or gray or green mastic - sample prep remains the
kingpin of all microscopical analysis just as it is in all analytical
testing.

My understanding is the current alert limits were based on measurements
made in asbestos mines and mills and extended to "normal" areas. This
level may be too low and in my opinion is a result of political games. It
seems some people have extreme sensitivity to asbestos and develop terminal
conditions at very low exposure levels. It is also my understanding these
studies were originally based on adults who were exposed as young adults
and older. I have not seen studies bases on exposure of children to
asbestos. So were do we draw the line? Yes, smoking makes it 400X more
likely to develop health complications (at least that was the number quote
when I did my asbestos certification training in Ohio. Not everyone who
was exposed to high levels developed health complications. I had a boss
who crawled through asbestos rewiring naval ships as summer work. He was a
long term chain smoker, and he lived into his 80's.

Government regulations created a industry of abatement and identification.
I have had the good fortune to participate at the identification and
quantification level for a number of years. The thing to remember is it
doesn't matter your personal beliefs or current scientific data when you're
compiling with a law, it is what the law says it is.

"Bard, Timothy
J." To: "Gordon Couger" {gcouger-at-provalue.net} ,
{Timothy.Bard-at-SYL "Microscopy (E-mail)" {microscopy-at-ns.microscopy.com}
VANIA.com} cc:
Subject: [Microscopy] RE: viaWWW: Identifying
05/24/2004 12:26 Asbestos Using optical Microscopy
PM

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Gordon,

It is hard to believe other forms of asbestos: amosite asbestos(grunerite),
actinolite-tremolite asbestos, anthophyllite (asbestos)and crocidolite
asbestos(riebeckite) are not harmful. Have any studies been done on this?
Chrysotile asbestos makes up to +90% of all asbestos in North America.
(please correct if somebody has published figures on this).

Asbestos has been linked to mesothelioma and, also, asbestos is the cause
of asbestosis(also harmful to humans). Isn't it?

I agree. If asbestos studies had been fully reviewed we would still using
asbestos it has unique chemical and physical properties, especially for a
mineral. The politicians used asbestos as a political football first
scaring the public then passing legislation covering asbestos in schools,
AHERA. Yes many problems have occurred as a result of this. The
regulation should be reviewed and changed(if if hasn't already been).

Yes, asbestos can be identified by polarized light microscopy, not OLM or
PCM. Using dispersion staining techniques to determine refractive indices,
a properly prepared asbestos fiber can be identified, by PLM. Other
measured properties: pleochroism, sign of elongation, and angle of
extinction plus physical characteristic further aid the PLM analyst in the
proper identification. Preparation of the fiber and proper training of the
analyst are the critical factors here. Binder/matrix effects may hinder
the analysis, for example chrysotile in vinyl floor tile.

Where are all the McCrone(ies) on this? Maybe this subject has been hashed
out in the past. If so pardon me for the repeated redundancy.

Regards,

Timothy J. Bard, Scientist
Scanning Electron Microscopy
OSRAM SYLVANIA
Towanda, PA

U

-----Original Message-----
} From: Gordon Couger [mailto:gcouger-at-provalue.net]
Sent: Saturday, May 22, 2004 5:09 PM
To: Chiphead; 'by way of MicroscopyListserver';
microscopy-at-ns.microscopy.com

Only one of the forms of asbestos is harmful to humans. Chrysotile
and then only if it is inhaled and the particle size is such it
lodges in the lung so it can form a site for cancer to get a start.
Chrysotile is only a small percentage of asbestos and the particle
size must fall in the 5 to 15 micron range to stay in the lungs.

These conditions are almost only found in asbestos worker and miners
and not in the general public. In the case of high exposure to
asbestos cigarette smoking is also a very large contributor to the
cancer caused by asbestos.

Had the asbestos studies been allowed to be fully peer reviewed
before legislation was passed we would probably still be using
asbestos in many applications today with more protection for
asbestos workers and minors and restrictions on some products such
as asbestos powder and asbestos cloth. Unfortunately the legislators
won't review their laws once they are passed and the western world
is spending needless billions of dollars in asbestos abatement in
every old building that is renovated.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Chiphead" {chiphead-at-sbcglobal.net}

:
: Warning: Non scientific answer:
:
: I remember an edition of "This Old House" or one of those types of
shows
: where they took some shingle samples to a lab for testing.
:
: The lab used polarized microscopy to do at least an "initial"
screening
: and determine that the shingles "most likely" contained asbestos.
:
: The "would do some additional testing" to verify (it was, and the
house
: needed to have a tent built around it, etc., etc.). I assume the
: additional testing was something along the lines of TEM, etc.
:
: The conclusion I drew was that if you had materials that you were
: expecting asbestos, this (polarized examination) was a good
screening
: tool. If the fibers didn't change from one specific color to
another as
: the analyzer was rotated, you didn't have asbestos. If they did,
you
: probably have asbestos, but there are other fibers that may do the
same
: thing.
:
: These were also fibers, not dust, and I don't know if that would
affect
: the results or not.
:
: Sorry if this wasn't useful.
:
: John R.
:
: -----Original Message-----
: } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
: Sent: Saturday, May 22, 2004 9:23 AM
: To: microscopy-at-ns.microscopy.com
: Subject: [Microscopy] viaWWW: Identifying Asbestos Using ptical
: Microscopy
:
:
:
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: Below is the result of your feedback form (NJZFM-ultra-55). It
was
: submitted by (antuni-at-aol.com) from
: http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday,
: May 21, 2004 at 16:19:26
: ------------------------------------------------------------------
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:
: Email: antuni-at-aol.com
: Name: Anthony Ribaudo
:
: Organization: Consultant
:
: Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
Using ptical
: Microscopy
:
: Question: Can one identify asbestos only utilizing optical
microscopy
: without the aid of electron diffraction/TEM ?
:
:
: Anthony Ribaudo
:
:
:
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From MicroscopyL-request-at-ns.microscopy.com Mon May 24 14:15:01 2004

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Dear Juha,

There are three commonly employed definitions of "HRTEM resolution". All depend on
how information is transferred by the objective lens from the specimen
"exit-surface wave" to the image intensity spectrum (the Fourier transform of the
image intensity).

(1) "Fringe" resolution, or "line" resolution (sometimes called "lattice-plane"
resolution), is measured from the highest spatial frequency that is present in the
image intensity spectrum (and is thus detectable in the optical diffractogram). It
may include non-physical detail, since it may include components from a
"second-order" or "non-linear" interference generating a half-spacing term with
spatial frequency up to twice that of the highest-frequency diffracted beam passed
by the objective aperture and the convergence cross-coefficient envelope
["Resolution-damping functions in non-linear images", M.A. O'Keefe, in 37th Ann.
Proc. EMSA, San Antonio, Texas (1979) 556-557]. For a properly aligned microscope,
it is not affected by microscope spread-of-focus and depends only on factors such
as vibration or detector MTF.

(2) "Linear-image" resolution, or "information-limit" resolution, is measured by
the highest spatial frequency transferred linearly from the amplitude spectrum (the
specimen "exit-surface wave") to the image intensity spectrum with any old phase.
Transferred frequencies fall within one or more passbands, but other (lower)
frequencies may be blocked. Increased underfocus will push the convergence-limited
damping function to higher frequencies, thus this limit (often called just the
"information limit") to point resolution is a function of microscope
spread-of-focus. Spread of focus is a function of objective lens chromatic
aberration and variations in lens current and in electron beam energy (and of
vertical vibration of the specimen within the lens).

(3) "Scherzer" resolution, or "structure-image" resolution (sometimes called
"point" resolution or "point-to-point" resolution) is measured by the highest
linearly-transferred spatial
frequency that can be passed when no lower frequencies are blocked or passed with
opposite phase. The Scherzer image is important because it is (an approximation
to) a projection of the specimen structure (to a limited resolution) in the
direction of the incident beam. For images obtained at the Scherzer "optimum"
defocus, the Scherzer resolution is generally defined by the upper limit of the
low-frequency same-phase passband. Scherzer resolution is a function of objective
lens spherical aberration and electron wavelength.

FEG-HRTEMs can transfer spatial frequencies out to quite high values (their
information limits are much better than their Scherzer resolutions). Since we
know how linear transfer varies with objective lens defocus, we can use a series of
images to produce a single reconstructed image containing correctly-phased
components all the way out to the microscope information limit [see work by Van
Dyck, Coene and Thust]. The latest issue of Microscopy Today shows an example of a
reconstructed image with 0.78 Angstrom resolution, although the microscope used has
a Scherzer resolution of only 1.7 Angstrom.

While the phases of linearly-transferred image components can be corrected so they
can be used to extend resolution out to the microscope information limit, the
non-lnear components that create the "fringe resolution" usually transfer no new
information. These "cross-aperture" components can be frequency-doubled -- for
example, a 200 beam from the specimen may interfere with a -200 beam to create a
400 image component. Then we will see spacings of a/4 in the image even though no
information about the a/4 spacing was transferred from the specimen. If we managed
to "dis-entangle" the image's non-linear 400 component with its a/4 spacing, it
would still only provide us with information on a/2 spacings in the specimen.

So the short answer to your question is -- the difference between "line resolution"
as opposed to the "information resolution" is that an image can contain specimen
information out to the "information resolution", but any finer image spacings --
out to the "line resolution" -- are not new information about the specimen, but
were generated by non-linear interferences in the objective lens.

Mike O'Keefe

Juha Dapper wrote:

} ------------------------------------------------------------------------------
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear microscopist experts,
}
} When I read literatures, I have been all the time
} confused by the resolution definition in transmission
} electron microscopy. Could you please kindly help?
}
} For a FEG-HRTEM, what is the "line resolution" as
} opposed to the "information resolution"? What is the
} difference between each other?
}
} How could I achieve the "line resolution" and the
} "information resolution" in TEM experiments? And, how
} can I resolve (identify, or "see") the "line
} resolution" and the "information resolution"
} respectively from a state-of-the-art HREM image?
}
} Thank you for your time. Wish you a nice weekend,
}
} -Juha
}
}
}
}
} __________________________________
} Do you Yahoo!?
} Yahoo! Domains – Claim yours for only $14.70/year
} http://smallbusiness.promotions.yahoo.com/offer

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 15:36:21 2004

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I have a water chiller from 1996 (Haskris RO75 with B H M + T options).

On checking the water level today, I noticed that the water was a bit green and
hence needed to be changed.
I drained the water storage tank, removed the nylon strainer,
replaced it with a clean spare
and as luck would have it I also needed to change the drain hose.

From experience I knew that when I first change the water, there is
normally a rinsing out
of the system and a noticeable amount of algae (? greenish gunk)
comes out of the discharge
pipe and I change the water another time before adding the
anti-algecid and closing up the system.

Today I got some air into the system and when I turned it back on the
water turned so turbid
that I could not see the bottom coils in the tank. I repeated the
draining/filling cycle at least
8 times until there was only a slight greenish cast to the water and
I gave up until tomorrow.

Does anyone have any idea why this would happen now and not before?
Is there any way that I can be assured that I have removed as much of
the algae from the
system as I can, other than to keep changing the water as long as I
can see small clumps
coming out into the water tank?

Thanks in advance,
Pat Connelly
Dept. of Biology
Univ. of PA
Philadelphia, PA 19104

From MicroscopyL-request-at-ns.microscopy.com Mon May 24 15:48:37 2004

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Hi, Timothy:

I seem to recollect that Neal Rowlands, who was Shared Experimental
Facilities Manager in our Center some years ago, had done some asbestos
research at McGill U. along the lines of your question. I recall him
saying that the difference in lung damage caused by different forms of
asbestos had to do with the difference in crystal shape. The tiny-needle
shape was the nastiest.

Best regards,

Libby Shaw

} Subject: [Microscopy] RE: viaWWW: Identifying Asbestos Using optical
} Microscopy
} Date: Mon, 24 May 2004 12:26:01 -0400
} From: "Bard, Timothy J." {Timothy.Bard-at-SYLVANIA.com}
} To: "Gordon Couger" {gcouger-at-provalue.net} ,
} "Microscopy (E-mail)" {microscopy-at-ns.microscopy.com}
}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Address: MIT Room 13-4149 Tel: 617-253-5045
77 Massachusetts Avenue Email: elshaw-at-mit.edu
Cambridge, MA 02139 Fax: 617-258-6478
http://web.mit.edu/cmse/www/
****************************************************************

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 01:05:16 2004

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To Students attending M&M2004 in Savannah,
If you are a student that will be attending (or would like
to the attend) the M&M meeting in Savannah this summer, we
would appreciate your help by assisting at the sessions.
You would be volunteering as a "projectionist" for various
sessions, most likely ones you would attend anyway. There
is a training session Sunday afternoon (details when you
volunteer).

What are the benefits of volunteering? Volunteers will be
given free registration--a badge, opening night reception
ticket and a CD of the abstracts.

Who to contact:
John Shields (see address below) at jshields-at-cb.uga.edu

--
John Shields
E.M. Lab, 151 Barrow Hall
University of Georgia
Athens, GA 30602
706-542-4080

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 03:13:08 2004

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Hi,

I just want to get this clear and look at the consequences of what you
write.

If a nonlinear component of frequency 2f is present in an image, will it
have been damped by the ctf-envelope just like the corresponding linear
component of frequency f? In that case the presence of a high-resolution
component doesn't say much about the quality of a microscope or a
micrograph as long as it is unclear whether the component is linear or
frequency doubled.
Now for the practical consequences:
With what sort of specimens would you expect frequency doubling? Could
it happen with protein crystals (10-20 nm thick) using a 200 or 300 kV
microscope?

Philip

-----Original Message-----
} From: Michael O'Keefe [mailto:MAOKeefe-at-lbl.gov]

(1) "Fringe" resolution, or "line" resolution (sometimes called
"lattice-plane" resolution), is measured from the highest spatial
frequency that is present in the image intensity spectrum (and is thus
detectable in the optical diffractogram). It may include non-physical
detail, since it may include components from a "second-order" or
"non-linear" interference generating a half-spacing term with spatial
frequency up to twice that of the highest-frequency diffracted beam
passed by the objective aperture and the convergence cross-coefficient
envelope

While the phases of linearly-transferred image components can be
corrected so they can be used to extend resolution out to the microscope
information limit, the non-linear components that create the "fringe
resolution" usually transfer no new information. These "cross-aperture"
components can be frequency-doubled -- for example, a 200 beam from the
specimen may interfere with a -200 beam to create a 400 image component.
Then we will see spacings of a/4 in the image even though no information
about the a/4 spacing was transferred from the specimen. If we managed
to "dis-entangle" the image's non-linear 400 component with its a/4
spacing, it would still only provide us with information on a/2 spacings
in the specimen.

So the short answer to your question is -- the difference between "line
resolution" as opposed to the "information resolution" is that an image
can contain specimen information out to the "information resolution",
but any finer image spacings -- out to the "line resolution" -- are not
new information about the specimen, but were generated by non-linear
interferences in the objective lens.

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 05:02:13 2004

Contents Retrieved from Microscopy Listserver Archives
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On May 24, 2004, at 1:48 PM, Pat Connelly wrote:

} From experience I knew that when I first change the water, there is
} normally a rinsing out
} of the system and a noticeable amount of algae (? greenish gunk) comes
} out of the discharge
} pipe and I change the water another time before adding the
} anti-algecid and closing up the system.
}
Dear Pat,
Are you sure that the gunk is algae and not Cu oxide? If the latter,
you should consider adding a corrosion inhibitor to the water.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 06:08:07 2004

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Hi,

I thought some people might be interested in a follow-up of this
discussion.
(Don't tell me if your not, just ignore me.)

I've taken some images of carbon film on our CM120 with a brand new
LaB6-filament just to get an idea of the limitations of this microscope.

I get information limits between 15 and 5 Angstrom depending on
magnification and defocus (only "biological" defocus values) and the
information limit does not improve with decreasing magnification as
suggested by CTF-explorer. In fact the opposite is true (at least for
constant exposure levels). Some similar data for a FEG would be
interesting.

One thing is clear: Reaching 10 Angstrom and slightly better should not
be a problem with a well maintained LaB6 microscope.

For the details see the link "reference data for the CM120" at
http://www.csb.ki.se/users/philip/philown.html. This is a big word file
so you have to be patient when you download it.

Philip

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 06:31:39 2004

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Hi Bill,

That's exactly what I was thinking, as well. Do you have any good
recommendations for use as a corrosion inhibitor?

Thanks,

David

David Bell
Scientist
Electron Microscopy Lab
Millipore Corporation
80 Ashby Road
Bedford, MA 01730
(781) 533-2108

Bill Tivol {tivol-at-caltech.edu}
05/24/2004 06:24 PM

To: microscopy-at-msa.microscopy.com
cc:
Subject: [Microscopy] [Detected by Millipore as possible Spam] Re: Haskris water
chiller/recycler

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On May 24, 2004, at 1:48 PM, Pat Connelly wrote:

} From experience I knew that when I first change the water, there is
} normally a rinsing out
} of the system and a noticeable amount of algae (? greenish gunk) comes
} out of the discharge
} pipe and I change the water another time before adding the
} anti-algecid and closing up the system.
}
Dear Pat,
Are you sure that the gunk is algae and not Cu oxide? If
the latter,
you should consider adding a corrosion inhibitor to the water.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 07:53:51 2004

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Bill
I'm pretty sure I have Cu oxide along the walls of my Haskris
chiller as it won't come off. What corrosion inhibitor do you suggest
and how do I remove the Cu oxide already present?

Tony Greco

--
Anthony M. Greco
Electron Microscope Manager
College of Marine Science
University of South Florida
140 7th Avenue S.
St. Petersburg, Fl 33701

voice: (727) 553-1595
email: tgreco-at-marine.usf.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 08:53:39 2004

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I'm glad that this issue is still being addressed. I have a Haskris chiller
(since 1988) which services our Philips CM10 TEM. We continually have this
"green algae" in the water and which seems to collect around the filter unit
in the system. I have been concerned about this in the past, and asked our
service engineer, but it doesn't appear to impede the flow of water or the
operation of the chiller. (We have had other minor problems with the
chiller that B & G has fixed, but nothing connected to the water). I was
interested to hear about the possibility of it due to Cu oxide. I would
also like to know what corrosion inhibitor can be added to the water.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: David_Bell-at-millipore.com [mailto:David_Bell-at-millipore.com]
Sent: Tuesday, May 25, 2004 7:43 AM
To: Bill Tivol
Cc: microscopy-at-msa.microscopy.com

Hi Bill,

That's exactly what I was thinking, as well. Do you have any good
recommendations for use as a corrosion inhibitor?

Thanks,

David

David Bell
Scientist
Electron Microscopy Lab
Millipore Corporation
80 Ashby Road
Bedford, MA 01730
(781) 533-2108

Bill Tivol {tivol-at-caltech.edu}
05/24/2004 06:24 PM

To: microscopy-at-msa.microscopy.com
cc:
Subject: [Microscopy] [Detected by Millipore as possible
Spam] Re: Haskris water
chiller/recycler

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On May 24, 2004, at 1:48 PM, Pat Connelly wrote:

} From experience I knew that when I first change the water, there is
} normally a rinsing out
} of the system and a noticeable amount of algae (? greenish gunk) comes
} out of the discharge
} pipe and I change the water another time before adding the
} anti-algecid and closing up the system.
}
Dear Pat,
Are you sure that the gunk is algae and not Cu oxide? If
the latter,
you should consider adding a corrosion inhibitor to the water.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 08:56:31 2004

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Thank you, Michael and Bill, for your kind reply. I
really appreciate your remarkable answers to my
questions.

After carefully reading your answers, I've got more
questions.

1. If the "line resolution" is so confusing and
untrustworthy, why TEM manufactures used to apply it
to claim the quality of a microscope?

2. If an HREM iamge was taken without a certain
objective aperture, how can we tell if a
high-frequency spacing present in the image (or the
corresponding spot in its FFT) is due to linear
transfer or just by "cross-aperture" non-linear
interference?

3. About the "non-linear interferences". Do they
happen already during the process of electron-specimen
interaction, or after the back-focal plane of the
objective lens during the electron wave propagation?

4. In Michael's email, it is said "Since we know how
linear transfer varies with objective lens defocus, we
can use a series of images to produce a single
reconstructed image containing correctly-phased
components all the way out to the microscope
information limit [see work by Van Dyck, Coene and
Thust]."

Did you mean that the reconstruction method using a
focal-series can only apply to the linear transfer
case, i.e. the case of a weak phase object? If not,
how the non-linear interference effects are treated?

5. In Bill's email, you mentioned that "The
information limit is best seen by shifting the image
during the exposure. This produces Young's fringes in
the power spectrum,".

Could you please tell me in more details about how to
"shift the image to produce Young's fringes"? This
may be very practical and helpful to me.

Again thank you very much for your instructions.

-juha

__________________________________
Do you Yahoo!?
Friends. Fun. Try the all-new Yahoo! Messenger.
http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 10:42:49 2004

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The Microscopy ListServer -- Sponsor: The Microscopy Society
of America On May 24, 2004, at 1:48 PM,
Pat Connelly {psconnel-at-sas.upenn.edu} wrote:
} } From experience I knew that when I first change the water,
there is normally a rinsing out of the system and
a noticeable amount of algae (? greenish gunk) comes out
of the discharge pipe and I change the water another time
before adding the anti-algecid and closing up the system. etc.
} }
} Dear Pat,
} Are you sure that the gunk is algae and not Cu oxide?
} If the latter, you should consider adding a corrosion
} inhibitor to the water.
} Bill Tivol, PhD
} EM Scientist and Manager
} Cryo-Electron Microscopy Facility
} Broad Center, Mail Code 114-96
} California Institute of Technology
} Pasadena CA 91125
} (626) 395-8833 tivol-at-caltech.edu
=======
Bill,
I took a sample from the fourth change of water and examined it
under a light microscope. I saw mostly tiny cellular clumps and
cellular sheets with a few very small, redish, spike like, crystals
embedded into them and that is why I thought of algae.
I do agree that the green color most likely comes from the copper
because there is no light in the system for photosynthesis.
I have sprinkled dichlorophene onto the water each time that
I have changed it since the first fill-up. The label states that
it is both a fungicide and a bactericide.
As the water supply, I use reverse osmosis water and some
Philadelphia tap water so that there are some ions.
The ph of both sources is usually acid, running about pH 5.5.
I did not check the pH of the water that I drained yesterday
but after rinning overnight the water resevoir is now also at
pH 5.5.

I am interested in your response as to a corrosion inhibitor.
Pat Connelly

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 12:24:55 2004

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Rosemary;
My recollection from the asbestos work I did at Lockheed was
that most of the asbestos fibers could produce mesothelioma, but that in
North America, chrysotile is the predominant type of asbestos. Sources
of exposure vary, but the connection to mesothelioma was first noticed
after WWII when a significant population that also smoked heavily was
involved in refitting steam ships that had large amounts of asbestos
insulation. The death of actor Steve McQueen highlighted the fact that
even something like dirt bike riding in areas naturally high in asbestos
could lead to a high risk exposure.

John Mardinly
Intel

-----Original Message-----
} From: Rosemary White [mailto:Rosemary.White-at-csiro.au]
Sent: Sunday, May 23, 2004 4:28 PM
To: microscopy-at-msa.microscopy.com

This is off the topic of identifying asbestos, but thought I should
comment
that just yesterday there was a program on the radio (streaming audio
available at http://www.abc.net.au/rn/talks/bbing/, transcript available
by
Thursday) about new cases of asbestosis and mesothelioma showing up.
The
young people (20s and 30s) now getting this lived in high asbestos areas
as
kids, were children of builders (and builders themselves) who demolished
or
renovated fibro houses, etc. Perhaps just an Australian problem....
Rosemary

} From: "Gordon Couger" {gcouger-at-provalue.net}
} Date: Sat, 22 May 2004 16:09:06 -0500
} To: "Chiphead" {chiphead-at-sbcglobal.net} , "'by way of
MicroscopyListserver'"
} {antuni-at-aol.com} , {microscopy-at-ns.microscopy.com}
} Subject: [Microscopy] Re: RE: viaWWW: Identifying Asbestos Using
ptical
} Microscopy
}
}
}
}
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America
} To Subscribe/Unsubscribe --
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} On-Line Help
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------}
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}
} Only one of the forms of asbestos is harmful to humans. Chrysotile
} and then only if it is inhaled and the particle size is such it
} lodges in the lung so it can form a site for cancer to get a start.
} Chrysotile is only a small percentage of asbestos and the particle
} size must fall in the 5 to 15 micron range to stay in the lungs.
}
} These conditions are almost only found in asbestos worker and miners
} and not in the general public. In the case of high exposure to
} asbestos cigarette smoking is also a very large contributor to the
} cancer caused by asbestos.
}
} Had the asbestos studies been allowed to be fully peer reviewed
} before legislation was passed we would probably still be using
} asbestos in many applications today with more protection for
} asbestos workers and minors and restrictions on some products such
} as asbestos powder and asbestos cloth. Unfortunately the legislators
} won't review thier laws once they are passed and the western world
} is spending needless billions of dollars in asbestos abatement in
} every old building that is renovated.
}
} Gordon
} Gordon Couger gcc-at-couger.com
}
} I collect links on information related to light microscopes.
} http://www.couger.com/microscope/links/gclinks.html
} Please forward any links or information you think might be useful to
} others.
} Microscope Manual at www.science-info.org
}
} } From: "Chiphead" {chiphead-at-sbcglobal.net}
}
} :
} : Warning: Non scientific answer:
} :
} : I remember an edition of "This Old House" or one of those types of
} shows
} : where they took some shingle samples to a lab for testing.
} :
} : The lab used polarized microscopy to do at least an "initial"
} screening
} : and determine that the shingles "most likely" contained asbestos.
} :
} : The "would do some additional testing" to verify (it was, and the
} house
} : needed to have a tent built around it, etc., etc.). I assume the
} : additional testing was something along the lines of TEM, etc.
} :
} : The conclusion I drew was that if you had materials that you were
} : expecting asbestos, this (polarized examination) was a good
} screening
} : tool. If the fibers didn't change from one specific color to
} another as
} : the analyzer was rotated, you didn't have asbestos. If they did,
} you
} : probably have asbestos, but there are other fibers that may do the
} same
} : thing.
} :
} : These were also fibers, not dust, and I don't know if that would
} affect
} : the results or not.
} :
} : Sorry if this wasn't useful.
} :
} : John R.
} :
} : -----Original Message-----
} : } From: by way of MicroscopyListserver [mailto:antuni-at-aol.com]
} : Sent: Saturday, May 22, 2004 9:23 AM
} : To: microscopy-at-ns.microscopy.com
} : Subject: [Microscopy] viaWWW: Identifying Asbestos Using
ptical
} : Microscopy
} :
} :
} :
} : ------------------------------------------------------------------
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} : ------------------------------------------------------------------
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} : -------
} :
} : Below is the result of your feedback form (NJZFM-ultra-55). It
} was
} : submitted by (antuni-at-aol.com) from
} : http://microscopy.com/MicroscopyListserver/MLFormMail.html on
} Friday,
} : May 21, 2004 at 16:19:26
} : ------------------------------------------------------------------
} ------
} : ---
} :
} : Email: antuni-at-aol.com
} : Name: Anthony Ribaudo
} :
} : Organization: Consultant
} :
} : Title-Subject: [Microscopy] [Filtered] Identifying Asbestos
} Using ptical
} : Microscopy
} :
} : Question: Can one identify asbestos only utilizing optical
} microscopy
} : without the aid of electron diffraction/TEM ?
} :
} :
} : Anthony Ribaudo
} :
} :
} :
} : ------------------------------------------------------------------
} ------
} : ---
} :
} :
} :
} :
} :
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 12:56:12 2004

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Dear Listers,

Does anyone else think it might be a useful exercise to try and
establish expiration dates for chemicals used in microscopy labs? I
understand that chemicals "expire" based upon what they are, what use
they are intended for, how they are used, what level of
accuracy/repeatability/etc. is expected from their use, how they are
stored, and many other factors. I have also read Rande Kline's
discussion of the problem in the July/August 2000 Microscopy Today on
the difficulties of establishing such dates (recommended).

The problem is that some work requires lab certification and strict
laboratory guidelines requiring that all chemicals be labeled with
expiration dates----whether or not those dates have any meaningful or
consistent basis in "reality". So far, I've been unable to find any
such set of standards and my strong impression is that labs set up their
own arbitrary chemical rotation regimen.

It might reasonably be suggested that MSA could be a clearinghouse for
establishing such standards for microscopy-related research. If enough
people think this is a useful project, I would be willing (please
somebody, stop me!!) to volunteer to put together a draft proposal. As
a starter, it would be useful to know how other labs handle this issue
and why.

Any thoughts?

Thanks,
Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 13:36:42 2004

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I've had a similar problem with my chiller system, though mine got clogged
up pretty well before I figured out what was going on. The turbo pump in my
SEM was the culprit, I think. The water jacket on the turbo is aluminum and
there are lots of brass fittings in the Haskris and the heat sinks in the
SEM. I got a bunch of stuff that looked like green kitty litter out of the
system that proved to have high aluminum and copper levels in it. I think
there is some sort of an electrochemical gradient set up that causes some
sort of corrosion product to build up over time (I'm a biologist, not a
chemist). Small amounts of it look like green sand in the bottom of the
reservoir. I cleaned the bigger clogs out of the water jacket with
alternating dilute HCl and NaOH using a big syringe and Tygon tubing,
rinsing with DIW in between (Rube Goldberg lives on). It's been fine for a
few months now, but I keep an eye on the flow rates.

Robert Simmons

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 14:18:48 2004

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On May 25, 2004, at 4:43 AM, David_Bell-at-millipore.com wrote:

} That's exactly what I was thinking, as well. Do you have any good
} recommendations for use as a corrosion inhibitor?
}
Dear David,
When I was at Albany NY, we used a product called Aquatreet 42, a
Mo-based inhibitor, and, judging from measurements of the water flow
through the lenses each year, there was little corrosion build-up.
That product can be obtained in a minimum of 5 gal--enough to last a
lifetime--from Aqua Labs, Inc., P.O. Box 645, Amesbury MA 01913. I
just spoke recently with Tom Cass, (800) 343-0213, and they still sell
the product to people in your area. He also told me that Skasol makes
a comparable product for the West Coast people. David Marchman, (800)
839-1000, is the contact for Skasol, and Chris Killian, (310) 749-8807
is the technical person. I have no affiliation with Aqua except as a
satisfied customer, and none with Skasol except as a potentially
satisfied customer.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 14:25:29 2004

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Hi,
Try dissolving it in 10% HCl. If it disappears its a Cu compound.

Best Regards,

Steve

Steve Buckingham
Service Manager
Kratos Analytical Inc.,
100 Red Schoolhouse Road, Bldg A
Chestnut Ridge, NY 10977
ph (845) 426 6700 ext 202
fx (845) 818 {mailto:4095steve-at-kratos.com} 4095

steve-at-kratos.com

-----Original Message-----
} From: psconnel-at-sas.upenn.edu [mailto:psconnel-at-sas.upenn.edu]
Sent: Tuesday, May 25, 2004 11:54 AM
To: Bill Tivol
Cc: Microscopy-at-msa.microscopy.com

----------------------------------------------------------------------------
--
The Microscopy ListServer -- Sponsor: The Microscopy Society
of America On May 24, 2004, at 1:48 PM,
Pat Connelly {psconnel-at-sas.upenn.edu} wrote:
} } From experience I knew that when I first change the water,
there is normally a rinsing out of the system and
a noticeable amount of algae (? greenish gunk) comes out
of the discharge pipe and I change the water another time
before adding the anti-algecid and closing up the system. etc.
} }
} Dear Pat,
} Are you sure that the gunk is algae and not Cu oxide?
} If the latter, you should consider adding a corrosion
} inhibitor to the water.
} Bill Tivol, PhD
} EM Scientist and Manager
} Cryo-Electron Microscopy Facility
} Broad Center, Mail Code 114-96
} California Institute of Technology
} Pasadena CA 91125
} (626) 395-8833 tivol-at-caltech.edu
=======
Bill,
I took a sample from the fourth change of water and examined it
under a light microscope. I saw mostly tiny cellular clumps and
cellular sheets with a few very small, redish, spike like, crystals
embedded into them and that is why I thought of algae.
I do agree that the green color most likely comes from the copper
because there is no light in the system for photosynthesis.
I have sprinkled dichlorophene onto the water each time that
I have changed it since the first fill-up. The label states that
it is both a fungicide and a bactericide.
As the water supply, I use reverse osmosis water and some
Philadelphia tap water so that there are some ions.
The ph of both sources is usually acid, running about pH 5.5.
I did not check the pH of the water that I drained yesterday
but after rinning overnight the water resevoir is now also at
pH 5.5.

I am interested in your response as to a corrosion inhibitor.
Pat Connelly

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 14:33:40 2004

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On May 25, 2004, at 4:11 AM, Philip Koeck wrote:

} I get information limits between 15 and 5 Angstrom depending on
} magnification and defocus (only "biological" defocus values) and the
} information limit does not improve with decreasing magnification as
} suggested by CTF-explorer. In fact the opposite is true (at least for
} constant exposure levels). Some similar data for a FEG would be
} interesting.
}
Dear Philip,
One of the acceptance tests for our Tecnai F30H was that we had to see
30 Thon rings at 2 um underfocus on a thin C specimen, which is
slightly beyond the 0.34 nm graphite spacing. We redo this test
periodically to be sure that the coherence of the beam is still up to
par. In fact, the service engineers were able to get many more Thon
rings than that. The spec on the info limit is 0.14 nm, but we can't
get Thon rings that far out at 2 um underfocus. To get the 30 Thon
rings, one has to find a good area of the C film, so we don't expect
that good a performance for biological specimens.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 15:42:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (amcelwai-at-bucknell.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, May 25, 2004 at 14:55:05
---------------------------------------------------------------------------

Email: amcelwai-at-bucknell.edu
Name: Andrew

Organization: Bucknell University Biology Department

Title-Subject: [Microscopy] [Filtered] MListserver: New Text/Manual

Question: Hi all,

I am a graduate student at Bucknell University and I am currently studying amphibian physiology. My thesis project involves studying skeletal muscles and liver tissue using both transmission electron microscopy, and light microscopy. I am interested in learning about new techniques in microscopy, or histology and I was hoping that someone could recommend a book that covers curent methodologies and, or the best ways of doing histology/microscopy research. All of the literature I have is from the 70's and the 80's and some of my colleagues suggested to me that my sources of information are a tad bit outdated.

I would appreciate any feedback. Thanks.

-Andrew

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 17:22:31 2004

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Hi everyone

I need some help.

I have used nanoplast resin for the first time following instructions
provided with the kit. When I came to examine the sections I found there
had been poor infiltration. I would welcome any suggestions from people
that have worked with the resin that could resolve this plus any other help
tips. Do I need to do a resin infiltration series similar to Araldite. I
did email Pelco (manufacturer of the resin) about this but so far not had a
response.

thanks Therese

From MicroscopyL-request-at-ns.microscopy.com Tue May 25 19:14:18 2004

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Dear Tony,

I had an Ice Wagon and a Nesslab chiller system. The green color you see
MIGHT BE algae. Everyone blames the green color on algae.

I know from chiller experience and being a chemist that copper pipes
corrode first to a black thin film of copper oxide material on the walls of
chiller copper pipes. Next a deposit of copper carbonate forms over the
initial copper oxide coating and on PE cartridge filters. The black color
only forms on copper surfaces.

Green deposits in chiller lines in my lab were always thicker AFTER going
through a diffusion pump. We had whole house filters before the DPs and
they collected a green scale. The lines between the filter and the DP
inlet were relatively clear of green deposits. Seems backwards, doesn't
it? FYI.

TESTING:
Remove the scale and look under a microscope as you add dilute HCl. If it
bubbles, it's most likely lime green copper carbonate, as I had. To find
out if it was copper and carboante, I would use the regular green water to
test for copper ions first. Take the green chiller solution and add HCl.
It will dissolve the turbidity and form a nice clear green solution. Add
enough ammonium hydroxide to make the solution fairly basic. If copper
ions are present, the solution will turn deep blue. Algae do not do this.
Next add more HCL and the solution will turn green again. If your solution
does this, it's copper carbonate. If you would like to reconfirm the blue
color again, you can repeat the NH4OH treatment on the same sample of
water. This reversible color change is not possible with algae. IMHO.

To test for carbonate, add some HCl to a new sample to just barely get a
clear solution. Adjust the pH to 7-9 with ammonium hydroxide. Don't use
NaOH as it has carbonate in it. Add some clear barium chloride solution to
this basic solution. Enough carbonate ions will remain dissolved to cause
a white precipitate of BaCO3 to form. That probably confirms the gas was
originally CO2. If you then add HCl, the white barium carbonate
precipitate disappears to form carbonic acid and barium chloride. This
chemical behavior confirms CO3 for sure.

If you find the problem is algae, then you can add a small amount of a
quaternary ammonium salt. This extremely long named chemical will end with
quaternary ammonium salt and can be bought at any swimming pool supply as
an algicide. Estimate the volume of your system and add the recommended
amount. As I recall, a quart treats about 5,000 to 10,000 gallons of pool
water. So you will add a very small amount, like teaspoons or tablespoons
of it. It will kill the algae, if that's really the problem. Any pool
owner can help you that uses iso-cyanurates for hypochlorous acid
(chlorine) disinfection. He might give you a few mls and save you the trip
to the pool store for a 40 year chiller supply of QAS long chained
surfactant.

You can state, "I have plastic pipes, so where is the copper coming from in
my system?" Our chiller coils were made of copper tubing and the reservoir
tank had copper tubing showing in our units. They're the source of the
copper ions. In our system we also had copper supply lines going to
various labs. A mistake! There are other copper sources too. Ask your
serviceman about potential EM sources like embedded lens cooling lines of
fittings.
Air is normally the source of the CO2 because the tank is normally open to
air.

} From experience, we learned the hard way to run distilled water. I then
put a tablespoon of bicarbonate of soda in the water in case the chiller
water tried to go acidic. This trace ion concentration cuts down on the
corrosive nature of pure distilled water. This bicarb is not necessary,
unless you know the pH in your system drops over time. "Isn't that the
source of the carbonate?" No, we had the problem when we used chloramine-T
and no bicarb. We used bicarb after we switched to distilled water for
trace ions and to slow down any decrease in pH.

You can get into a green color spiral with chloramine-T (CT). You add CT
and the water eventually turns green. You measure the available chlorine
after awhile and it's too low. You add more CT and the available chlorine
goes up. After some time the available chlorine drops and the green color
intensity increases. You add more CT. The water keeps 'growing algae' and
turning a darker green all the time. Copper levels continue to climb and
precipitate.
We went this route and finally I said, "There is no way we logically have
this bad an algae problem." I had saved samples along the way and so I ran
AA on them and did the blue-green test. I found out that the more CT we
added, the more the copper ion concentration increased along with the
darker green color. All this led me to the correct answer.
It's copper carbonate in the water and on the walls of the pipes, not algae!

We replaced the coppper lines to labs and I saved the green scale from
inside the copper pipes. After 4 years, the dried 'green algae' are still
green because the green scale is really copper carbonate.

Disclaimer: Some algae might be present with the carbonate but AA
confirmed the copper increased with CT addition and time. This green color
can develop with pure distilled water also. It just takes longer.

Everything you ever wanted to know about green chiller water but were
afraid to ask.

What do you do if you have reduced flow through your TEM or SEM lens
cooling lines, DP lines, rubber hoses, or electronic heat sinks? Check
with your serviceman. Let him do those jobs and assume the risk.

Paul Beauregard
Senior Research Associate
travail chasse

At 08:57 AM 05/25/04 -0400, Tony Greco wrote:
}
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From MicroscopyL-request-at-ns.microscopy.com Wed May 26 04:18:27 2004

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That's another question I've just come across.

I have some test images (defocus around 1000 nm) from a FEG-TEM where
Young fringes seem to extend up to twice as far as Thon rings. Is that
usual and if so which of the two defines the information limit?
What do manufacturers mean by information limit?
Do Young fringes really show up to which resolution I can get useful
information from a micrograph?
At least in TEM of non-periodic biological specimens you normally don't
expect anything beyond the last clearly visible Thon ring.

Philip

-----Original Message-----
} From: Juha Dapper [mailto:juha_dapper-at-yahoo.com]

5. In Bill's email, you mentioned that "The
information limit is best seen by shifting the image
during the exposure. This produces Young's fringes in
the power spectrum,".

Could you please tell me in more details about how to
"shift the image to produce Young's fringes"? This
may be very practical and helpful to me.

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 05:21:43 2004

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I think this is a good idea. I am still using chemicals
that predate my start here (1989). I had to renew some
sodium phosphate this year when the plastic container
disintegrated! More seriously I have started making up
sodium cacodylate 0.2M stock and adding a set volume of HCL
(from Glauert's book) just before use. As my flagon of HCL
is over 15yrs old I replaced it this week with a supply
from a lab with a higher turnover. I plan to replace the
HCL annually unless someone comes up with an informed
suggestion!

Dave

On Tue, 25 May 2004 13:08:29 -0500 "Tindall, Randy D."
{TindallR-at-missouri.edu} wrote:

}
}
} ------------------------------------------------------------------------------
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} -------------------------------------------------------------------------------
}
} Dear Listers,
}
} Does anyone else think it might be a useful exercise to try and
} establish expiration dates for chemicals used in microscopy labs? I
} understand that chemicals "expire" based upon what they are, what use
} they are intended for, how they are used, what level of
} accuracy/repeatability/etc. is expected from their use, how they are
} stored, and many other factors. I have also read Rande Kline's
} discussion of the problem in the July/August 2000 Microscopy Today on
} the difficulties of establishing such dates (recommended).
}
} The problem is that some work requires lab certification and strict
} laboratory guidelines requiring that all chemicals be labeled with
} expiration dates----whether or not those dates have any meaningful or
} consistent basis in "reality". So far, I've been unable to find any
} such set of standards and my strong impression is that labs set up their
} own arbitrary chemical rotation regimen.
}
} It might reasonably be suggested that MSA could be a clearinghouse for
} establishing such standards for microscopy-related research. If enough
} people think this is a useful project, I would be willing (please
} somebody, stop me!!) to volunteer to put together a draft proposal. As
} a starter, it would be useful to know how other labs handle this issue
} and why.
}
} Any thoughts?
}
} Thanks,
} Randy
}
} Randy Tindall
} EM Specialist
} Electron Microscopy Core Facility---We Do Small Well!
} W122 Veterinary Medicine
} University of Missouri
} Columbia, MO 65211
} Tel: (573) 882-8304
} Fax: (573) 884-5414
} Email: tindallr-at-missouri.edu
} Web: http://www.biotech.missouri.edu/emc/
}
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 07:45:01 2004

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Hi, Philip,

According to the previous email by Mike O'Keefe,
"Increased underfocus will push the
convergence-limited damping function to higher
frequencies," and in my own opinion, magnification
should be high enough to show up the information
limit. Did you compare Young fringes and Thon rings on
the same scale with high enough MAG and underfocus?

By the way, could you describe how to produce Young
fringes with your microscope? Thanks.

Juha

--- Philip Koeck {Philip.Koeck-at-biosci.ki.se} wrote:
}
}
}
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} Microscopy Society of America
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}
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}
} That's another question I've just come across.
}
} I have some test images (defocus around 1000 nm)
} from a FEG-TEM where
} Young fringes seem to extend up to twice as far as
} Thon rings. Is that
} usual and if so which of the two defines the
} information limit?
} What do manufacturers mean by information limit?
} Do Young fringes really show up to which resolution
} I can get useful
} information from a micrograph?
} At least in TEM of non-periodic biological specimens
} you normally don't
} expect anything beyond the last clearly visible Thon
} ring.
}
} Philip
}
} -----Original Message-----
} } From: Juha Dapper [mailto:juha_dapper-at-yahoo.com]
}
}
} 5. In Bill's email, you mentioned that "The
} information limit is best seen by shifting the image
} during the exposure. This produces Young's fringes
} in
} the power spectrum,".
}
} Could you please tell me in more details about how
} to
} "shift the image to produce Young's fringes"? This
} may be very practical and helpful to me.
}
}
}

__________________________________
Do you Yahoo!?
Friends. Fun. Try the all-new Yahoo! Messenger.
http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 13:53:32 2004

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I have been watching the discussion on TEM resolution with great interest and am very impressed by the power of some of the more recent models of TEM.

As a contribution to this discussion, I think it is important to remind everyone that instrument resolution is only half of the story. We must also take into account the resolution available in the specimen. For the people using these modern microscopes and imaging biological specimens at high resolutions it is taken for granted that optimal specimen preparation has occurred. Usually this means that small particles have been vitrified in the thin film of water and then imaged while still frozen.

For most people who use aldehyde-fixed and embedded sections, or for people who are just starting in EM, it is important to remember that high resolution electron microscopes are not much use for examining their samples. The reason being that the aldehyde fixation and subsequent dehydration at ambient temperature will either extract or condense the biological molecules. The end result is that there is no high resolution detail to examine in the specimens.

Better specimen preparation protocols are available for resin sectioners but they come at a price. Recent work has clearly shown that high pressure freezing followed by freeze substitution is able to preserve biological material better than the conventional methods. This approach may become the routine specimen preparation method of the future.

Until then, we have to keep our eyes open for the many fixation artifacts, including extraction and condensation, that are common in the scientific literature. There is a large community of scientists who know very little about EM but who are in positions where they review scientific literature and reseach grants. They need to know our strengths and limitations.

Regards,

Paul Webster.

Paul Webster, Ph.D.
House Ear Institute
2100 West Third Street
Los Angeles
CA 90057
phone (213) 273 8026
fax (213) 413 6739
email: pwebster-at-hei.org

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 16:44:51 2004

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Fellow List Members,

The Midwest Microscopy and Microanalysis Society has held student poster
competitions in the past, and would like to begin doing so again. The
Executive Council plans to review our previous practices and those of
the MSA, but we would also like input from Affiliate Societies or other
groups about guidelines for sponsoring a successful student poster
competition. Suggestions as to how you handle issues such as
eligibility, format judging, combining or separating materials science
and biological, etc., would be welcome.

Please send replies directly to me at eschumacher-at-mccrone.com. Your
input is very much appreciated.

Elaine Schumacher
Materials Science Director
Midwest Microscopy and Microanalysis Society

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 17:13:59 2004

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Fellow Listmembers,

Our Mini-Workshop Series on "Cryoultramicrotomy for Materials Sciences" is
coming to Texas!

The first session will be held at the University of Texas-Austin. Details
are given below.

When:
Wednesday, June 16 and Thursday, June 17, 2004, 9:00am-4:00pm

Where:
Department of Chemical Engineering
Room 2.222, Chemical and Petroleum Engineering Building
(Ground Floor)
Speedway and Dean Keeton Streets
University of Texas at Austin
Austin, TX 78712

(Parking structure is located just across Speedway from the Chemical and
Petroleum Engineering Building. Pay as you leave; credit cards accepted.)

What:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair
probes), glass knife making, evaluation of glass knives, care and cleaning of
diamond knives and operation of the cryoultramicrotome.

Attendees are welcome to bring specimens to the workshop. If you will be
bringing specimens, please let us know the nature of your specimens when you RSVP
and reserve a place in the workshop (see below).

Background:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing" at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

Important Info:
There is no charge for this workshop.
Meals and refreshments will be served!
Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryoultramicrotomy
hands-on sessions on the second day.

Contacts:
To RSVP and to reserve a spot for the hands-on sessions, please contact
either Kim Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262)
or Graham Bird at Atomic Spectroscopy Instruments, Inc.
( {grbird-at-thegateway.net} , 512-695-8865).

Sponsors and Organizers:
University of Texas at Austin
Department of Chemical Engineering (Dr. Don Paul's Group)
RMC Products Group, Boeckeler Instruments, Inc.
Atomic Spectroscopy Instruments, Inc.

See you in Austin!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 17:34:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (maloneyb-at-fiu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, May 26, 2004 at 13:57:23
---------------------------------------------------------------------------

Email: maloneyb-at-fiu.edu
Name: Barb

Organization: FIU/FCAEM

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Group: what are the advantages to having a Pana CL and a cold stage hooked up to your LV SEM? I'm asking for all applications across the board, not just semi-conductors, etc. would like to see biological applications too.
Thanks
Barb

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 18:30:00 2004

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In a message dated 5/26/04 7:04:06 PM Eastern Daylight Time,
eschumacher-at-mccrone.com writes:

{ {we would also like input from Affiliate Societies or other
groups about guidelines for sponsoring a successful student poster
competition} }

Elaine:

This is how we judged the posters at the NESM Spring Symposium at Woods Hole.

{ {
Judging Criteria:
The posters are not judged on their scientific merit!
The Point Scale ranges from 1-5 for each Judging Category. If the presenter
does not wish to be included in the competition, indicate "d".

Microscope Adjustment: Do the photomicrographs or images illustrate that the
microscope was properly adjusted? Is the specimen in focus? For SEM images,
did the sample charge up? Was the proper accelerating voltage used? For
light microscopes, is there a uniform field of illumination? For AFM, DIC,
Confocal, or other techniques, are the images free of distortions or artifacts?
Quality of Images: Is the subject properly in the field of view? Are the
images relatively free of lines or dust specks? Was the film or digital image
correctly printed? Is there a scale?
Clarity of Graphics: Are the graphics well-drawn? Are the axes of any
graphs labeled? Is color or black & white used effectively? Do the graphics stand
alone, or must one refer to the text?
Clarity of Text: Does the text tell the story clearly and concisely? Is any
necessary jargon clearly explained? Are complete sentences used?
Layout of Poster: Is the poster easy to follow? Are arrows or numbers used
to guide the reader from one part of the poster to the other? Is the title
and subject of the poster obvious?
Interaction with Judges: Is the presenter enthusiastic and personable? Is
the presenter professionally attired and groomed? Does the presenter answer
simple questions in a clear, concise and knowledgeable manner? (Suggestions:
What microscopes did you use for this work? When and how were they calibrated?)
} }

Steve Stokowski
President-elect
New England Society for Microscopy

Contact Information:
Stone Products Consultants
10 Clark St., Ste. A
Ashland, Mass. 01721-2145
508-881-6364 (ph. & fax)

From MicroscopyL-request-at-ns.microscopy.com Wed May 26 20:21:57 2004

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Hi Juha,

You certainly raise some interesting questions!

1. Well, if you had to sell a microscope with a point-to-point resolution of 2.4
Angstrom and an information limit of 1.4 Angstrom and a "line resolution" of 0.8
Angstrom, which figure would you mention to a customer who wanted the best high
resolution? Especially if your competitor's brochure quoted their microscope's
"line resolution". :-)

2. As you suggest, the best way is to use an objective aperture of a known size --
then any higher-frequency spots in the diffractogram of the image must be due to
"cross-aperture" non-linear interferences. A less direct way is to compare images
with simulations for a well-known specimen, assuming you have a good idea of the
microscope parameters and the specimen parameters (thickness...). Of course,
there's holography, if you have a biprism.

3. The "non-linear interferences" are part of the imaging process and will not be
present in the diffraction pattern (which is an "image" of electron distribution at
the back focal plane). The convolution that produces the interferences in the
image intensity spectrum in k-space comes from the squaring of the image amplitude
to form the image intensity in real space. Thinking another way, electrons leaving
the same position at the specimen have not yet been brought together at the back
focal plane (although electrons leaving the specimen at the same scattering angle
have).

4. The "paraboloid method" is able to extract just the linear contributions to the
images in the focal series because these contributions (sums of interferences)
occupy different positions to those of the non-linears in the 3-space generated by
the 3-D FFT of a set of images "stacked" in order of defocus. The 3-D "super
diffractogram" has the usual u and v axes (in the x,y planes of the images) while
the vertical w axis has the dimension of one over defocus. Then the linears lie on
a paraboloid in this space, while the non-linears are off the paraboloid and can be
filtered out, allowing the reconstruction of the exit-surface wave from just the
linear terms. See, for example, M&M 2002, (Quebec, Canada) 474-475 by Tadahiro
Kawasaki and Yoshizo Taka, and reference [16] at
http://nano.cirse.nagoya-u.ac.jp/kawa-paperlist.html

5. One way is to take two exposures with a shift of 10 or so Angstrom between
them, then add and FFT. Another is to introduce an abrupt image shift halfway
through the exposure of a single image, then FFT. A shift with the image-shift
coils avoids the danger of vibration that could occur with a shift of the
specimen. Young's fringes will occur at frequencies where features in the two
images are correlated -- the high-frequency noise will be different in each image
and thus not produce fringes. However, any second-order (non-linear) detail will
be present in both images. I think an image shift of 10 Angstrom will produce 10
fringes out to the 1 Angstrom point in the diffractogram.

I look forward to the next set of questions!

Michael

Juha Dapper wrote:

} ------------------------------------------------------------------------------
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} -------------------------------------------------------------------------------
}
} Thank you, Michael and Bill, for your kind reply. I
} really appreciate your remarkable answers to my
} questions.
}
} After carefully reading your answers, I've got more
} questions.
}
} 1. If the "line resolution" is so confusing and
} untrustworthy, why TEM manufactures used to apply it
} to claim the quality of a microscope?
}
} 2. If an HREM iamge was taken without a certain
} objective aperture, how can we tell if a
} high-frequency spacing present in the image (or the
} corresponding spot in its FFT) is due to linear
} transfer or just by "cross-aperture" non-linear
} interference?
}
} 3. About the "non-linear interferences". Do they
} happen already during the process of electron-specimen
} interaction, or after the back-focal plane of the
} objective lens during the electron wave propagation?
}
} 4. In Michael's email, it is said "Since we know how
} linear transfer varies with objective lens defocus, we
} can use a series of images to produce a single
} reconstructed image containing correctly-phased
} components all the way out to the microscope
} information limit [see work by Van Dyck, Coene and
} Thust]."
}
} Did you mean that the reconstruction method using a
} focal-series can only apply to the linear transfer
} case, i.e. the case of a weak phase object? If not,
} how the non-linear interference effects are treated?
}
} 5. In Bill's email, you mentioned that "The
} information limit is best seen by shifting the image
} during the exposure. This produces Young's fringes in
} the power spectrum,".
}
} Could you please tell me in more details about how to
} "shift the image to produce Young's fringes"? This
} may be very practical and helpful to me.
}
} Again thank you very much for your instructions.
}
} -juha
}
}
}
} __________________________________
} Do you Yahoo!?
} Friends. Fun. Try the all-new Yahoo! Messenger.
} http://messenger.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 04:30:37 2004

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Barb writes ...

} Question: Dear Group: what are the advantages to having
} a Pana CL and a coldstage hooked up to your LV SEM? I'm
} asking for all applications across the board, not just
} semi-conductors, etc. would like to see biological
} applications too.

Speaking for CL from quartz, a cold stage does indeed increase the
luminescence, but we found it disapponiting. That is, it didn't raise the
CL from unique areas, (rather than from everywhere), and contrast from
regions of unique emission was reduced. Moderate gain can come from
lowering the temp to a range of 0 to -30C, but I imagine this can be
accomplished with Peltier cooling rather than LN2.

hth & genuinely ... michael shaffer :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 05:20:06 2004

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Hi again,

I think I need to restate my question about expiration dates on lab
chemicals, since I may have been unclear in my first posting.

I know that expiration dates are arbitrary and maybe even meaningless in
many cases, because they depend on so many variables. However,
sometimes we are required to put them on our reagents because of rules
regarding certain research projects.

For example, if a lab should perform electron microscopy as part of a
project involving a pharmaceutical company, chances are that the company
will require certain types of documentation, traceability, instrument
calibration, standardization of methods, etc. Expiration dates on
chemicals are often (maybe always) part of such requirements.
Diagnostic work is another probable example.

My question or proposal is this: Given that we are sometimes REQUIRED to
use expiration dates, wouldn't it be reasonable if there was some
consensus in our field we could point to and say "Our lab follows the
(for example) MSA standards on chemical usage."? As it is, I have not
yet been able to locate a set of standards to guide us in any sort of
meaningful compliance with such outside requirements. Phil Oshel has
suggested that the histotech community has been dealing with this for
some time, so I'm checking this out now (thanks for the suggestion,
Phil).

On the other hand, maybe this is something that doesn't need fixing,
because it ain't broke. I'm just curious what others think about it.

Thanks all.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 08:29:40 2004

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After following this discussion for a few days now, I could no longer
resist the
temptation to participate in what still, after all these years, appears
to be a
subject with a wide variety of opinions.

I spent a few years in the testing end of the asbestos business, with
most of
my time spent on a PLM. It is indeed an excellent tool for identifying
asbestos,
and, according to Mr. McCrone, just about anything that can be made to fit
on to a microscope slide. However, I must admit that it is highly
dependant
on the abilities of the microscopist, and good quality control is a
must. Having
completed one of Mr. McCrone's PLM courses, it is difficult to argue
against
even the most impressive claims regarding the PLM's capabilities, but that
was with Mr. McCrone himself at the helm, and no one knows the PLM the
way he does. (I guess that makes me a "McCrone(ie)").

My biggest concern in this discussion is the comment that only one form of
asbestos is harmful to humans. During my time in the industry I went to
a lot
of seminars and read a lot of literature on asbestos, and although I
have been
out of the business for many years now, I would be very surprised to
find out
that amosite, crocidolite and the other forms of asbestos had been found
to be
harmless. All of the minerals in the asbestos family have a similar
crystal structure.
It is that unique structure that produces the very fine fibers that get
trapped in the
lungs and, under the now considered rare conditions, causes cancer and
mesothelioma. It is true that crysotile was the most commonly used form of
asbestos, but the others are every bit as dangerous.

I have been very pleased to see that a much more reasonable approach has
been adopted by the regulatory agencies that control the industry and
originally
created such a panic throughout the country, however a part of me still
feels
that getting asbestos out of the schools might have been the one good thing
that resulted from that panic. There is obviously still a lot we do not
know
about asbestos and it's long term effects. Removing it from the
buildings that
our children spend so much time in was a reasonable precaution at the time.

Doug Price

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 10:05:16 2004

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Dear Members,

Question: In the TEM, the exit wave (the wave leaving
the specimen)is complex-valued in general, which can
be written as g = f1 + i*f2, where f1 and f2 are real
numbers. Is it true/false that f2 has no sign changes,
i.e. if positive, always positive?

With best regards,

Zhongyi Liu
Argonne National Lab
Argonne, IL60439

____________________________________________________________
Yahoo! Messenger - Communicate instantly..."Ping"
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From MicroscopyL-request-at-ns.microscopy.com Thu May 27 10:21:38 2004

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Elaine,

The International Metallographic Society and ASM International have been
cosponsoring the International Metallographic Contest and Exhibit since
1972. The contest is held in conjunction with the annual convention of the
International Metallographic Society, which, since 2002, has become an
intrical part of the M&M annual meeting. Entries, in the form of posters,
use photographs and captions to describe how metallography helped solve a
problem or to introduce a unique, unusual, or new metallographic technique.
The entries are mailed rather than presented, but perhaps some of the rules
and judging criteria would be applicable to your contest.

There are twelve different classes of competition in order to give everybody
a fair chance. For example light microscopy is separate from electron
microscopy, metals and their alloys are separate from other materials,
color is separate from black and white. Students are welcome to enter any of
the classes, but they are encouraged to enter the two specifically for
undergrads. That way the students are not competing directly with
professionals in their individual classes.

Please visit www.metallography.com/ims/contest.htm for additional details or
download www.metallography.com/ims/imcjudges.doc for a history of the
contest and some insight into the judging process. This year's contest is
scheduled for Saturday, July 31 in Savannah. Deadline for entries is July
19. All entries will be on exhibit for the duration of the M&M meeting. If
you'll be attending the meeting, I invite you to come visit the display.

Best regards,

Jeff Stewart
International Metallographic Contest Chair
Metallographic Laboratory Manager
Stern-Leach Co.
49 Pearl Street
Attleboro, MA 02703 USA
Phone: 508-222-7400 extension 1329
Fax: 508-699-4030
E-mail: jeff-at-metallography.com

----- Original Message -----
} From: "Elaine F. Schumacher" {eschumacher-at-mccrone.com}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, May 26, 2004 5:56 PM

Dear Michael,

Thank you for your crystal answers that really cheer
me up by clarifying those doubts hanging around my
mind so far. Your papers in Ultramicroscopy 89 (2001)
215–241 helps a lot too in understanding those
questions.

I do have another few very fundamental questions. I
really hesitate to ask without your encouragement.

In your first email, and also in the article I listed
above,(actually all people say so): at the Scherzer
defocus, there is a largest passband where all linear
spacial frequescy components are transfered to the
image with the "same sign", or say the "same-phase
passband" transfer.

To be clear,I put my questions into three as follows
although they are much related.

1. In my understanding, the phase shift that are
imposed by the objective lens on a diffracted beam is
a function of spacial frequescy (k). It means each k
component will be shifted (displaced) in the image by
a unique amount, even within the Scherzer passband. So
what does the "same-sign transfer" really mean here?
Is it true that "the same sign is in the same way"?

2. For a certain focus condition, it seems we can
divided those transfer into just two portions (in
additon to those zero-cross): "+ sign" transfer and "-
sign" transfer. However, from "+ sign" to "- sign",
the difference in phase-shift can be very little, for
instance, from 179(degree) to 181(degree). So what and
how large difference may we expect from the sign
transfer of the two k components that just transit
from + (179) to - (181)?

3. As I described above, even within the Scherzer
passband, different k components will be displaced in
the image by different amounts depending on the phase
shifts they suffer from the lens. So how to estimate
delocalization effect in a Scherzer image, especially
with a non-periodic object. And, more important, how
the delocalization effect is handled in FEG-HREM
focal-series reconstruction where such effect can be
really serious?

Thank you again.

-juha

--- Michael O'Keefe {MAOKeefe-at-lbl.gov} wrote:
}
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}
} Hi Juha,
}
} You certainly raise some interesting questions!
}
} 1. Well, if you had to sell a microscope with a
} point-to-point resolution of 2.4
} Angstrom and an information limit of 1.4 Angstrom
} and a "line resolution" of 0.8
} Angstrom, which figure would you mention to a
} customer who wanted the best high
} resolution? Especially if your competitor's
} brochure quoted their microscope's
} "line resolution". :-)
}
} 2. As you suggest, the best way is to use an
} objective aperture of a known size --
} then any higher-frequency spots in the diffractogram
} of the image must be due to
} "cross-aperture" non-linear interferences. A less
} direct way is to compare images
} with simulations for a well-known specimen, assuming
} you have a good idea of the
} microscope parameters and the specimen parameters
} (thickness...). Of course,
} there's holography, if you have a biprism.
}
} 3. The "non-linear interferences" are part of the
} imaging process and will not be
} present in the diffraction pattern (which is an
} "image" of electron distribution at
} the back focal plane). The convolution that
} produces the interferences in the
} image intensity spectrum in k-space comes from the
} squaring of the image amplitude
} to form the image intensity in real space. Thinking
} another way, electrons leaving
} the same position at the specimen have not yet been
} brought together at the back
} focal plane (although electrons leaving the specimen
} at the same scattering angle
} have).
}
} 4. The "paraboloid method" is able to extract just
} the linear contributions to the
} images in the focal series because these
} contributions (sums of interferences)
} occupy different positions to those of the
} non-linears in the 3-space generated by
} the 3-D FFT of a set of images "stacked" in order of
} defocus. The 3-D "super
} diffractogram" has the usual u and v axes (in the
} x,y planes of the images) while
} the vertical w axis has the dimension of one over
} defocus. Then the linears lie on
} a paraboloid in this space, while the non-linears
} are off the paraboloid and can be
} filtered out, allowing the reconstruction of the
} exit-surface wave from just the
} linear terms. See, for example, M&M 2002, (Quebec,
} Canada) 474-475 by Tadahiro
} Kawasaki and Yoshizo Taka, and reference [16] at
} http://nano.cirse.nagoya-u.ac.jp/kawa-paperlist.html
}
} 5. One way is to take two exposures with a shift of
} 10 or so Angstrom between
} them, then add and FFT. Another is to introduce an
} abrupt image shift halfway
} through the exposure of a single image, then FFT. A
} shift with the image-shift
} coils avoids the danger of vibration that could
} occur with a shift of the
} specimen. Young's fringes will occur at frequencies
} where features in the two
} images are correlated -- the high-frequency noise
} will be different in each image
} and thus not produce fringes. However, any
} second-order (non-linear) detail will
} be present in both images. I think an image shift
} of 10 Angstrom will produce 10
} fringes out to the 1 Angstrom point in the
} diffractogram.
}
} I look forward to the next set of questions!
}
} Michael
}
} Juha Dapper wrote:
}
} }
}
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} }
} } Thank you, Michael and Bill, for your kind reply.
} I
} } really appreciate your remarkable answers to my
} } questions.
} }
} } After carefully reading your answers, I've got
} more
} } questions.
} }
} } 1. If the "line resolution" is so confusing and
} } untrustworthy, why TEM manufactures used to apply
} it
} } to claim the quality of a microscope?
} }
} } 2. If an HREM iamge was taken without a certain
} } objective aperture, how can we tell if a
} } high-frequency spacing present in the image (or
} the
} } corresponding spot in its FFT) is due to linear
} } transfer or just by "cross-aperture" non-linear
} } interference?
} }
} } 3. About the "non-linear interferences". Do they
} } happen already during the process of
} electron-specimen
} } interaction, or after the back-focal plane of the
} } objective lens during the electron wave
} propagation?
} }
} } 4. In Michael's email, it is said "Since we know
} how
} } linear transfer varies with objective lens
} defocus, we
} } can use a series of images to produce a single
} } reconstructed image containing correctly-phased
} } components all the way out to the microscope
} } information limit [see work by Van Dyck, Coene and
} } Thust]."
} }
} } Did you mean that the reconstruction method using
} a
} } focal-series can only apply to the linear transfer
} } case, i.e. the case of a weak phase object? If
} not,
} } how the non-linear interference effects are
} treated?
} }
} } 5. In Bill's email, you mentioned that "The
} } information limit is best seen by shifting the
} image
} } during the exposure. This produces Young's fringes
} in
} } the power spectrum,".
} }
} } Could you please tell me in more details about how
} to
} } "shift the image to produce Young's fringes"?
} This
} } may be very practical and helpful to me.
} }
} } Again thank you very much for your instructions.
} }
} } -juha
} }
} }
} }
} } __________________________________
} } Do you Yahoo!?
} } Friends. Fun. Try the all-new Yahoo! Messenger.
} } http://messenger.yahoo.com/
}
}

__________________________________
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From MicroscopyL-request-at-ns.microscopy.com Thu May 27 10:46:49 2004

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randy

on the virology/tissue culture side of things we are very compulsive
about our chemistry. on the EM side we are much more lax. i have
chemicals that are up to 35 years old - no, not my glutaraldehyde and
osmium.... periodically i go on a cleaning spree and get rid of old
organics, solvents, and bottles of DMP-30. at the first hint of
moisture in acetone, ethanol or dichloroethane i discard the contents or
ship the bottles off to chemical safety for appropriate disposal. once
a year i clean out all accumulated preparations of negative and positive
stains, small as those stocks are. but i have ancient bottles of UA,
uranyl sulfate, etc. which i use to make those stains and most other
solutions.

but what is expiry, and what is a good basis for change. it is not
universally established. as an example, dogma states that PTA and UA
are only good for short periods of time, 2-3 months. i know from
controlled tests that PTA and UA are good for negative staining for up
to a year if stored correctly, but i still have them replaced every 2-3
months, although i sometimes get debate on this from the techs, an
action which i encourage.

my lab is probably very normal - especially for those headed up by my
fellow dinosaurs, who have been doing this for 30+ years.

your points are very valid, and deserve some follow up. i hope you will
post what you find from the histology community.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 11:14:28 2004

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Hi Andrew:

The princples of tissue preparation for light and/or electron
microscopy are ancient, at least by the standards your "colleagues" seem
to be using (I hope theses colleagues are not on the faculty, condeming
work based solely on the date of publication is demonstrates
ignorance). For electron microscopy, glutaradehyde fixation followed by
osmium post-fixation was worked out in the early 1960's, embedding in
epoxy resins dates from the late 1950s. Of course, the basic methods for
light microscopy are much older.
So the question is, what exactly are you trying to do? Are you
interested in applying a new technique to an older problem? If so, the
technique you select should show some promise of answering the question
you are asking! That may seem very obvious, but as all researchers
(should) know, "the road to hell is paved with good intentions." A good
experiment does not have to be fancy or use the latest hot technique.
The best work is often rather simple, the elegance residing in the
concepts of mating the question with the method used to answer it. Plus
a lot of hard work.

Geoff

by way of MicroscopyListserver wrote:

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--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 11:35:07 2004

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I've noticed over the past few months that I needed to set my ultramicrotome
thicker and thicker to get the same thin sections [using an Ultracut-E].
Finally I often ended up having to cut using the "thick" setting, and
cutting about 1.1 micrometers according to that microtome to cut thin
sections.

This was using a DDK knife that I've used for 11 years, with about 5 or 6
years on the same side of the knife. But yesterday I changed knives to a
resharpened knife, and found that I only need to set my ultratome at about
76 nanometers to get my same silver/gold sections.

Is this really what happens when one's diamond knife gets dull? - or is
this just a coincidence? This is the first time in 20 years that I've
observed this phenomenon. I'd be interested in hearing about the
experiences of others on this.

Garry Burgess

Charge Technologist
Electron Microscopy Laboratory MS-336
Department of Pathology
Health Sciences Centre
820 Sherbrook Street
Winnipeg, Manitoba, Canada
R3A 1R9

Phone: (204) - 787 -1508
Fax: (204) - 787- 2381

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 12:15:46 2004

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Dear listers,

About 2 years ago we upgraded our WDS microspec 2a unit with Oxford system,
but the old system was still operational at the time. If anyone is
interested in acquiring the old unit please contact me offline.

Regards,

Pavel Lozovyy
ATC SEM Lab
(216)692-6637
http://www.atclabs.com/SEM.htm

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 14:04:40 2004

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I could be wrong, but 5 or 6 years on a knife, without sharpening, seems a long
stretch. How much use does it get?

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Garry Burgess [mailto:GBurgess-at-exchange.hsc.mb.ca]
Sent: Thursday, May 27, 2004 12:47 PM
To: 'Microscopy-at-MSA.Microscopy.com'

I've noticed over the past few months that I needed to set my ultramicrotome
thicker and thicker to get the same thin sections [using an Ultracut-E].
Finally I often ended up having to cut using the "thick" setting, and
cutting about 1.1 micrometers according to that microtome to cut thin
sections.

This was using a DDK knife that I've used for 11 years, with about 5 or 6
years on the same side of the knife. But yesterday I changed knives to a
resharpened knife, and found that I only need to set my ultratome at about
76 nanometers to get my same silver/gold sections.

Is this really what happens when one's diamond knife gets dull? - or is
this just a coincidence? This is the first time in 20 years that I've
observed this phenomenon. I'd be interested in hearing about the
experiences of others on this.

Garry Burgess

Charge Technologist
Electron Microscopy Laboratory MS-336
Department of Pathology
Health Sciences Centre
820 Sherbrook Street
Winnipeg, Manitoba, Canada
R3A 1R9

Phone: (204) - 787 -1508
Fax: (204) - 787- 2381

This e-mail and/or any documents in this transmission is intended for the
address(s) only and may contain legally privileged or confidential information.
Any unauthorized use, disclosure, distribution, copying or dissemination is
strictly prohibited. If you receive this transmission in error, please notify
the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 16:25:21 2004

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Hi,

I was wondering if it is possible to buy sharpened scanning tunnel
microscope tips? I have a colleague who is having trouble getting a
sharp tip from Pt/Ir wire.

Bettye

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 17:20:08 2004

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False.
At least in simulated exit-waves.
For example, in simulations for GaN at 300keV, the exit-wave Argand-plane vector at
the Ga position starts at f2 = 0 for zero thickness, then describes an approximate
circle that extends from f2 = +1.3 to -1.5 electrons.
Mike

Zhongyi Liu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear Members,
}
} Question: In the TEM, the exit wave (the wave leaving
} the specimen)is complex-valued in general, which can
} be written as g = f1 + i*f2, where f1 and f2 are real
} numbers. Is it true/false that f2 has no sign changes,
} i.e. if positive, always positive?
}
} With best regards,
}
} Zhongyi Liu
} Argonne National Lab
} Argonne, IL60439
}
}
}
}
}
} ____________________________________________________________
} Yahoo! Messenger - Communicate instantly..."Ping"
} your friends today! Download Messenger Now
} http://uk.messenger.yahoo.com/download/index.html

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 17:57:57 2004

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Hi, Listers and Posters

Does anyone have any experience, positive or negative, with cleaning EPMA analysing
crystals?

TAP and PET, I suspect, as the LIF deals with harder X-Rays.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 19:00:21 2004

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}
} I've noticed over the past few months that I needed to set my ultramicrotome
} thicker and thicker to get the same thin sections [using an Ultracut-E].
} Finally I often ended up having to cut using the "thick" setting, and
} cutting about 1.1 micrometers according to that microtome to cut thin
} sections.
}
} This was using a DDK knife that I've used for 11 years, with about 5 or 6
} years on the same side of the knife. But yesterday I changed knives to a
} resharpened knife, and found that I only need to set my ultratome at about
} 76 nanometers to get my same silver/gold sections.
}
} Is this really what happens when one's diamond knife gets dull? - or is
} this just a coincidence? This is the first time in 20 years that I've
} observed this phenomenon. I'd be interested in hearing about the
} experiences of others on this.
}
} Garry Burgess
}
Garry -

Not enough information here. What sort of samples do you cut? How
did you clean the old knife? Do both knives have the same clearance
and cutting angles?

Caroline

--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Thu May 27 19:39:18 2004

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You may be amused that this e-mail, with the original title reference
to "Thick and Thicker", was flagged by my system's spam detector.
Cute.

} From: "Sherwood, Margaret " {MSHERWOOD-at-PARTNERS.ORG}
To: "'Garry Burgess'" {GBurgess-at-exchange.hsc.mb.ca} ,
"'Microscopy-at-MSA.Microscopy.com'" {Microscopy-at-msa.microscopy.com}

You can arbitrary reference the phase. If the phase is referenced to an
undisturbed wave at the same plane (wave if there is no specimen) then I
would say yes - the imaginary part for weak phase specimens should be
always negative. Any material has positive inner potential. When the
electron wave traverses the area of the specimen it will experience a
negative phase shift due to the positive potential in that area (phase
retardation). If the magnitude of the phase shift is small (less than
Pi) then f2 in your expression will always be negative.

Regards,

Rado

} -----Original Message-----
} From: Michael O'Keefe [mailto:MAOKeefe-at-lbl.gov]
} Sent: Friday, May 28, 2004 7:32 AM
} To: Zhongyi Liu
} Cc: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] Re: imaginary part of exit wave
}
}
}
}
} --------------------------------------------------------------
} ----------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line
} Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} --------------------------------------------------------------
} -----------------
}
} False.
} At least in simulated exit-waves.
} For example, in simulations for GaN at 300keV, the exit-wave
} Argand-plane vector at the Ga position starts at f2 = 0 for
} zero thickness, then describes an approximate circle that
} extends from f2 = +1.3 to -1.5 electrons. Mike
}
} Zhongyi Liu wrote:
}
} }
} ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line
} Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} -----------------
} }
} } Dear Members,
} }
} } Question: In the TEM, the exit wave (the wave leaving
} } the specimen)is complex-valued in general, which can
} } be written as g = f1 + i*f2, where f1 and f2 are real
} numbers. Is it
} } true/false that f2 has no sign changes, i.e. if positive, always
} } positive?
} }
} } With best regards,
} }
} } Zhongyi Liu
} } Argonne National Lab
} } Argonne, IL60439
} }
} }
} }
} }
} }
} } ____________________________________________________________
} } Yahoo! Messenger - Communicate instantly..."Ping"
} } your friends today! Download Messenger Now
} } http://uk.messenger.yahoo.com/download/index.html
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 08:00:01 2004

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Dear Microscopists,

According to the research of Andrew Churg of the University of British Columbia's Department of Pathology, the average 60 year old North American's lung contains about 400,000 fibers of asbestos. 20% of those fibers are of the "carcinogenic" amphibole variety. The balance being harmless chrysotile asbestos. See "Health Effects of Mineral Dusts" Mineralogical Society of America Reviews in Mineralogy Volume 28.

"Asbestos" has become an antique term of convenience value only. It referred to fibrous silicate minerals in two groups. Those were the serpentine group (chrysotile) and the amphibole group (amesite, riebeckite ((crocidolite)) etc.).

The better term is "asbestosform" minerals. This term includes the most hazardous fibrous silicates which are in the zeolite group of minerals. Offretite and erionite are brittle, very finely fibrous minerals which are known to occur in large zeolitized lake-bed deposits, often near human inhabitation. Their aspect ratio and stiffness is ideally suited to create lesions in the lungs. Many human deaths in Turkey are associated with offretite and erionite. Similar deposits occur in the U.S., but are not near population centers.

Chyrsotile is a relatively benign material with remarkably useful physical properties that are NOT duplicated by any other material. Yet the regulators have taken it away from us. Brake linings made from chrysotile are far more fade resistant than those made from chrysotile's replacement. PIG HAIR !!! And beware, most other modern and synthetic substitutes have unknown health factors.

Nevertheless, it is only amphibole "asbestos" that has been shown to be carcinogenic by classic studies. Its major source was South Africa. Amphibole asbestos was far more expensive than chrysotile asbestos and was only used for high temperature applications such as ship boilers. Chysotile converts to brittle forsterite at 800 degrees C whereas amphibole asbestos stay fibrous above 1300 degrees C. This makes it more suitable for high temp boiler applications. At the end of WW II there were stockpiles of amphibole asbestos which were sold off at chrysotile prices. In this way some harmful amphibole asbestos found its way into residential applications. A "glitter" ceiling (mica with asbestos binder) installed pre-1950 may be dangerous, but not the later ones since the stockpiles of amphibole asbestos were generally spent.

Amphibole asbestos has been in the news recently due to media play on the former vermiculite mines in Libby, Montana. There the amphibole is richterite and occurs intergrown with the vermiculite in trace quantities. Mining operations placed the fibers in the air and asbestosis has resulted mostly among the mine workers, but some evidence shows asbestosis and mesothelioma among the families of mine workers. Tavern talk indicates that the mine workers often cut holes in their respirators to facilitate the insertion of cigarettes. Cigarette smoking is usually a key associated behavior in the contraction of fatal mesothelioma. One Libby mine worker / smoker has indignantly shown his chest x-ray to the media as proof of the mining company's irresponsible actions. He was 83 three years ago. We should all live so long.

I have much more should anyone be interested in contacting me offline.

Bart Cannon
Cannon Microprobe
Seattle

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 08:20:48 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mpendleton-at-mic.tamu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, May 27, 2004 at 11:25:06
---------------------------------------------------------------------------

Email: mpendleton-at-mic.tamu.edu
Name: Mike Pendleton

Organization: Texas A&M U. Micros. & Imaging Center

Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to 8bit tif

Question: With our image capture system used for the JEOL 6400 SEM we need a windows based system to convert 16 bit Sun Raster grayscale images into 8 bit grayscale tif images. I use the free XnView program to convert 8 bit grayscale Sun Raster images to 8 bit grayscale tif images so I can cut down on the tedious conversion process I am currently using, but still have to make the 16 to 8 bit conversion using the Sun program connected to the scope. I think the new version of Photoshop will convert 16 bit Sun Raster to 8 bit tif, but this is costly just to be able to convert files. Is there an inexpensive program to convert 16 bit Sun Raster images to 8 bit tif images? I would appreciate any information to solve this problem. Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 11:01:13 2004

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(5/28/04 8:33) by way of MicroscopyListserver {mpendleton-at-mic.tamu.edu} wrote:

} Email: mpendleton-at-mic.tamu.edu
} Name: Mike Pendleton
}
} Organization: Texas A&M U. Micros. & Imaging Center
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to 8bit tif
}
} Question: With our image capture system used for the JEOL 6400 SEM we need a windows based system to convert 16 bit Sun Raster
} grayscale images into 8 bit grayscale tif images. I use the free XnView program to convert 8 bit grayscale Sun Raster images to 8
} bit grayscale tif images so I can cut down on the tedious conversion process I am currently using, but still have to make the 16 to 8
} bit conversion using the Sun program connected to the scope. I think the new version of Photoshop will convert 16 bit Sun Raster to
} 8 bit tif, but this is costly just to be able to convert files. Is there an inexpensive program to convert 16 bit Sun Raster images to 8
} bit tif images? I would appreciate any information to solve this problem. Thanks.

Mike,

You are correct that Photoshop will do this. You might find, however, that Photoshop isn't as expensive as you think. It has been my experience that many universities these days have negotiated site licenses with Adobe, so that installing Photoshop on a university-owned machine is essentially free. You'd want to speak with your campus IT department to see if that is the case. Even if you don't have a site license, you will probably be able to get the educational version of Photoshop through your student bookstore, which is incredibly cheap.

This does beg the question of why you're wanting to throw away those 8-bits of data. I realize that SEM isn't going to give you much more than 8 bits of real data, but are you sure that the conversion isn't throwing away an equal amount of signal as noise? We usually recommend to folks that if they're getting 16 bits out, they should do their processing and measurement on that 16-bit image. This is especially important if you want to do any Fourier processing, for obvious reasons. When people ask me about the differences between Fovea Pro and the Image Processing Tool Kit, this usually comes up, since Fovea supports 16-bit images in Photoshop.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 11:01:29 2004

Contents Retrieved from Microscopy Listserver Archives
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You might try looking at Graphic Converter. There are two versions out
there.

One is for the PC at Version 2.5. Go to http://www.graphic-converter.net/.
It converts 30 file formats. It's hard to tell if it reads Sun Raster file
formats, the site is rather brief in its descriptions. The software is
available online for $19.95

One is for the Mac at Version 5.1.1. Go to
http://www.lemkesoft.de/en/index.htm. This software imports 175 file formats
and exports 75 formats. This version will import Sun Raster file format in 8
or 24 bit per pixel. The software is available online for $35 ($30 w/o CD).

} Email: mpendleton-at-mic.tamu.edu
} Name: Mike Pendleton
}
} Organization: Texas A&M U. Micros. & Imaging Center
}
} Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to
} 8bit tif
}
} Question: With our image capture system used for the JEOL 6400 SEM we need a
} windows based system to convert 16 bit Sun Raster grayscale images into 8 bit
} grayscale tif images. I use the free XnView program to convert 8 bit
} grayscale Sun Raster images to 8 bit grayscale tif images so I can cut down on
} the tedious conversion process I am currently using, but still have to make
} the 16 to 8 bit conversion using the Sun program connected to the scope. I
} think the new version of Photoshop will convert 16 bit Sun Raster to 8 bit
} tif, but this is costly just to be able to convert files. Is there an
} inexpensive program to convert 16 bit Sun Raster images to 8 bit tif images?
} I would appreciate any information to solve this problem. Thanks.
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 11:43:03 2004

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On May 25, 2004, at 11:08 AM, Tindall, Randy D. wrote:

} Does anyone else think it might be a useful exercise to try and
} establish expiration dates for chemicals used in microscopy labs? I
} understand that chemicals "expire" based upon what they are, what use
} they are intended for, how they are used, what level of
} accuracy/repeatability/etc. is expected from their use, how they are
} stored, and many other factors. I have also read Rande Kline's
} discussion of the problem in the July/August 2000 Microscopy Today on
} the difficulties of establishing such dates (recommended).
}
} The problem is that some work requires lab certification and strict
} laboratory guidelines requiring that all chemicals be labeled with
} expiration dates----whether or not those dates have any meaningful or
} consistent basis in "reality". So far, I've been unable to find any
} such set of standards and my strong impression is that labs set up
} their
} own arbitrary chemical rotation regimen.
}
Dear Randy,
Count me as one of the interested parties. Especially since there are
several chemicals that we use sporadically, we need to know what must
be made up fresh, and how long things keep.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 13:51:55 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I would also like to see something done with this. We have recently been
advise that we should not keep 'useless' chemicals around the lab. Its a
long story, the rest of this message summarizes some our experiences.

We are being treated to a series of regulatory inspections. First, it was
by an agency concerned about 'hazardous waste'. Now it is by agencies
looking at the way we ship and receive goods to and from campus.

The hazardous waste guys might have been the EPA, but I'm not sure. We (the
campus) were given the opportunity to do a 'self audit'. In a self audit,
our EH&S guys got to go around and get everyone up to speed on proper
disposal and storage methods for hazardous waste. Mostly, it was the normal
stuff, but a new wrinkle for me was that I may no longer keep anything
marked as 'waste' in the lab for more than 6 months. Has something to do
with accumulation rules and shipping it off campus.

The deal with the 'self audit' is that you get one 'get out of jail free'
card, sort of. If you do a good job and come clean with any violations,
then those violations will not be held against you if they ever do an
official audit. Official audits can be big time trouble, expensive and a
pain. For example, fines, big ones, may be assessed and you may be told to
fix something right now, whether there is money to do it or not. We just
barely beat a bad situation by having the proper hoods and venting for the
storage of some special compound. Had we not had it right, the EH&S guys
said the inspector could have demanded that we install an expensive system
within something like 90 days, or abandon the use of that compound.

As a sideline to the audit thing, our EH&S folks are encouraging us to get
rid of anything we don't need or use regularly. They say,'It will never get
cheaper to dispose of hazardous waste than it is today'. The cost of
disposal will only go up, so if you aren't going to use it, get rid of it.
I wonder about this because I tend to keep some old stuff around in case a
starving student needs something like embedding resin. I have a bunch left
over from various kits, but can I trust it? If not, it should go, but its
hard to toss things that may be useful.

We are currently involved in another 'self audit'. This one being done to
check on what and how we ship things to and from campus. Dept. of Commerce
and Homeland Security have lists of things that are not allowed, like wet
suits to North Korea, etc. The list is pages, maybe hundreds, long with
some of the weirdest things. Lots of things like chemicals and biological
samples show up. Same deal, admit to any wrong doing and say how you will
correct it will keep you off the hook. Forget something or make a mistake
after the audit and you could go to jail.

So, in the interest of staying out of jail, not paying fines, and keeping
our EH&S staff happy, I would like to get some ideas about how long to keep
things around before moving them out. I will just have to deal with the
guilt of tossing perfectly good materials on my own.

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 14:11:44 2004

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On May 26, 2004, at 2:30 AM, Philip Koeck wrote:

} I have some test images (defocus around 1000 nm) from a FEG-TEM where
} Young fringes seem to extend up to twice as far as Thon rings. Is that
} usual and if so which of the two defines the information limit?
} What do manufacturers mean by information limit?
} Do Young fringes really show up to which resolution I can get useful
} information from a micrograph?
} At least in TEM of non-periodic biological specimens you normally don't
} expect anything beyond the last clearly visible Thon ring.
}
Dear Philip,
Do you generate the Young's fringes by shifting the image in the scope
during the exposure, or do you use a computer to generate a shifted
image and sum it with the unshifted image? In the latter case, the
noise, which does not have a CTF related to the lenses, is perfectly
correlated, so there will be fringes, but no rings. In the former
case, the noise is independent for the shifted and unshifted parts of
the image, so it will not add as much intensity to the fringes (there
will be some correlation of random noise, so some intensity). The
information limit is measured by the Thon rings. Whether the
information from Thon rings beyond the first zero of the CTF is useful
depends on the nature of the specimen, the accuracy with which the
exact value of the defocus can be measured, and the processing
algorithm used to compensate for the CTF. For thick, non-periodic
biological specimens, the defocus varies through the specimen, the
contrast is low, and the dose is low, so the S/N is low. It is still a
matter of discussion whether such techniques as CTF compensation or
focal series reconstruction are of benefit.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 14:33:22 2004

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At the moment, Photoshop 7 can be obtained on the net for $60.
Photoshop 7 is a perfectly respectable version and is available
inexpensively because Photoshop 8 (or CS) is out. You however will love
Photoshop 7 as well.
Just a thought,
Judy Murphy

Doug Baldwin wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} You might try looking at Graphic Converter. There are two versions out
} there.
}
} One is for the PC at Version 2.5. Go to http://www.graphic-converter.net/.
} It converts 30 file formats. It's hard to tell if it reads Sun Raster file
} formats, the site is rather brief in its descriptions. The software is
} available online for $19.95
}
} One is for the Mac at Version 5.1.1. Go to
} http://www.lemkesoft.de/en/index.htm. This software imports 175 file formats
} and exports 75 formats. This version will import Sun Raster file format in 8
} or 24 bit per pixel. The software is available online for $35 ($30 w/o CD).
}
} } Email: mpendleton-at-mic.tamu.edu
} } Name: Mike Pendleton
} }
} } Organization: Texas A&M U. Micros. & Imaging Center
} }
} } Title-Subject: [Microscopy] [Filtered] MListserver:Conversion 16bit raster to
} } 8bit tif
} }
} } Question: With our image capture system used for the JEOL 6400 SEM we need a
} } windows based system to convert 16 bit Sun Raster grayscale images into 8 bit
} } grayscale tif images. I use the free XnView program to convert 8 bit
} } grayscale Sun Raster images to 8 bit grayscale tif images so I can cut down on
} } the tedious conversion process I am currently using, but still have to make
} } the 16 to 8 bit conversion using the Sun program connected to the scope. I
} } think the new version of Photoshop will convert 16 bit Sun Raster to 8 bit
} } tif, but this is costly just to be able to convert files. Is there an
} } inexpensive program to convert 16 bit Sun Raster images to 8 bit tif images?
} } I would appreciate any information to solve this problem. Thanks.
} }
} } ---------------------------------------------------------------------------
} }

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 14:48:06 2004

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Randy,

I agree that this is an important issue and that some standard re: expiration
of chemicals would be great. But is it reasonable?

I don't think it is--manufacturers of chemicals and reagents are a good source:
they test these chemicals and assign a shelf-life. But, ultimately it depends
on how the user handles the chemical. For example, our lab uses
photosensitizers, which need to be kept at -20 in the dark. If you aliquot the
photosensitizer and keep them at -20, only using what you need, then it will
(probably) be OK. But, if you don't, and open the vial (even in the dark),
every day to take an aliquot, then each time it is opened, it loses it's
efficacy.

We also know that most chemicals are still OK even if the expiration date listed
on the bottle has passed. I believe most of us have to use our own judgment:
if the procedure is critical (i.e. immunohistochemistry-antibodies), aliquot
them, store according to MSDS and use a fresh aliquot, if the procedure is not
(routine buffers using basic compounds), continue to use the chemical: it is
pretty stable. This method is not good, or scientific, but it's probably the
best we can do.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Tindall, Randy D. [mailto:TindallR-at-missouri.edu]
Sent: Thursday, May 27, 2004 9:35 AM
To: microscopy-at-sparc5.microscopy.com

Hi again,

I think I need to restate my question about expiration dates on lab
chemicals, since I may have been unclear in my first posting.

I know that expiration dates are arbitrary and maybe even meaningless in
many cases, because they depend on so many variables. However,
sometimes we are required to put them on our reagents because of rules
regarding certain research projects.

For example, if a lab should perform electron microscopy as part of a
project involving a pharmaceutical company, chances are that the company
will require certain types of documentation, traceability, instrument
calibration, standardization of methods, etc. Expiration dates on
chemicals are often (maybe always) part of such requirements.
Diagnostic work is another probable example.

My question or proposal is this: Given that we are sometimes REQUIRED to
use expiration dates, wouldn't it be reasonable if there was some
consensus in our field we could point to and say "Our lab follows the
(for example) MSA standards on chemical usage."? As it is, I have not
yet been able to locate a set of standards to guide us in any sort of
meaningful compliance with such outside requirements. Phil Oshel has
suggested that the histotech community has been dealing with this for
some time, so I'm checking this out now (thanks for the suggestion,
Phil).

On the other hand, maybe this is something that doesn't need fixing,
because it ain't broke. I'm just curious what others think about it.

Thanks all.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 15:15:13 2004

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My first EM job was at a hospital. Coindentially, I
started work in the midst of a CAP inspection. I
checked and doubled checked all the reagents for
proper labeling. Reagents that were formulated in the
lab were given a 6-month expiration date from the prep
date. Most of the time, reagents 'keep' beyond the
expiration date. When making reagents, I try to make
a minimum volume that would generally last for 6
months. It helps to make minimum volumes to reduce
waste, too. And, unless your lab is especially
problem free when it comes to solution viability, it
helps to keep reagents for a set time in order to
maximize specimen quality during processing, staining,
etc. Hope that helps.
Sara Goldston

Bill Tivol {tivol-at-caltech.edu} wrote:

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy
Society of America

On May 25, 2004, at 11:08 AM, Tindall, Randy D. wrote:

} Does anyone else think it might be a useful exercise
to try and
} establish expiration dates for chemicals used in
microscopy labs? I
} understand that chemicals "expire" based upon what
they are, what use
} they are intended for, how they are used, what level
of
} accuracy/repeatability/etc. is expected from their
use, how they are
} stored, and many other factors. I have also read
Rande Kline's
} discussion of the problem in the July/August 2000
Microscopy Today on
} the difficulties of establishing such dates
(recommended).
}
} The problem is that some work requires lab
certification and strict
} laboratory guidelines requiring that all chemicals
be labeled with
} expiration dates----whether or not those dates have
any meaningful or
} consistent basis in "reality". So far, I've been
unable to find any
} such set of standards and my strong impression is
that labs set up
} their
} own arbitrary chemical rotation regimen.
}
Dear Randy,
Count me as one of the interested parties. Especially
since there are
several chemicals that we use sporadically, we need to
know what must
be made up fresh, and how long things keep.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

__________________________________
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From MicroscopyL-request-at-ns.microscopy.com Fri May 28 16:17:45 2004

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Dear Members,

Anyone knowing how to calculate models for amorphous
structure mentioned in Wharton's email? Thanks.
Zhongyi, ANL.

--- "Sinkler, Wharton" {Wharton.Sinkler-at-uop.com}
wrote: }
} Zhongyi,
}
} For an amorphous structure much of the same argument
} applies: If you drop
} the assumption about the atomic columns then you'll
} generally have some
} non-atom-like bound state functions, which oscillate
} in precisely the same
} way. However the eigenvalues (which determine the
} frequency of the
} oscillations) will be considerably smaller. Thus
} the oscillatory behavior
} won't show up until significantly larger thickness.
} Unfortunately I don't
} offhand know of any calculations for models of
} amorphous structures which
} specify the period of the oscillation for the
} deepest channeling state (a
} topic for a paper?, or maybe someone else on the
} list will be able to help).
}
}
} Wharton
}
}
} -----Original Message-----
} From: Zhongyi Liu [mailto:liu_zhongyi-at-yahoo.com]
} Sent: Thursday, May 27, 2004 2:23 PM
} To: Sinkler, Wharton
} Subject: [Microscopy] RE: imaginary part of exit
} wave
}
}
} Dear Wharton,
}
} Thank you very much for the answer. I will consult
} with your paper for details. A quick question again:
} if the specimen is an amorphous object (without
} well-defined atomic columns like crystals),and it
} cannot be approximated as weak phase object
} (metallic
} material and tens of nanometers in thickness), any
} idea how f2 will behave in this case, anything
} different from a general case?
}
} Thanks again.
}
} Zhongyi
}
} --- "Sinkler, Wharton" {Wharton.Sinkler-at-uop.com}
} wrote: }
} } Zhongyi,
} }
} } It is not generally true that the imaginary part
} of
} } the wave is always
} } positive (as it is by convention for a weak phase
} } object).
} }
} } A nice way to consider this is electron channeling
} } theory, a kind of
} } simplified dynamical theory which is approximately
} } correct for high
} } energies, and is most useful in the case that the
} } electron beam is aligned
} } with well-defined atomic columns. In this theory
} } the exit wave at an atomic
} } column looks like the column's projected
} potential,
} } but is modulated by a
} } function (exp(ik'z)-1). Here z goes through the
} } sample thickness and k' is
} } a constant which depends on what atoms occupy the
} } column.
} }
} } (Actually this is for the scattered part of the
} } wave, or y(r)-1, where the 1
} } represents the incident beam intensity)
} }
} } As you can see, when the argument of the
} exponential
} } is small everything is
} } zero (nothing is scattered yet). As z gets bigger
} } the imaginary part gets
} } positive at first (like the weak phase object
} } approximation), but then
} } swings around and becomes negative. For a typical
} } inorganic sample
} } containing say a column of first-row transition
} } metals, the function will
} } oscillate several times in a typical
} high-resolution
} } sample thickness of one
} } or two hundred angstroms, so this is not some
} } esoteric case but really
} } occurs in standard TEM conditions.
} }
} } This is a simplified model, but the agreement with
} } full dynamical
} } calculations is quite good. If you'd like to see
} a comparison (as
} } well as convince yourself that f2 does indeed go
} negative)
} } you can read more for
} } example in a paper by myself and Laurie Marks, J.
} } Microscopy vol. 194
} } (1999). Or if you have access to a multislice
} wave
} } simulation you can try
} } it for yourself.
} }
} } Best Regards,
} }
} } Wharton
} }
} }
}
****************************************************************
} } Wharton Sinkler, PhD.
} } UOP LLC
} } 25 E. Algonquin Rd.
} } Des Plaines, IL 60017-5017
} } tel. 847-391-3878
} } fax. 847-391-3719
} } mailto Wharton.Sinkler-at-uop.com
} }
} }
} }
} } -----Original Message-----
} } From: Zhongyi Liu [mailto:liu_zhongyi-at-yahoo.com]
} } Sent: Thursday, May 27, 2004 10:18 AM
} } To: Microscopy-at-MSA.Microscopy.Com
} } Subject: [Microscopy] imaginary part of exit wave
} }
} }
} }
} }
} }
}
----------------------------------------------------------------------------
} } --
} } The Microscopy ListServer -- Sponsor: The
} } Microscopy Society of America To
} } Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} }
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
}
----------------------------------------------------------------------------
} } ---
} }
} } Dear Members,
} }
} } Question: In the TEM, the exit wave (the wave
} } leaving
} } the specimen)is complex-valued in general, which
} can
} } be written as g = f1 + i*f2, where f1 and f2 are
} } real
} } numbers. Is it true/false that f2 has no sign
} } changes,
} } i.e. if positive, always positive?
} }
} }
} } With best regards,
} }
} } Zhongyi Liu
} } Argonne National Lab
} } Argonne, IL60439
} }
} }
} }
} }
} }
} }
} }
}
____________________________________________________________
} } Yahoo! Messenger - Communicate instantly..."Ping"
} } your friends today! Download Messenger Now
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From MicroscopyL-request-at-ns.microscopy.com Fri May 28 17:11:11 2004

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our EHS office has equally tough rules on how long we can keep "used
materials" which is what the rest of the world calls waste. we can't have
any "waste" since we are qualified to assess it. i got dinged for having a
metal can for "waste razor blades". but, on the other hand, my EHS office
did one great thing and I encourage you all to get you own schools to do
it. They have a building with chemicals that are no longer needed by an
individual lab. rather than my storing some "potassium permanganate" or
"lead nitrate" that I would never use again, they take it and keep it for
any faculty member who wants it. I go over a couple of times a year and
get a "free" bottle of some chemical that i am sure is not outdated. this
includes osmium in sealed ampules, lead nitrate, etc. They keep a running
total of how much they "save" consumers so they look good to the
administration but they are also saving disposal costs, minimizing unused
hazardous chemicals kept in labs that don't need them, and helping to save
the environment. check out the website at
http://www.missouri.edu/~muehs/recycling.htm and then tell your EHS people
to start their own Chemical Recycling program.

At 11:57 AM 05/28/04 -0700, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri May 28 20:23:55 2004

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This has been an interesting thread. I'd like to offer a couple of
observations:

My basic premise is that each laboratory needs to have at least minimal
documentation that lists reagents that are critical to the analysis where
expiration dates have been documented to be important and what those dates
are. Additionally, the laboratory quality system needs to have a minimal
complaint/anomaly recording-tracking system where either an investigator or
a client can question a result. When a result is questioned, the samples,
reagents, procedures, and instruments are scrutinized for bias. This process
can lead to refinement of the list of critical reagents. Every quality
system our company has used over the years has required something like this.
The "minimalist system" we now use requires just this. Auditors have always
been "data driven" and been satisfied when I had records that showed I did
what I said I did... By the way, an enthusiastic attitude helps here. A
belligerent attitude is a big mistake.

Like others have noted before, over the years we have noticed some reagents
are more sensitive than others. Our most frequent problem these days is
water contamination of solvents for casting uniform support films for TEM.

On the other hand, we have some reasonably old reagents that still work
well. We have some epoxy embedding resins that are approaching ten years
old. We found that by doubling the hardener from the levels we used "new"
that we still get good results. Just this week I floated several holey
cellulose acetate butyrate films that I had prepared on the slide in August,
1990. (When we make them, we make a lot of them...) The resulting holey
carbon films were just as sturdy as the films I floated back in 1990. I also
have an ethanol dispersion of graphitic carbon originally prepared back in
1982 from a small amount of graphitic carbon that I obtained from a vendor
application specialist who used to work for a carbon company. Any time I
need a test specimen, I sonicate the dispersion and spot some on a new holey
carbon support film. Each of these has been stored properly and is stable.

The key in all this is understanding the materials one uses, being alert to
variability, and keeping appropriate records of observed anomalies. This is
simply good laboratory practice that should have been stressed in our first
lab classes. Now we realize why our high school chemistry teachers collected
our lab notebooks and graded them (big grin.)

John Minter
jrminter-at-rochester.rr.com

From MicroscopyL-request-at-ns.microscopy.com Sat May 29 02:19:19 2004

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Last days for Fluorescence School in Genoa
Visit www.lambs.it and link to Fluorescence School on the opening page.
All my best
Alberto

------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat May 29 09:13:27 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (alvarobq-at-fcien.edu.uy) from http://www.msa.microscopy.org/Ask-A-Microscopist.html on Friday, May 28, 2004 at 09:41:06
---------------------------------------------------------------------------

Email: alvarobq-at-fcien.edu.uy
Name: Alvaro D. Olivera

Organization: Science Faculty

Education: Graduate College

Location: Montevideo, Uruguay

Question: I achieved a flat embedding (in Durcupan, Fluka)for TEM (over a glass slide)with immuno peroxidase - DAb(ABC Kit, Vector)tested tissue pieces of 50 microns and obtained very good results under light microscopy. After dissected the interest area, sticked it on a Araldite block. I cut 60 nm sections and mounted over 200 mesh Cu grids covered with Coat-Pen, and stained whith Uranyl acetate 5% in Ethanol(15 minutes)and after that with ReynoldĄs Lead citrate(7 minutes). When we observed under TEM (80 KV) it was good stained but we canĄt be sure to recognize the reaction correctly.I suppose what the electron density of the reaction itĄs not enough.
So what can I do? Do you use any enhancement kit?
Many thanks for your response. Alvaro.

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From MicroscopyL-request-at-ns.microscopy.com Sun May 30 12:25:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ottagonosole-at-tiscali.it) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, May 29, 2004 at 15:15:22
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Email: ottagonosole-at-tiscali.it
Name: giovanni de caro

Organization: museo laboratorio di scienze naturali "S. Eugenio de Mazenod" - Ripalimosani - Italia

Title-Subject: [Microscopy] [Filtered] MListserver: AMR 1000 A SEM parts wanted

Question: "THE "S. EUGENIO DE MAZENOD" NATURAL SCIENCE MUSEUM AND LABORATORY IS A NO PROFIT SELF FUNDED PROJECT BASED IN SOUTHERN ITALY CREATED WITH THE AIM TO FOSTER SCIENTIFIC EDUCATION OF YOUNGSTERS (SEE OUR WEBSITE: http://web.tiscali.it/bimbononno). WE HAVE BEEN DONATED AN OLD AMR-LEITZ 1000 A SCANNING ELECTRON MICROSCOPE WHICH WE WISH TO RESTORE AND USE FOR OUR TEACHING ACTIVITIES. THE INSTRUMENT IS NOT WORKING; WE NEED SOME SPARE PARTS TO RESTART IT. IF ANYONE CAN HELP US PLEASE CONTACT US AT : ottagonosole-at-tiscali.it.
THANK YOU".

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We would like to purchase a filter slider for epi-illuminator on Nikon Diaphot .

From MicroscopyL-request-at-ns.microscopy.com Mon May 31 08:43:12 2004

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Alvaro,
You should try either staining with uranyl acetate (aqueous) alone
or look at unstained samples, sometimes the full staining
(UA + PB) may hide the DAB product (by bringing up the rest
of the sample). Also try cutting thicker samples (0.15-.2
um) to have more reaction product. good luck.

Michael Delannoy

----- Original Message -----
} From: alvarobq-at-fcien.edu.uy (by way of MicroscopyListserver)

Hello Everybody...

We are planning to buy a TEM. We want to learn whether LEO 906 is still produced by Zeiss. Because we couldn't find any information about LEO 906 in their official web page. However the dealer of Zeiss in Turkey told us it is still being produced by Zeiss. We couldn't trust him since he told us LEO 906 is not produced any more in our previous conversation with him.
If anybody help us about this problem we would be very happy.
Thanks in advance...

Dr. Necat Yžlmaz

From MicroscopyL-request-at-ns.microscopy.com Mon May 31 12:06:26 2004

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Dear colleagues,
Do you have any experience of setting the sensitivity of EM 4489 films in
TEM? I found the default value (11) in JEOL 2010F did not work very well.
Your suggestions will be much appreciated.

best regards,
zejian liu
University of North Carolina at Chapel Hill
Chapel Hill, NC 27599

________________________________________________________________

This message was sent using UNC Physics' Webmail
http://webmail.physics.unc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon May 31 13:12:54 2004

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There isn't much in DAB alone that is electron dense. You might
have more luck using the Nickel intensifying system with the DAB.

Date sent: Mon, 31 May 2004 09:57:48 -0400
} From: MICHAEL J DELANNOY {delannoy-at-jhmi.edu}

}
} We are planning to buy a TEM. We want to learn whether LEO 906 is
} still produced by Zeiss. Because we couldn't find any information
} about LEO 906 in their official web page. However the dealer of Zeiss
} in Turkey told us it is still being produced by Zeiss. We couldn't
} trust him since he told us LEO 906 is not produced any more in our
} previous conversation with him. If anybody help us about this problem
} we would be very happy. Thanks in advance...
}

Boy, just wait till the manager of Zeiss reads this!

And some of us occasionally grumble about our local agents!

Let me hasten to add that I am very satisfied with my local microscopy
reps.

good luck

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599
ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon May 31 16:40:17 2004

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You need to make an "exposure series": set exposure time manually to let
say 1.5 sec (my favorite); obtain illumination on the screen (with image or
without) you usually use (spread beam weel enough); take first picture at
sensitivity let say 8, next - 9, 10, 11, 12 and so on. Then develop film
at your normal condition and choose the image with optimal (to you)
density. More "scientific" way to do so is to measure the optical density
of the developed (fixed washed and dried) film in spectrophotometer. I
don't remember exactly, but 0.5-07 OU (optical units, visual area of the
spectrum) should be OK, I guess (hey, EM community, correct me if I am
wrong). You also have to be aware of recent (relatively) modification
Kodak introduces in 4489 formulation (see huge communication on this
subject in Archive). I hope it helps. Sergey

At 01:21 PM 5/31/2004 -0400, you wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Mon May 31 18:09:31 2004

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Colleagues

The May Archives are now on-line at:

http://www.microscopy.com/MicroscopyListserver

Cheers....

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 03:19:06 2004

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As you mentionned, sensitivity 11 is close to normal value but can vary
due to your developping time and developping temperature.
If 11 is too much developped (too dark) then you can try higher number
(usually until 14) to tell microscope that film is more sensitive , in
another way use lower number for film not enough developped (too blank)

Michel RIBARDIERE
TEM MANAGER
JEOL (EUROPE)S.A.

-----Message d'origine-----
De : zejianl-at-physics.unc.edu [mailto:zejianl-at-physics.unc.edu]
Envoyé : lundi 31 mai 2004 19:22
Ŕ : Microscopy-at-MSA.Microscopy.Com
Objet : Kodak EM4489 films sensitivity

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------
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Dear colleagues,
Do you have any experience of setting the sensitivity of EM 4489 films
in
TEM? I found the default value (11) in JEOL 2010F did not work very
well.
Your suggestions will be much appreciated.

best regards,
zejian liu
University of North Carolina at Chapel Hill
Chapel Hill, NC 27599

________________________________________________________________

This message was sent using UNC Physics' Webmail
http://webmail.physics.unc.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 08:36:27 2004

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A little different slant on this thread:

Has anybody noticed a second round of changes in this film?

A while back there was a discussion about the "New Formulation" of this
film and all the problems it caused with thin, patchy negatives. We
finally got our new agitation procedures and exposures worked out and
were getting good results again. Then, some months ago our negatives
began coming out consistently too dark, so we began diluting our D-19
developer by an additional 25%, which gave us good results again.

Just last week we ran tests on MACO TEM film as a possible cheaper
replacement for 4489. We processed a batch taken with three different
exposure settings on our JEOL 1200EX and two agitation procedures. One
procedure was our new current one of two seconds of nitrogen burst every
10 seconds, with one manual agitation every 30 seconds (lift and tilt
five seconds each side), and the other was our old method of 10 seconds
nitrogen burst every minute, with no manual agitation. To my surprise,
the 4489 film came out beautifully using the old agitation method----no
streaks or patchiness.

This leads me to think that there's a possibility that this film was
reformulated yet again at some point, since nothing obvious changed in
our procedures. Any similar experiences out there?

Thanks,
Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 09:51:05 2004

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First off, make sure your developer is fresh, properly diluted and at
the correct temperature (68F/20C or a bit higher). I am always amazed at
how some people will try to stretch old developer. Chemistry is the
cheapest part of electron microscopy. Then do an exposure series as
others have suggested.

Geoff

zejianl-at-physics.unc.edu wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 12:50:15 2004

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We use Kodak 4489 film, and have for ages in a Philips CM10. Lately,
I've noticed when I take the film out of the film box from the microscope,
some of the film is not flat, but has popped up just a little on the edge
of the film cassette that is open where you slide the film in. They
aren't all popped up, just some. And others, if I take them out, can
watch them pop up as they sit on the counter in the cassette. Possibly
it's just from moisture in the air? I'm hoping they are flat in the
scope and only pop up when removed from the scope, but I don't know. And
have never noticed this before. Has anyone else encountered this? The
images all look fine after development, I don't notice any out of focus
spots on one side, but we haven't been doing any real high mag work lately.

Nancy Piatczyc

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 13:52:22 2004

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On May 31, 2004, at 2:56 PM, Sergey Ryazantsev wrote:

} I don't remember exactly, but 0.5-07 OU (optical units, visual area of
} the spectrum) should be OK, I guess (hey, EM community, correct me if
} I am wrong).

Dear Sergey,
We always calculated our exposure for 4489 so that we got an OD of
1.0. 4489 has a linear range to about OD 2--better than SO163--so the
larger OD is still well within the linear response range and provides a
really good image for prints and enlargements.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 14:32:55 2004

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You can enhance/intensify the DAB reaction product with osmium, or
nickel or nickel+cobalt before you embedd the tissue in Durcupan (or
whatever). After embedding ......... I don't know. Cutting thicker
sections might help a bit, also, staining with only UA (as someone else
suggested) might allow the DAB to show up better. You could etch the
sections with 10% hydrogen peroxide for a few minutes then try 1-2%
osmium, that might give you enough contrast. Good luck.

Geoff

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 1 16:05:57 2004

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Quoting Nancy.P.Piatczyc-at-williams.edu:
} We use Kodak 4489 film, and have for ages in a Philips CM10.
} Lately, I've noticed when I take the film out of the film box
} from the microscope, some of the film is not flat,
} but has popped up just a little on the edge
} of the film cassette that is open where you slide the film in.
} They aren't all popped up, just some.
} And others, if I take them out, can watch them pop up
} as they sit on the counter in the cassette.
} Possibly it's just from moisture in the air?
} I'm hoping they are flat in the scope and only pop up
} when removed from the scope, but I don't know. And
} have never noticed this before. Has anyone else encountered this?
} The images all look fine after development,
} I don't notice any out of focus spots on one side,
} but we haven't been doing any real high mag work lately.
}
} Nancy Piatczyc
==================
Nancy,
I have just loaded three cassettes of 4489 film and it does
seem to curl more than I had remembered but not to the point
where it was difficult to load.

Is there much play in the slots that the film slides into?
If there is, you might consider applying a LITTLE pressure
with a vise, just to reduce the gap a bit. My holders are
a different type and periodically I need to open up the slots
a bit when the film no longer slides into the holder.

Pat Connelly
Dept of Biology
Univ. of Pennsylvania
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 2 07:58:53 2004

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Fellow List Members,

On behalf of the Executive Council of the Midwest Microscopy and
Microanalysis Society, I would like to thank those of you who responded
to my request for student poster session guidelines. The information
that you provided will be very helpful to us, and we appreciate
receiving so much useful feedback in such a short time.

Regards,

Elaine

Elaine Schumacher
Senior Research Scientist
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539 USA
630-887-7100 (tel)
630-887-7417 (fax)
E-mail: eschumacher-at-mccrone.com
Web Site: www.mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 2 11:07:32 2004

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Seems like everyone makes a digital camera for light microscope applications. I would appreciate hearing any recommendations or experiences with any of the high resolution cameras available. This is for a metallurgical microscope with a c-mount and would need at least 1300x1000 resolution in color and a fast, TV like refresh rate for previewing. Any ideas?

Robert W. Skwarok
Syncrude Research Center
9421-17 Ave.
Edmonton, Alberta
Canada, T6N-1H4
ph: 780-970-6931
fax: 780-970-6805
skwarok.robert-at-syncrude.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 00:28:21 2004

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Hi

We use a Nikon DXM 1200F - excellent camera, 12 megapixel - so max pixel
resolution is 3840 X 3072 and minimum 640 X 480 (10 different sizes to
choose from). Image formats JPEG, BMP and TIFF. Very user friendly and
everything is software driven through the PC.

I have no connection with the company - I am just a satisfied user!

Med vänliga hälsningar/With best regards

Gareth

***Come to Stockholm in 2004 to the 26th IFBLS congress*** Take a look at
http://www.vardforbundet.se/ifbls2004

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 04:06:36 2004

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Hi,

Dear Bill and list-members,

The images were taken by people at Jeol in Japan. As far as I understand
they introduced an image shift during exposure.
(If you just shift the same image in the computer you get fringes all
the way to the edge of the micrograph, which is not the case with the
test images.)

} From the Young fringes Jeol claims an information limit better than 2
Angstroms, but I haven't seen Thon rings beyond about 4 Angstroms in any
of the images. (I think you might have misunderstood this point: Young
fringes extend up to twice as far as the outermost Thon ring, not only
beyond the first zero.)

} From this discussion I got the impression that manufacturers use Young
fringes because they extend further than Thon rings and somehow show the
true information limit (which brings me back to my original question
about the meaningfulness of the Youngfringe criterion).

} From Michael O'Keefes E-mails (offline) I understand that he
distinguishes between information limit and convergence limit. Maybe
that's what we are seeing here. (All these images were taken at
magnifications around 50K and defocus between 1000 and 2000 nm.)

The main question for me is how to compare microscopes for the sort of
microscopy we intend to do. Does the information limit really tell us
what sort of resolution our reconstructions will have or is that
determined by the extent of Thon rings.

I can send some images offline or put them on my homepage, if anybody
wants to see them.

Philip

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: 28 May 2004 21:29
On May 26, 2004, at 2:30 AM, Philip Koeck wrote:
} I have some test images (defocus around 1000 nm) from a FEG-TEM where
} Young fringes seem to extend up to twice as far as Thon rings. Is that
} usual and if so which of the two defines the information limit?
} What do manufacturers mean by information limit?
} Do Young fringes really show up to which resolution I can get useful
} information from a micrograph?
} At least in TEM of non-periodic biological specimens you normally
don't
} expect anything beyond the last clearly visible Thon ring.
}
Dear Philip,
Do you generate the Young's fringes by shifting the image in the
scope
during the exposure, or do you use a computer to generate a shifted
image and sum it with the unshifted image? In the latter case, the
noise, which does not have a CTF related to the lenses, is perfectly
correlated, so there will be fringes, but no rings. In the former
case, the noise is independent for the shifted and unshifted parts of
the image, so it will not add as much intensity to the fringes (there
will be some correlation of random noise, so some intensity). The
information limit is measured by the Thon rings. Whether the
information from Thon rings beyond the first zero of the CTF is useful
depends on the nature of the specimen, the accuracy with which the
exact value of the defocus can be measured, and the processing
algorithm used to compensate for the CTF. For thick, non-periodic
biological specimens, the defocus varies through the specimen, the
contrast is low, and the dose is low, so the S/N is low. It is still a
matter of discussion whether such techniques as CTF compensation or
focal series reconstruction are of benefit.
Yours,
Bill Tivol, PhD

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 08:00:31 2004

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I thought I posted this a week ago, but I never saw it come up. Curious. Here goes again (TIA):

Hello Listers,

I have a colleague who has been trying to use TEM to look at isolated chloroplasts from a marine alga (Bryopsis). She has also tried looking at intact algae. The problem is that following a standard protocol (Gta fix using isolation media, Os, UA en bloc, dehyd in ethanols and PO, 'epon' embedment; and Pb and UA on-grid), the membranes along the perimeter of both the isolates as well as the supposedly intact algae appear fragmented, or missing. Mostly missing. The cytoplasmic matrix and internal membrane-bound structures such as thykaloids appear essentially normal in terms of electron density and membrane integrity, so on first inspection it would appear the membranes are disappearing following initial fixation, or, they are stubbornly invisible.

We thought the missing isolated chloroplast membrane was attributable to the isolation procedure, until the intact algae also came up with no plasma membrane.

Any comments on ways to keep the PM intact? Or is this a usual appearance for these tissues? As others have noted, the chloroplasts do remain mostly green following Os.

There was a recent thread regarding missing membranes. We plan to test the acetone dehydration idea, and we already incorporate some of the suggestions in our standard protocol such as en bloc UA, so before we embark on a voyage of discovery using additives, I thought I would toss this problem out to any marine algae experts out there. Or anyone else who has another thought to share.

Thanks, all!

Ann Lehman

++++++++++++++++++++++++++++++++++++++
Ann Hein Lehman
Assistant Director, Electron Microscopy Facility
Mailstop: LSC-314
Trinity College
300 Summit Street
Hartford, CT 06106
v. 860-297-4289
e. ann.lehman-at-trincoll.edu
f. 860-297-2538
www.trincoll.edu/~alehman

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 12:08:18 2004

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-----Original Message-----
} From: James Chalcroft
Sent: Thursday, June 03, 2004 7:21 PM
To: 'Lehman, Ann R'

I thought I posted this a week ago, but I never saw it come up. Curious. Here goes again (TIA):

Hello Listers,

I have a colleague who has been trying to use TEM to look at isolated chloroplasts from a marine alga (Bryopsis). She has also tried looking at intact algae. The problem is that following a standard protocol (Gta fix using isolation media, Os, UA en bloc, dehyd in ethanols and PO, 'epon' embedment; and Pb and UA on-grid), the membranes along the perimeter of both the isolates as well as the supposedly intact algae appear fragmented, or missing. Mostly missing. The cytoplasmic matrix and internal membrane-bound structures such as thykaloids appear essentially normal in terms of electron density and membrane integrity, so on first inspection it would appear the membranes are disappearing following initial fixation, or, they are stubbornly invisible.

We thought the missing isolated chloroplast membrane was attributable to the isolation procedure, until the intact algae also came up with no plasma membrane.

Any comments on ways to keep the PM intact? Or is this a usual appearance for these tissues? As others have noted, the chloroplasts do remain mostly green following Os.

There was a recent thread regarding missing membranes. We plan to test the acetone dehydration idea, and we already incorporate some of the suggestions in our standard protocol such as en bloc UA, so before we embark on a voyage of discovery using additives, I thought I would toss this problem out to any marine algae experts out there. Or anyone else who has another thought to share.

Thanks, all!

Ann Lehman

++++++++++++++++++++++++++++++++++++++
Ann Hein Lehman
Assistant Director, Electron Microscopy Facility
Mailstop: LSC-314
Trinity College
300 Summit Street
Hartford, CT 06106
v. 860-297-4289
e. ann.lehman-at-trincoll.edu
f. 860-297-2538
www.trincoll.edu/~alehman

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 13:22:43 2004

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I was just reading a superb paper by Mobius et al (2002 J. Histochem.
Cytochem. 50(1):43-55) in which they use PHEM buffer for their fixatives
and immunostaining. PHEM is 60 mM PIPES, 25 mM HEPES, 2 mM MgCl2, 10 mM
EGTA, pH 6.9. Can anyone comment on the rationale behind the design of
this buffer? Specifically, why EGTA? In addition, why a PIPES/HEPES
mixture rather than just PIPES or HEPES? Thanks, Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 13:22:28 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (tauria-at-hotmail.com) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Thursday, June 3, 2004 at 11:29:54
---------------------------------------------------------------------------

Email: tauria-at-hotmail.com
Name: FRANCIS J. PRONESTI

Organization: INDEPENDENT CONSULTANT

Education: Graduate College

Location: CASTELLANA GROTTE, BARI, ITALY

Question: HELLO,
I HAVE JUST PURCHASED A PHILIPS SEM 505, WHICH WAS SOLD AS SURPLUS
FROM A UNIVERSITY, DUE TO UPGRADING. THIS INSTRUMENT WAS FUNCTIONING
WHEN REMOVED FROM SERVICE AND APPEARS TO BE IN EXCELLENT SHAPE.
UNFORTUNATELY, LIKE IN ALL THESE CIRCUNSTANCES, NO ONE NEW ANYTHING
ABOUT SET UP DOCUMENTATION AND OPERATING INSTRUCTIONS. WHILE I AM NOT
A COMPLETE NEOPHYTE WHEN IT COMES TO ELECTRON MICROSCOPES, I HAVE NO
KNOWLEDGE NOR EXPERIENCE WITH THIS PARTICULAR MAKE AND MODEL. I HAVE
CONTACTED PHILIPS AT THEIR WEBSITE REQUESTING ASSISTANCE, BUT SO FAR
I HAVE HEARD NOTHING. CAN YOU DIRECT ME TO ANY SOURCE OF
DOCUMENTATION FOR THIS MICROSCOPE? I WOULD BE VERY GRATEFUL.
BEST REGARDS, FRANCIS J. PRONESTI (MSME.MSEE,PhD, IEEE MEMBER NO.41399650)

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 14:02:38 2004

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On Jun 3, 2004, at 2:21 AM, Philip Koeck wrote:

} The images were taken by people at Jeol in Japan. As far as I
} understand
} they introduced an image shift during exposure.
} (If you just shift the same image in the computer you get fringes all
} the way to the edge of the micrograph, which is not the case with the
} test images.)
}
} From the Young fringes Jeol claims an information limit better than 2
} Angstroms, but I haven't seen Thon rings beyond about 4 Angstroms in
} any
} of the images. (I think you might have misunderstood this point: Young
} fringes extend up to twice as far as the outermost Thon ring, not only
} beyond the first zero.)
}
} From this discussion I got the impression that manufacturers use Young
} fringes because they extend further than Thon rings and somehow show
} the
} true information limit (which brings me back to my original question
} about the meaningfulness of the Youngfringe criterion).
}
} From Michael O'Keefes E-mails (offline) I understand that he
} distinguishes between information limit and convergence limit. Maybe
} that's what we are seeing here. (All these images were taken at
} magnifications around 50K and defocus between 1000 and 2000 nm.)
}
} The main question for me is how to compare microscopes for the sort of
} microscopy we intend to do. Does the information limit really tell us
} what sort of resolution our reconstructions will have or is that
} determined by the extent of Thon rings.
}
} I can send some images offline or put them on my homepage, if anybody
} wants to see them.
}
Dear Philip,
JEOL did do the test properly, but the Thon rings do not go out as far
as they might. One has to find an appropriate area of the proper
specimen to get good Thon rings. Two of the better specimens are
Pt/Ir, which is strongly scattering and has both crystals (which give
high-res Bragg spots) and amorphous parts (which give continuous
scattering power), and amorphous C, which has continuous scattering
power, but is more weakly scattering and, therefore, a more stringent
test of performance.
The acceptance tests for our scope were performed with Au on C, so
there is continuous power from the C out to ~0.3 nm, and Au Bragg spots
at 0.2 nm and 0.14 nm (as well as some even further out). The Thon
rings do not extend as far out as the Bragg spots, primarily due to the
low scattering power of C beyond 0.3 nm, but one can see segments of
rings in the Bragg spots, so the envelope function has not yet become
zero. Clearly, the scattering into the Bragg spots is real
information, not an artifact, and it corresponds to lattice fringes
visible in the image.
I routinely take images of amorphous C at 2 um underfocus and count
Thon rings to monitor the coherence of the FEG, and the rings extend
beyond the 0.34 nm graphite peak. The scope has to be pretty well
aligned and stigmated to get all the rings, and a thin, flat area of
the specimen has to be found, otherwise areas at different heights will
be at different defocus, and the Thon rings will be washed out. The
service people were able to get many more than 30 rings--I think the
record exceeds 45--but I don't remember the specimen or defocus value
for which they were able to achieve this.
Another potential difficulty may be the mag you chose. 50 kx may be
too low if you are using a CCD, since the Nyquist limit may be a lot
larger than 0.3 nm. For a given pixel size, any spatial frequency one
wishes to measure must correspond to a wavelength greater than or equal
to 2 pixels. Film may also present a problem at that mag; Nyquist is
larger than the film grains, but your scanner may not go to high enough
spatial frequency. We took many films (SO163) at that mag, and we used
several scanners, and only one gave sufficient results to see Thon
rings to 0.3 nm, despite the fact that all the scanners claimed 4000
dpi resolution. The specimen was Pt/Ir, and one could see the 0.2 nm
fringes, even at 2 um underfocus (it took some experience to find them
at this defocus), so we knew that we were getting info at high spatial
frequency, but most of the scanned images (from the poor scanners) had
nothing in the power spectrum at those frequencies.
I'm not sure what your specimens are, so I don't know what would be
acceptable performance. For focal series reconstructions of materials
specimens, you will need to have information out to the spatial
frequency corresponding to the resolution you want, and for something
like biological single-particle analysis, where different particles are
at slightly different defocus you still need information from each
particle beyond the desired resolution, so that averaging the signal
from a large number of particles will give acceptable S/N; however, in
the first case, the resolution you need is likely to be near the info
limit of the instrument, whereas, in the second case, radiation damage
limits the attainable resolution to much poorer than the info limit,
but the ability to obtain maximum resolution in the reconstruction
depends upon how rapidly the envelope function decays. Since we do the
latter, we want to be sure that we get Thon rings out to ~0.3 nm at a
suitable defocus with a weakly-scattering specimen, and the info limit
is less important.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 14:20:13 2004

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On Jun 3, 2004, at 6:16 AM, Lehman, Ann R wrote:

} I have a colleague who has been trying to use TEM to look at isolated
} chloroplasts from a marine alga (Bryopsis). She has also tried looking
} at intact algae. The problem is that following a standard protocol
} (Gta fix using isolation media, Os, UA en bloc, dehyd in ethanols and
} PO, 'epon' embedment; and Pb and UA on-grid), the membranes along the
} perimeter of both the isolates as well as the supposedly intact algae
} appear fragmented, or missing. Mostly missing. The cytoplasmic matrix
} and internal membrane-bound structures such as thykaloids appear
} essentially normal in terms of electron density and membrane
} integrity, so on first inspection it would appear the membranes are
} disappearing following initial fixation, or, they are stubbornly
} invisible.
}
} We thought the missing isolated chloroplast membrane was attributable
} to the isolation procedure, until the intact algae also came up with
} no plasma membrane.
}
} Any comments on ways to keep the PM intact? Or is this a usual
} appearance for these tissues? As others have noted, the chloroplasts
} do remain mostly green following Os.
}
} There was a recent thread regarding missing membranes. We plan to test
} the acetone dehydration idea, and we already incorporate some of the
} suggestions in our standard protocol such as en bloc UA, so before we
} embark on a voyage of discovery using additives, I thought I would
} toss this problem out to any marine algae experts out there. Or anyone
} else who has another thought to share.
}
Dear Ann,
If you have access to the appropriate equipment, you might try
cryo-fixation and cryo-substitution.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 14:47:41 2004

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Dear List,
I am trying to track down a good description--including figures, if
possible--of why the image shifts as a consequence of beam tilt when
the image is defocussed, but not when it is focussed. I have only
found a very short, and not entirely satisfactory, description in a
Royal Microscopy Society handbook from 1984. I have, of course, seen
references to beam-tilt-induced image shift, but not the details of the
mechanism, in several EM texts. Can anyone point me in the right
direction? TIA.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 14:52:42 2004

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On Jun 3, 2004, at 11:34 AM, Tom Phillips wrote:

} I was just reading a superb paper by Mobius et al (2002 J. Histochem.
} Cytochem. 50(1):43-55) in which they use PHEM buffer for their
} fixatives and immunostaining. PHEM is 60 mM PIPES, 25 mM HEPES, 2 mM
} MgCl2, 10 mM EGTA, pH 6.9. Can anyone comment on the rationale behind
} the design of this buffer? Specifically, why EGTA? In addition, why
} a PIPES/HEPES mixture rather than just PIPES or HEPES? Thanks, Tom
}
Dear Tom,
I don't know the pKs of PIPES and HEPES off hand, but that may be a
clue why both are included. EGTA is a Ca++ chelator, so it is
undoubtedly there to lower or buffer the [Ca++]. Since there is quite
likely to be some Ca impurity in the MgCl2, it makes sense to add EGTA,
which binds Ca, but not Mg.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 3 16:59:13 2004

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Not all membranes are equally reactive with osmium. Protein storage
vacuoles in plant cells have a region known as the "globoid" which contains
phytic acid crystals. It was thought to be a non-membrane bound region
within vacuole's matrix. Conventional aldehyde and osmium fixation fails
to show any sign of a membrane. When we used KMnO4 as a fixative, however,
a unit membrane was present surrounding this compartment (Jiang et al.,
2001 J. Cell Biol 155(6):991-1002). This type of phenomenon has been
reported before. Plastid envelopes were observed to become progressively
less distinct using conventional fixation in the fern Paesia but they could
still be seen using KMnO4. Mitochondria membranes in the same cells were
always stained so it seemed to be due to changes in plastid membrane lipids
and not some trivial problem related to the osmication procedure as a whole
(Bell 1983 Eur J Cell Biol 30:279-282). so maybe your membranes aren't
missing - just hiding!

2:41 PM 06/03/04 -0700, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 4 03:27:50 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Bill,

The principle of the beam wobbler to assist focusing (originally an
invention by Le Poole, patented by Philips back in the late 1940s as far
as I remember) has been developed over recent years by Abraham (Bram)
Koster and his group in Utrecht for application in computer-aided
automatic focusing systems for 3D TEM tilt reconstructions. He should be
able to help you.
His publication list may be found in:
http://www.bio.uu.nl/mcb/3dem/publications.html
Best wishes,

Jim

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Thursday, June 03, 2004 10:09 PM
To: microscopy-at-msa.microscopy.com

Dear List,
I am trying to track down a good description--including figures,
if
possible--of why the image shifts as a consequence of beam tilt when
the image is defocussed, but not when it is focussed. I have only
found a very short, and not entirely satisfactory, description in a
Royal Microscopy Society handbook from 1984. I have, of course, seen
references to beam-tilt-induced image shift, but not the details of the
mechanism, in several EM texts. Can anyone point me in the right
direction? TIA.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 4 03:36:50 2004

Contents Retrieved from Microscopy Listserver Archives
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Tom,
THe PHEM buffer was introduced by Manfred Schliwa and von
(van?) Blerkum (OK, I probably didn't spell that one right) in the
mid 80's for their ultrastructural studies of the cytoskeleton. The
idea of the EGTA to remove calcium which can cause cytoskeletal
degradation and supposedly the pH buffering of pipes + hepes works
better than either alone. They may have reported some other reasons
for mixing pipes and hepes, its been a while since I read that
paper. I do think that they showed (or at least reported) that they
got better results with both pipes and hepes than with either alone.
The buffering business is odd because I would have thought that pipes
does just fine thanks at pH 6.9. It also seems odd to me that one
needs to worry about calcium causing depolymerization in the presence
of aldehyde fixatives. In my own work on plant cells, we have found
far better preservation of both actin and microtubules when calcium
replaces the EGTA in a pipes buffer. It is true that animal
microtubules are more sensitive to calcium than are plant
microtubules, so it may well be needed there.
Hope this helps,
Tobias

}
}
} I was just reading a superb paper by Mobius et al (2002 J.
} Histochem. Cytochem. 50(1):43-55) in which they use PHEM buffer for
} their fixatives and immunostaining. PHEM is 60 mM PIPES, 25 mM
} HEPES, 2 mM MgCl2, 10 mM EGTA, pH 6.9. Can anyone comment on the
} rationale behind the design of this buffer? Specifically, why EGTA?
} In addition, why a PIPES/HEPES mixture rather than just PIPES or
} HEPES? Thanks, Tom
}
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 4 03:43:31 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Bill,

The principle of the beam wobbler to assist focusing (originally an
invention by Le Poole, patented by Philips back in the late 1940s as far
as I remember) has been developed over recent years by Abraham (Bram)
Koster and his group in Utrecht for application in computer-aided
automatic focusing systems for 3D TEM tilt reconstructions. He should be
able to help you.
His publication list may be found in:
http://www.bio.uu.nl/mcb/3dem/publications.html
Best wishes,

Jim

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Thursday, June 03, 2004 10:09 PM
To: microscopy-at-msa.microscopy.com

Dear List,
I am trying to track down a good description--including figures,
if
possible--of why the image shifts as a consequence of beam tilt when
the image is defocussed, but not when it is focussed. I have only
found a very short, and not entirely satisfactory, description in a
Royal Microscopy Society handbook from 1984. I have, of course, seen
references to beam-tilt-induced image shift, but not the details of the
mechanism, in several EM texts. Can anyone point me in the right
direction? TIA.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 4 03:44:12 2004

Contents Retrieved from Microscopy Listserver Archives
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Greetings,
In his comment about the "missing membranes", Jim Chalcroft
wrote, in part...
}
} Although not directly relevant in your case, some help might come
} from the discovery recently by P. Walther that cell membranes, which
} are notoriously poorly contrasted after freeze substitution, are
} rendered easily visible if 1 - 5% water is maintained in the
} substitution fluids.

Can Jim (or anyone else) give citation to that result? It
sounds extremely interesting, if a little iconoclastic considering
all the wise advice given over the years to eliminate water
ruthlessly from freeze substitution routines.

Thanks,
Tobias
--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 4 04:20:51 2004

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Dear Debby, Richard, Tobias etc.,

Yes, the following published paper refers to his discovery:
Walther P, Ziegler A. (2002) Freeze Substitution of High-Pressure Frozen Samples: The Visibility of Biological Membranes is Improved when the Substitution Medium Contains Water. Journal of Microscopy 208, 3-10.

Jim

-----Original Message-----
} From: Debby Sherman [mailto:dsherman-at-purdue.edu]
Sent: Thursday, June 03, 2004 9:28 PM
To: James Chalcroft

Hi

If it is of assistance to you I have some basic instructions in the
operation of the Philips 505 that I would be happy to mail on to you? In
our training courses we have and use our own operating procedures for most
SEM, TEM and EDS systems

Good luck

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0)7711 606967
www.emcourses.com

----- Original Message -----
} From: "by way of Ask-A-Microscopist" {tauria-at-hotmail.com}
To: {microscopy-at-ns.microscopy.com}
Sent: Thursday, June 03, 2004 7:45 PM

Dear listers: below is a job listing that I am posting for a colleague.
Please do not respond to me. Respond to the addresses supplied in the
announcement. The position is for US citizens only, as this is a secure
facility. Good luck.

Materials and Device Characterization Scientist/Engineer

Maxion Technologies, Inc., located near the University of Maryland,
College Park campus, has a post-doctoral/contractor position open for a
physicist, materials scientist or electrical engineer with experience in
micro-structural, chemical, electrical and optical characterization of
advanced compound semiconductor materials and devices using a scanning
electron microscope and associated tools including Energy /Wavelength
Dispersive X-Ray Analysis, Cathodoluminescence, Electron Beam Induced
Current and Electron Backscattered Kikuchi Pattern Imaging (EBKP). The
primary job responsibility will be to characterize bulk materials and
thin films as well as complex device structures with the objective of
shedding fundamental light on the material and device properties,
thereby assisting with ongoing projects. Ph.D in Physics, Materials
Science or Electrical Engineering is preferred. Candidates with MS or BS
degree but with 3-5 years of relevant experience in the field will also
be considered. The position is for an initial period of 1-2 years with a
possibility for extension. The successful candidate will work with both
Maxion and Army Research Laboratory (ARL) scientists/engineers at the
ARL site in Adelphi, Maryland. US Citizenship is required. Maxion is an
equal opportunity employer. Send resume to dwortman-at-maxion.com
{mailto:dwortman-at-maxion.com } . For specific job related questions,
please send email to prboyd-at-arl.army.mil {mailto::prboyd-at-arl.army.mil}

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 05:13:27 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (sswaffe-at-abv.bg) from
http://microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on
Sunday, June 6, 2004 at 04:07:47
---------------------------------------------------------------------------

Email: sswaffe-at-abv.bg
Name: Veselin

Organization: 54 st.Ivan Rilski

Education: 6-8th Grade Middle School

Location: Sofia, Bulgaria

Question: Should I use solvents when cleaning lenses from immersion
oil or just otical lens tissue?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 08:56:38 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (donaldawbrey-at-texashealth.org) from
http://www.microscopy.org/MicroscopyListserver/MLFormMail.html on
Monday, June 7, 2004 at 07:43:28
---------------------------------------------------------------------------

Email: donaldawbrey-at-texashealth.org
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Image Analysis

Title-Subject: [Microscopy] [Filtered] Image Analysis Salary Question

Question: Hello fellow micronetters,

Does anyone know of any salary information for image analysis technicians.

I happen to be a histotechnician with 15 years experience. As far as
I know I may be one of very, very few people who are histotechnicians
and also do IA. Most of the people who perform this task are
cytology technicians.

That is my quandry.......

I am paid a histotechnician's salary and I believe that I am not
being compensated properly.

If any one knows anything about IA salary please respond.

Thank you very much.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 08:55:37 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (wharton.sinkler-at-uop.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Monday, June 7, 2004 at 07:03:05
---------------------------------------------------------------------------

Email: wharton.sinkler-at-uop.com
Name: Wharton Sinkler

Organization: UOP LLC

Title-Subject: [Microscopy] [Filtered] MListserver:

Question:
I'm curious whether there are commercially available attachments for
SEM which can measure micro-hardness, or crush strength (with an
indenter) on particles down to the 20 micron range. I can
envisualize something in which a highly tilted sample would be imaged
and simultaneously impinged on by an indenter diamond or steel tip,
subjected to a ramping force, then recording the force at which the
crushing or a specific indentation depth occurs. I would imagine an
SEM would be a suitable tool for imaging and positioning the tip.

If anyone is aware of such an attachment please inform. Similarly if
you have experience with something of this nature I'd be curious to
know some of the details.

Thanks,
Wharton

****************************************************************
Wharton Sinkler, PhD.
UOP LLC
25 E. Algonquin Rd.
Des Plaines, IL 60017-5017
tel. 847-391-3878
fax. 847-391-3719
mailto Wharton.Sinkler-at-uop.com

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 11:02:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Jun 7, 2004, at 7:22 AM, by way of MicroscopyListserver wrote:

} Question:
} I'm curious whether there are commercially available attachments for
} SEM which can measure micro-hardness, or crush strength (with an
} indenter) on particles down to the 20 micron range. I can envisualize
} something in which a highly tilted sample would be imaged and
} simultaneously impinged on by an indenter diamond or steel tip,
} subjected to a ramping force, then recording the force at which the
} crushing or a specific indentation depth occurs. I would imagine an
} SEM would be a suitable tool for imaging and positioning the tip.
}
Dear Wharton,
This also may be a question for the AFM people. Not being one of
them, I have no idea whether an AFM tip can exert sufficient force
without damaging itself, but it could probably detect the dimple
afterwards.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 11:48:56 2004

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There was an article entitled "Lens Cleaning - Best Practices Review," by
C.V. Duke in the July issue of Microscopy Today. I will send you a PDF of
the article in a separate email.

Ron Anderson, Editor
Microscopy Today

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:sswaffe-at-abv.bg]
Sent: Monday, June 07, 2004 6:40 AM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (sswaffe-at-abv.bg) from
http://microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on
Sunday, June 6, 2004 at 04:07:47
---------------------------------------------------------------------------

Email: sswaffe-at-abv.bg
Name: Veselin

Organization: 54 st.Ivan Rilski

Education: 6-8th Grade Middle School

Location: Sofia, Bulgaria

Question: Should I use solvents when cleaning lenses from immersion
oil or just otical lens tissue?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 13:22:54 2004

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Wharton: contact a company called Ominprobe
(http://www.omniprobe.com). They have something to do, I believe. They
love this sort of thing.

by way of MicroscopyListserver wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (wharton.sinkler-at-uop.com) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Monday, June 7, 2004 at 07:03:05
} ---------------------------------------------------------------------------
}
}
} Email: wharton.sinkler-at-uop.com
} Name: Wharton Sinkler
}
} Organization: UOP LLC
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question:
} I'm curious whether there are commercially available attachments for
} SEM which can measure micro-hardness, or crush strength (with an
} indenter) on particles down to the 20 micron range. I can envisualize
} something in which a highly tilted sample would be imaged and
} simultaneously impinged on by an indenter diamond or steel tip,
} subjected to a ramping force, then recording the force at which the
} crushing or a specific indentation depth occurs. I would imagine an
} SEM would be a suitable tool for imaging and positioning the tip.
}
} If anyone is aware of such an attachment please inform. Similarly if
} you have experience with something of this nature I'd be curious to
} know some of the details.
}
} Thanks,
} Wharton
}
} ****************************************************************
} Wharton Sinkler, PhD.
} UOP LLC
} 25 E. Algonquin Rd.
} Des Plaines, IL 60017-5017
} tel. 847-391-3878
} fax. 847-391-3719
} mailto Wharton.Sinkler-at-uop.com
}
}
}
} ---------------------------------------------------------------------------
}
}
}

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 15:06:47 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello all,

I'm looking for spring metal clips that I will screw into one portion
of a stage insert (that is being machined custom), that will hold
down a slide set in this insert.

Good source anyone?

Sorry for the double post for some.

Best,

Gary

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 7 15:29:42 2004

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Hi
We have an old, not-worth-saving, Philips 410 TEM. If there are
some small parts etc. you would like please let me know and I will see if
we can send them to you. I may be able to remove the small and large
screens if anyone wants those - they had been recently recoated and are in
good condition. Parts are free but you must pay for shipping (fedX number?).
Also I have some film holder plates (like new) from an EM300 (fits
both 410 and 300 series) as well as EM300 specimen holder exchange tips.

Jon Mulholland, Director
Cell Sciences Imaging Facility
Beckman Center, B050
Stanford University School of Medicine
Stanford, CA 94305-5301

voice 650-725-7532
fax 650-725-4951

http://taltos.stanford.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 06:18:53 2004

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hi all!

just a simple question about SEM!

how can I calculate a FE-SEM resolution ? does some calculation theories
exist?
how can it be verified practicaly??

thanx in advance...

Sylvain Maury

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 09:22:19 2004

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Hello,

Does anyone know what the depreciation period is for a Transmission
electron microscope?

Thanks,

Mike G

Michael P. Goheen
Electron Microscopy Lab
Dept. of Pathology & Lab Medicine
Indiana University School of Medicine
Tel. 317-274-7604
Fax 317-274-5346
mgoheen-at-iupui.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 10:07:37 2004

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Try here for a start.

http://www.tut.fi/units/ms/elm/laitteet/ensem.htm

FCM

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: Becky Holdford [mailto:r-holdford-at-ti.com]
Sent: Monday, June 07, 2004 2:41 PM
To: wharton.sinkler-at-uop.com
Cc: microscopy-at-ns.microscopy.com

Wharton: contact a company called Ominprobe
(http://www.omniprobe.com). They have something to do, I believe. They

love this sort of thing.

by way of MicroscopyListserver wrote:

}
}
} ----------------------------------------------------------------------
} --------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (wharton.sinkler-at-uop.com) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Monday, June 7, 2004 at 07:03:05
}
------------------------------------------------------------------------
---
}
}
} Email: wharton.sinkler-at-uop.com
} Name: Wharton Sinkler
}
} Organization: UOP LLC
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question:
} I'm curious whether there are commercially available attachments for
} SEM which can measure micro-hardness, or crush strength (with an
} indenter) on particles down to the 20 micron range. I can envisualize

} something in which a highly tilted sample would be imaged and
} simultaneously impinged on by an indenter diamond or steel tip,
} subjected to a ramping force, then recording the force at which the
} crushing or a specific indentation depth occurs. I would imagine an
} SEM would be a suitable tool for imaging and positioning the tip.
}
} If anyone is aware of such an attachment please inform. Similarly if
} you have experience with something of this nature I'd be curious to
} know some of the details.
}
} Thanks,
} Wharton
}
} ****************************************************************
} Wharton Sinkler, PhD.
} UOP LLC
} 25 E. Algonquin Rd.
} Des Plaines, IL 60017-5017
} tel. 847-391-3878
} fax. 847-391-3719
} mailto Wharton.Sinkler-at-uop.com
}
}
}
} ----------------------------------------------------------------------
} -----
}
}
}

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 11:49:27 2004

Contents Retrieved from Microscopy Listserver Archives
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That's a question for the accountants and the IRS.

-----Original Message-----
} From: Goheen, Michael P. [mailto:mgoheen-at-iupui.edu]
Sent: Tuesday, June 08, 2004 10:40 AM
To: Microscopy-at-MSA.Microscopy.com

Hello,

Does anyone know what the depreciation period is for a Transmission
electron microscope?

Thanks,

Mike G

Michael P. Goheen
Electron Microscopy Lab
Dept. of Pathology & Lab Medicine
Indiana University School of Medicine
Tel. 317-274-7604
Fax 317-274-5346
mgoheen-at-iupui.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 13:02:27 2004

Contents Retrieved from Microscopy Listserver Archives
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The annual EMBO EM course will be held this year at the Pasteur Institute in Paris, France. Course dates are September 12 - 22 2004. More details can be found on the following web page.

http://www.embl-heidelberg.de/courses/ElectronMicroscopy04/

Regards,

Paul Webster.

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 13:21:29 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

We have been a large EM unit for many years and have had
several TEMs (currently running 9). I cannot remember
disposing of any of them less than 20 years old.

It would be different if you had only one TEM and wanted to
keep up with new developments, 5 to 7 years?

Regards,
Ron

On Tue, 8 Jun 2004 09:40:05 -0500 "Goheen, Michael P."
{mgoheen-at-iupui.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hello,
}
} Does anyone know what the depreciation period is for a Transmission
} electron microscope?
}
} Thanks,
}
} Mike G
}
} Michael P. Goheen
} Electron Microscopy Lab
} Dept. of Pathology & Lab Medicine
} Indiana University School of Medicine
} Tel. 317-274-7604
} Fax 317-274-5346
} mgoheen-at-iupui.edu
}
}
}
}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 15:06:12 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,
When I was at a Fortune 500 Company Microscopy Lab we depreciated all of
our TEMs for 10 yrs. We had 4 TEMs.
Regards,
Judy Murphy

Ron Doole wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi,
}
} We have been a large EM unit for many years and have had
} several TEMs (currently running 9). I cannot remember
} disposing of any of them less than 20 years old.
}
} It would be different if you had only one TEM and wanted to
} keep up with new developments, 5 to 7 years?
}
} Regards,
} Ron
}
} On Tue, 8 Jun 2004 09:40:05 -0500 "Goheen, Michael P."
} {mgoheen-at-iupui.edu} wrote:
}
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } Hello,
} }
} } Does anyone know what the depreciation period is for a Transmission
} } electron microscope?
} }
} } Thanks,
} }
} } Mike G
} }
} } Michael P. Goheen
} } Electron Microscopy Lab
} } Dept. of Pathology & Lab Medicine
} } Indiana University School of Medicine
} } Tel. 317-274-7604
} } Fax 317-274-5346
} } mgoheen-at-iupui.edu
} }
} }
} }
} }
} }
}
} ----------------------
} Mr. R.C. Doole
} Department of Materials,
} University of Oxford.
} Parks Road, Oxford. OX1 3PH. UK.
} Phone +44 (0) 1865 273701
} Fax +44 (0) 1865 283333
} ron.doole-at-materials.ox.ac.uk
} http://www-em.materials.ox.ac.uk/
} *********************************

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 15:27:52 2004

Contents Retrieved from Microscopy Listserver Archives
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I am doing basic ultramicrotomy on lowricryl embedded lung tissue. When thin
sectioning the bottome of the tissue sticks to the knife causing it to
crinkle. I have changed every parameter I could think of from water level to
clearance angle. Does anyone have any suggestions?

Todd Hamm
Oklahoma Medical Research Foundation
Oklahoma City, Ok

_________________________________________________________________
FREE pop-up blocking with the new MSN Toolbar – get it now!
http://toolbar.msn.click-url.com/go/onm00200415ave/direct/01/

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 15:33:09 2004

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Hi all,
Does anyone on the list have experience imaging DNA after rotary
shadowing and/or negative staining?
I need some advice and would like to correspond off-list.
thanks!

Beth
**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 16:18:19 2004

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Assuming it is the same as a SEM, you can
use either accelerated or straight line depreciation.
Typical depreciation period is five years. But you
only get 10% the first year.

gary g.

At 07:40 AM 6/8/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 17:04:59 2004

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If there is a way to calculate resolution directly,
that would be terrific. However, the only way I
know is by experiment. The method is not all that
exact and is not easy to perform. But if you want
to compare one SEM vs. another, it will work.

What is needed is a very (very) sharp edge. I use
a 30u Pt aperture Faraday cup. Center an edge
at zero tilt on the display. Increase mag as high
as you can reasonably get and handle (at high mag,
all things become significant obstacles). Make
the image range between black and white, i.e., full
dynamic range. If the SEM has a waveform display
mode, use that to get from top limit to bottom limit.

What you will see is:

---
\
\
\
\
\
-----

as the beam moves from the aperture body (left side) to
the aperture hole (right side). Then measure the
transcending horizontal distance from 90% to 10% P-P
and this is your resolution figure...so to speak.

For modest resolutions of perhaps 50-100A, this method
may work OK. For higher resolution SEMs, I doubt that
it would work since the margin is so small. I have
not tried it on SEMs with really high resolution figures.

No claim of authorship for this method, and I forget
how I came across this. I probably got it from this
list some years ago.

An alternate method may be to measure the "clarity" of an atomic lattice
using EBSD (if you have it). Since the lattice spacing
is known, how well the SEM can resolve this ought to
be a method of determining resolution. But perhaps
this is wild speculation on my part. I may try this
later on.

gary g.

At 04:37 AM 6/8/2004, you wrote:

} hi all!
}
} just a simple question about SEM!
}
} how can I calculate a FE-SEM resolution ? does some calculation theories
} exist?
} how can it be verified practicaly??
}
} thanx in advance...
}
} Sylvain Maury

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 8 17:52:47 2004

Contents Retrieved from Microscopy Listserver Archives
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I had been active in microscopy for nearly 30 years until I was 'kicked
upstairs' a few years back. At our federal department here in
'almost-Stanley-Cup-hockey-champions-land', we have some 35 microbeam
instruments scattered across the country, with an average age of 13 years.
In my former lab, we had a workhorse EM400T that was 20 years old, yet still
useable. One of the principal reasons for that longevity was the
acquisition of a CM20 FEG ~12 years ago, which picked up a lot of the load.
When I was Group Leader I never hesitated to trot out the '10 year' figure,
except that I used it, not in the depreciation sense, but more in the 'now
outmoded' sense.

Now, here's the problem, be very careful of what figures you quote and to
whom. We were audited by the Canadian federal Auditor-General last year and
it was a most enlightening/frightening experience. These people (and
probably accountants from Finance Depts, etc) don't know an SEM from a probe
(literally, they even had side-by-side pictures of the two and claimed them
as evidence of 'identical scientific instruments'). Holding an old
instrument together with binder twine and scotch tape made no impresssion
whatsoever. So long as an innocent tech replied that 'we use this
instrument only about 10% of the time" (emergency backup, spare parts, etc),
that was all they wanted to know and hung us out to dry for poor utilization
of capability.

The other side of the coin is when you know you really need a current
generation instrument, quote the 10 year number, but then have to explain to
management why the incumbent still runs reasonably well, and perhaps even is
still just fine for clients with simple requests.

A murky picture to which I have no clear answers, other than to proceed
cautiously!

Tom

Dr. Tom Malis
Scientist Advisor
Natural Resources Canada
Govt. of Canada
Phone: 613-995-7358
cell: 613-371-4577
FAX: 613-947-6606
malis-at-nrcan.gc.ca

-----Original Message-----
} From: Judy Murphy
To: Ron Doole; home; office
Cc: Goheen, Michael P.; Microscopy community
Sent: 6/8/2004 4:22 PM

Hi,
When I was at a Fortune 500 Company Microscopy Lab we depreciated all of
our TEMs for 10 yrs. We had 4 TEMs.
Regards,
Judy Murphy

Ron Doole wrote:
}
}
------------------------------------------------------------------------
------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
} Hi,
}
} We have been a large EM unit for many years and have had
} several TEMs (currently running 9). I cannot remember
} disposing of any of them less than 20 years old.
}
} It would be different if you had only one TEM and wanted to
} keep up with new developments, 5 to 7 years?
}
} Regards,
} Ron
}
} On Tue, 8 Jun 2004 09:40:05 -0500 "Goheen, Michael P."
} {mgoheen-at-iupui.edu} wrote:
}
} }
} }
} }
------------------------------------------------------------------------
------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} } To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
------------------------------------------------------------------------
-------
} }
} } Hello,
} }
} } Does anyone know what the depreciation period is for a Transmission
} } electron microscope?
} }
} } Thanks,
} }
} } Mike G
} }
} } Michael P. Goheen
} } Electron Microscopy Lab
} } Dept. of Pathology & Lab Medicine
} } Indiana University School of Medicine
} } Tel. 317-274-7604
} } Fax 317-274-5346
} } mgoheen-at-iupui.edu
} }
} }
} }
} }
} }
}
} ----------------------
} Mr. R.C. Doole
} Department of Materials,
} University of Oxford.
} Parks Road, Oxford. OX1 3PH. UK.
} Phone +44 (0) 1865 273701
} Fax +44 (0) 1865 283333
} ron.doole-at-materials.ox.ac.uk
} http://www-em.materials.ox.ac.uk/
} *********************************

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 02:08:40 2004

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The method and period of depreciation should take into account the
reason you are deprecating the equipment. If it is to properly
charger the user. It should be reflect the expected usage reflect
the increasing maintenance cost if the cost does increase with age.
If it is for tax reasons you need to consult you tax accountants and
do what is most advantageous to the bottom line.

If you choose a heavily loaded front end depreciation document your
reasons very well so you don't run in the problems that Tom has and
discuss it with the auditor before the fact and get him to sign off
on it to stay out of that kind of problem.

Billing the cost of the equipment unfairly is second only to space
wars in problems in facility meetings. Be sure that you don't run a
fowl of IRS if you are running a store or the new rules on billing
that came into effect a few years ago if you are in the USA.

When we increased billing on vehicles so there was money to replace
them the professors that purchased the vehicles and put them in the
common pool were very unhappy at paying for them twice. They
continued to be upset for over a year. So finding a fair way to bill
uses is important.

Gordon
Gordon Couger

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

:
:
: ------------------------------------------------------------------
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America
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: ------------------------------------------------------------------
-------------
:
: I had been active in microscopy for nearly 30 years until I was
'kicked
: upstairs' a few years back. At our federal department here in
: 'almost-Stanley-Cup-hockey-champions-land', we have some 35
microbeam
: instruments scattered across the country, with an average age of
13 years.
: In my former lab, we had a workhorse EM400T that was 20 years old,
yet still
: useable. One of the principal reasons for that longevity was the
: acquisition of a CM20 FEG ~12 years ago, which picked up a lot of
the load.
: When I was Group Leader I never hesitated to trot out the '10
year' figure,
: except that I used it, not in the depreciation sense, but more in
the 'now
: outmoded' sense.
:
: Now, here's the problem, be very careful of what figures you quote
and to
: whom. We were audited by the Canadian federal Auditor-General
last year and
: it was a most enlightening/frightening experience. These people
(and
: probably accountants from Finance Depts, etc) don't know an SEM
from a probe
: (literally, they even had side-by-side pictures of the two and
claimed them
: as evidence of 'identical scientific instruments'). Holding an
old
: instrument together with binder twine and scotch tape made no
impresssion
: whatsoever. So long as an innocent tech replied that 'we use this
: instrument only about 10% of the time" (emergency backup, spare
parts, etc),
: that was all they wanted to know and hung us out to dry for poor
utilization
: of capability.
:
: The other side of the coin is when you know you really need a
current
: generation instrument, quote the 10 year number, but then have to
explain to
: management why the incumbent still runs reasonably well, and
perhaps even is
: still just fine for clients with simple requests.
:
: A murky picture to which I have no clear answers, other than to
proceed
: cautiously!
:
: Tom
:
: Dr. Tom Malis
: Scientist Advisor
: Natural Resources Canada
: Govt. of Canada
: Phone: 613-995-7358
: cell: 613-371-4577
: FAX: 613-947-6606
: malis-at-nrcan.gc.ca
:
:
: -----Original Message-----
: } From: Judy Murphy
: To: Ron Doole; home; office
: Cc: Goheen, Michael P.; Microscopy community
: Sent: 6/8/2004 4:22 PM
: Subject: [Microscopy] Re: Re: Depreciation period
:
:
:
: ------------------------------------------------------------------
------
: ------
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America
: To Subscribe/Unsubscribe --
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: On-Line Help
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: ------------------------------------------------------------------
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: -------
:
: Hi,
: When I was at a Fortune 500 Company Microscopy Lab we depreciated
all of
: our TEMs for 10 yrs. We had 4 TEMs.
: Regards,
: Judy Murphy
:
:
:
:
:
: Ron Doole wrote:
: }
: }
: ------------------------------------------------------------------
------
: ------
: } The Microscopy ListServer -- Sponsor: The Microscopy Society of
: America
: } To Subscribe/Unsubscribe --
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: } On-Line Help
: http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
: }
: ------------------------------------------------------------------
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: -------
: }
: } Hi,
: }
: } We have been a large EM unit for many years and have had
: } several TEMs (currently running 9). I cannot remember
: } disposing of any of them less than 20 years old.
: }
: } It would be different if you had only one TEM and wanted to
: } keep up with new developments, 5 to 7 years?
: }
: } Regards,
: } Ron
: }
: } On Tue, 8 Jun 2004 09:40:05 -0500 "Goheen, Michael P."
: } {mgoheen-at-iupui.edu} wrote:
: }
: } }
: } }
: } }
: ------------------------------------------------------------------
------
: ------
: } } The Microscopy ListServer -- Sponsor: The Microscopy Society
of
: America
: } } To Subscribe/Unsubscribe --
: http://www.msa.microscopy.com/MicroscopyListserver
: } } On-Line Help
: http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
: } }
: ------------------------------------------------------------------
------
: -------
: } }
: } } Hello,
: } }
: } } Does anyone know what the depreciation period is for a
Transmission
: } } electron microscope?
: } }
: } } Thanks,
: } }
: } } Mike G
: } }
: } } Michael P. Goheen
: } } Electron Microscopy Lab
: } } Dept. of Pathology & Lab Medicine
: } } Indiana University School of Medicine
: } } Tel. 317-274-7604
: } } Fax 317-274-5346
: } } mgoheen-at-iupui.edu
: } }
: } }
: } }
: } }
: } }
: }
: } ----------------------
: } Mr. R.C. Doole
: } Department of Materials,
: } University of Oxford.
: } Parks Road, Oxford. OX1 3PH. UK.
: } Phone +44 (0) 1865 273701
: } Fax +44 (0) 1865 283333
: } ron.doole-at-materials.ox.ac.uk
: } http://www-em.materials.ox.ac.uk/
: } *********************************
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 02:21:40 2004

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because i'm an intern in a microelectronics analysis laboratory in France, working
on a HR FE-SEM, and because of that, i have to know all details and informations on
SEM and methods used for...as much as possible.

The manufacturer gave a resolution of about 15A at low voltage and 9A at high
voltage.
i just want to know how can i verify it with theory and practice.
I think i'll call the vendor...and get a copy of Goldstein (a little expensive for
me :-[ )

thanx.

Sylvain

Warren E Straszheim a écrit :

} I would think that would be quite dependent on the conditions and the
} sample. A program like Electron Flight Simulator might be able to estimate
} a value given the appropriate parameters. Still, it may only produce the
} maximum possible resolution. Actual performance will depend on your skill
} in operation.
}
} Most vendors should be able to quote a number, but that will depend on the
} sample. Maybe than can suggest the maximum possible resolution for your
} sample, but maybe not.
}
} Why do you ask?
}
} Warren
}
} At 06:37 AM 6/8/2004, you wrote:
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } hi all!
} }
} } just a simple question about SEM!
} }
} } how can I calculate a FE-SEM resolution ? does some calculation theories
} } exist?
} } how can it be verified practicaly??
} }
} } thanx in advance...
} }
} } Sylvain Maury

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 04:05:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (caneiro-at-cab.cnea.gov.ar) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, June 8, 2004 at 14:19:23
---------------------------------------------------------------------------

Email: caneiro-at-cab.cnea.gov.ar
Name: Alberto Caneiro

Organization: Instituto Balseiro

Title-Subject: [Microscopy] [Filtered] CRT for EDAX PV9900

Question: We have a PV9900 EDAX EDS system. We are having problems
with the monitor (CRT) of this equipment. We are looking for a
replacement for it. We are willing to purchase it at a reasonable
price from whoever can supply it.

Many thanks in advance.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 04:13:43 2004

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For measurement of the spatial resolution have a look at
D. C. Joy: "SMART - a program to measure SEM resolution and imaging performance"
Journal of Microscopy, vol. 208 (2002) 24-34.

Best regards,
Jorgen.

{:::} --- {:::} --- {:::} --- {:::} --- {:::} --- {:::}

Joergen B. Bilde-Soerensen
Senior Research Scientist, Ph. D.
Materials Research Department
Risoe National Laboratory
DK-4000 Roskilde
Denmark

e-mail: j.bilde-at-risoe.dk
phone: +45 4677 5802 (direct)
phone: +45 4677 4677 (switchboard)
fax: +45 4677 5758
website: http://www.risoe.dk/afm/Personal/jqbi/jqbi.htm

-----Original Message-----
} From: sylvain maury [mailto:sylvain.maury-at-thalesgroup.com]
Sent: 8. juni 2004 13:37
To: Microscopy community

Hello listers,

We have in our TEM storeroom several LKB knifemakers which have not been
used for some years since everyone here prefers the comfort and edge
longevity of diamond knives for ultrathin sectioning. Recently I
received advertising material referring to an add-on device called a
GUM-symparter which apparently converts the LKB knifemaker into a
wondrous instrument by applying the "newest principles of equilibrium
weighting" to produce optimal triangular glass knives. Could this be a
useful acquisition for labs like ours?
I would be interested to hear from any lab that has bought and used this
attachment; in particular as to whether it has lived up to expectations.
Best wishes,

Jim

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 06:47:30 2004

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When I worked for a major US rubber company instrument depreciation was
used more as a tool for determining department budgets then a tool for up
grading. While I remain blissfully ignorant of the booking/tax conditions
of management, we were often told that long depreciation such as 10 years
on a GC helped increase the department budget, even if the GC was just a
shell with the detector, column and ports stripped off of it. We
transferred a SEM to another department (they had a EDS unit but no SEM, we
had a SEM but no EDS) and for one year we had extra money because we no
longer had a depreciating SEM to payoff. The following year we had less
money because we no longer had that SEM. If this sounds confusing, it is.
If I remember correctly we depreciated everything for 10 years and sometime
(?) ran a second 10 years.

More to the point, the problem with long depreciation appears to be the
inability to purchase new equipment while an old and now obsolete or
non-functioning instrument still has appreciable value due to the extended
depreciation. I've seen instruments, which existed, only as nameplates and
owner's manuals in a desk drawer, still listed on the equipment roster
because the depreciation value was too high to be dispose of.

The second most limiting parameter is being forced to answer the
replacement question: "What can't you do today that you could do
yesterday?" This question is more of a political and cultural limitation
and a good topic for another day.

Frank Karl

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 08:00:21 2004

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Todd:

How long did you polymerize the blocks and at what temperature. Usually I
polymerize the Lowicryl with UV light at -20C for 2-3 days and then an
additional day or two at room temperature (this room temp polymerization
does not affect any of the immunoEM labeling sensitivity). The resin is
much more cuttable.

Also, if your diamond knife is a little dull try another one or if the edge
is not really clean sometimes the sections cling to whatever film is on that
knife edge from previous cutting sessions.

good luck

Karen Bentley

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

-----Original Message-----
} From: todd hamm [mailto:ripbnowell-at-hotmail.com]
Sent: Tuesday, June 08, 2004 4:47 PM
To: Microscopy-at-MSA.Microscopy.Com

I am doing basic ultramicrotomy on lowricryl embedded lung tissue. When thin

sectioning the bottome of the tissue sticks to the knife causing it to
crinkle. I have changed every parameter I could think of from water level to

clearance angle. Does anyone have any suggestions?

Todd Hamm
Oklahoma Medical Research Foundation
Oklahoma City, Ok

_________________________________________________________________
FREE pop-up blocking with the new MSN Toolbar - get it now!
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From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 08:46:52 2004

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Has anyone / Is anyone running the JEOL DSG software (i.e. DSGPlus)
under Win NT or 2K rather than Win 9x? If so how did you get things
running?

Thanks.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Supervisor
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 09:49:44 2004

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Hi all,

I am not very happy with my current supplier of secondary gold
immunoreagents. I would appreciate input regarding potential new
suppliers, as well as general comments about, say, the shelf-life,
stability, sensitivity of your favorite immunoreagent brand.

Thanks--Peter

_______________________________
Peter Rohloff, PhD
Laboratory of Molecular Parasitology
Medical Scholars Program
University of Illinois at Urbana-Champaign

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 10:34:34 2004

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Does anyone know how CT numbers are mapped to the pixel values in a DICOM
image?

_________________________________________________________________
FREE pop-up blocking with the new MSN Toolbar – get it now!
http://toolbar.msn.click-url.com/go/onm00200415ave/direct/01/

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 11:34:04 2004

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Which Lowacryl resin are you using? This makes a very big difference in
sectioning characteristics.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 6/9/04 8:18 AM, "Bentley, Karen" {Karen_Jensen-at-URMC.Rochester.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Todd:
}
} How long did you polymerize the blocks and at what temperature. Usually I
} polymerize the Lowicryl with UV light at -20C for 2-3 days and then an
} additional day or two at room temperature (this room temp polymerization
} does not affect any of the immunoEM labeling sensitivity). The resin is
} much more cuttable.
}
} Also, if your diamond knife is a little dull try another one or if the edge
} is not really clean sometimes the sections cling to whatever film is on that
} knife edge from previous cutting sessions.
}
} good luck
}
} Karen Bentley
}
} Karen L. Bentley, M.S.(previously Jensen)
} Associate Scientist & Project Manager
} Electron Microscope Research Core
} University of Rochester Medical Center
} Rochester, NY 14642
} 585-275-1954
}
}
} -----Original Message-----
} } From: todd hamm [mailto:ripbnowell-at-hotmail.com]
} Sent: Tuesday, June 08, 2004 4:47 PM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] Sectioning Lowricryl
}
}
}
}
} ----------------------------------------------------------------------------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ----------------------------------------------------------------------------
} ---
}
} I am doing basic ultramicrotomy on lowricryl embedded lung tissue. When thin
}
} sectioning the bottome of the tissue sticks to the knife causing it to
} crinkle. I have changed every parameter I could think of from water level to
}
} clearance angle. Does anyone have any suggestions?
}
} Todd Hamm
} Oklahoma Medical Research Foundation
} Oklahoma City, Ok
}
} _________________________________________________________________
} FREE pop-up blocking with the new MSN Toolbar - get it now!
} http://toolbar.msn.click-url.com/go/onm00200415ave/direct/01/
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 12:54:15 2004

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In a message dated 6/9/04 2:03:46 PM, tommy91779-at-hotmail.com writes:

} Does anyone know how CT numbers are mapped to the pixel values in a DICOM
} image?

The DICOM standard describes in detail the greyscale standard display
function that presents normalized rendering of image values. It is heavily based on
the non-linear response of human vision to luminance changes. You can download
the standard and much other information on DICOM formats in pdf format from
{www.dclunie.com} . There is even a tool to import DICOM files into Photoshop.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 13:00:08 2004

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Hi listers,

I have an MT2C, actually, but I have a problem with too much laxity in the
binoch head. I am trying to get this old microtome into usable shape. I
was fnally able to free the up and down part of the arm to raise and lower
the binoch (it's a bit stiff but can now be adjusted).

Now I have too much wiggle in the bit that allows the binoch head to move
up and down (similar to a nodding motion). I somehow need to increase the
tension or friction or something so the binoch head hold steady now matter
what the pivot. Now it just keeps nodding off, you know, resting it;s
little head on the fluorescent light. Like a new baby this thing can't
hold it head up.

Any suggestions? I'm trying to take the joint apart and figure it out, but
I'm stumped as to how to increase the tension/pressure whatever it is.

On a similar theme-- Does anybody know where I can get a
reconditioned/refurbished ultramicrotome? I have an old LKB that gives all
the users a little jolt every time they complete the circuit with their
bodies by touching the microtome and the controller box. We are tired of
having sectioning be a shocking experience and we'd like to replace it.
I'd like something newer than the LKB or MT2C, something like an Ultracut
E. Any ideas?

Nodding off in Norfolk,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 13:24:32 2004

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Peter,
Immunogold reagents are a peculiar lot. The characteristics of the gold
particle itself is dependant on which reducing agent is
used. Unfortunately, the most common method involves the reduction of
chloroauric acid with citrate-tannic acid. There is a stochiometric
relationship between the ratio of the chemicals used and diameter of the
gold particle produced. This results in tremendous affinity for
cytoskeletal components. Tannic acid is a mordant often used to preserve
microtubules. However, if the reducing agent is sodium borohydride, one
can circumvent this affinity. Jansen used to be the only company that
advertised that their gold was produced by the reduction of chloroauric
acid by sodium borohydride. I believe they were purchased by Amersham, who
treats this procedure as a trade secret. In addition, it is paramount that
one uses teleostan fish gelatin as a stabilizer instead of BSA. Amersham
also sells a immunogold quality teleostan fish gelatin. (Reference:
Birrel, et al, "Pitfalls of Immunogold Labeling," Journal of Histo. &
Cyto., 35(8): 843-53 (1987). I have no interest in any of these companies,
except as a consumer.

At 10:09 AM 6/9/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 13:54:39 2004

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When labeling e.g. lowicryl sections using indirect immunogold (primary
antibody - secondary antibody conjugated to gold), is there a consensus
for the typical (or maximal, that may be easier) distance between the
antigen and the particle? I do understand this will never be a discrete
number, I would like to have an idea what people think.

Thanks,

Michael Jarnik

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 9 16:13:09 2004

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Hello Jim
Leica used to utilize this principle in their knifemaker (which is actually
originated from LKB). The idea is that you made squares not from the end
of strip (as in LKB), but cutting glass strip in half every time until you
got perfect squares. Leica has sort of rail with stops for the glass
strip. The position of stops are: half of the glass strip length, 1/4, 1/8
and so on. Last stop is at the length for square. I could assume
somebody made similar device for old LKB knifemaker. I don't think it
would convert your old knifemaker into brand new machine: quality of knifes
depends not only from way of glass breaking but from preciseness of
mechanics. Old machine would not perform like new even breaking glass in
new way. From another hand, it'll definitely improved the quality of the
knifes. I have to tell you (no financial interest) Leica's knifemaker made
fantastic knifes even with 10 mm glass. I used to use glass knifes for
teaching purpose and diamond for science. Sergey

At 11:49 AM 6/9/2004 +0200, you wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 06:33:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (viviana.torres-at-gmail.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Wednesday, June 9, 2004 at 18:56:28
---------------------------------------------------------------------------

Email: viviana.torres-at-gmail.com
Name: Viviana Torres

Organization: Stanford

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello,

I need to do EM analysis of microsomal pellets obtained from rat brain.

My main problem is how to keep the pellets in the eppendorf tube
during the whole EM processing

I will appreciate if someone with experience on these kind of samples
can provide me a protocol

regards

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 06:32:57 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (pblanken-at-wisc.edu) from
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Wednesday, June 9, 2004 at 16:01:04
---------------------------------------------------------------------------

Email: pblanken-at-wisc.edu
Name: Peter Blankenheim

Organization: Madison Area Technical College

Title-Subject: [Microscopy] [Filtered] Savannah Share Trip

Question: I'm driving to the Savannah Convention from Madison Wi, and
I'm looking for someone to share the car, possibly driving, and
possibly lodging. 50 yr old male.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 08:40:01 2004

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Many people will probably respond to your query. Whenever I fix small numbers
of cells, etc., the easiest method is to spin them down in 2% agar (after
fixation, even through the Osmium stage)in small eppendorf tubes. You then can
remove the agar from the tube, cut off the tip with the cells, whatever, and
continue to process like a piece of tissue. Avoids constant centrifugation and
loss of material with each spin.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: viviana.torres-at-gmail.com [mailto:viviana.torres-at-gmail.com]
Sent: Thursday, June 10, 2004 8:00 AM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (viviana.torres-at-gmail.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Wednesday, June 9, 2004 at 18:56:28
---------------------------------------------------------------------------

Email: viviana.torres-at-gmail.com
Name: Viviana Torres

Organization: Stanford

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello,

I need to do EM analysis of microsomal pellets obtained from rat brain.

My main problem is how to keep the pellets in the eppendorf tube
during the whole EM processing

I will appreciate if someone with experience on these kind of samples
can provide me a protocol

regards

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 09:01:33 2004

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Michael:

I have a an excellent book entitled "Electron Microscopic
Immuncytochemistry" edited by Julia Polak and John Priestley, Oxford
University Press, 1991. They state on page 74 of Chapter 3 entitled
"Post-embedding Electron Microscopic Immunocytochemistry":

"The minimum theorectical lateral resolution (i.e. distance between the
centre of the gold particle and the epitope recognized by the primary
antibody) that can be achieved with the protein-A gold technique is about 16
nm, using a colloidal gold particle of 3 nm. Using the immunoglobulin-gold
technique with a gold particle of 10 nm the lateral resolution is
approximately 21 nm. It is clear that the bigger the gold particle, the
less satisfactory is the lateral resolution of the technique."

Hope this answers your question.

Karen Bentley

Karen L. Bentley, M.S.
Associate Scientist & Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 12:48:58 2004

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Hi Karen,

The statment in the Polak & Priestley book makes an assumption that when the specimen is dried, the antibodies and gold probe fall to one side (presumably in a random direction).

As there is no evidence to support the statement, other than it was published in a book, may I propose the possibility that the gold particles have an equally good chance (or better) of drying on top of the antibodies. This would mean that the lateral resolution in practice is much better than predicted by what is expected theoretically. The resolution in three dimensions may not be so good in that the gold will end up above the antigen but this should not concern us when we examine the sections in the TEM

The theoretical resolution predicted in the Polak and Priestley book, assumes the gold particles will be bound to the far end of the antibody molecule, when in fact the particles are more likely to bind closer to the hinge region (Baschong & Wrigley 1989 small colloidal gold conjugated to FAB fragments or to immunoglobulin G as high resolution labels for electron microscopy. A technical overview. J. Electron Microsc. Tech. 14:313-323), thus reducing the theorectical resolution predicted by Polak & Priestley.

Anyone who performs immuno-EM on a routine basis will tell you that gold particles are very often much closer to the antigen site than could be expected if the gold was "falling off the pile of protein". Quite often the gold is located in precisely the location predicted.

A good demonstration of how precise immunolabeling can be is seen in the study by Sodeik et al (1997 Microtuble-mediated transport of incoming Herpes simplex virus 1 capsids to the nucleus. J. Cell Biol 136:1007-1021). An antibody to dynein (which attaches the capsid to microtubules) labels exactly 40 - 50 nm away from the virus, where the antigen is predicted to be. If the immunolabeling were to be as poor resolution as predicted by theorectical considerations, the technicnique could not be used for such high resolution studies as it has been applied.

Obviously we need more experimentation, and thus more data, to continue this discussion and to provide Michael with the answer he wants.

Regards,

Paul Webster.

Paul Webster, Ph.D.
House Ear Institute
2100 West Third Street
Los Angeles
CA 90057
phone (213) 273 8026
fax (213) 413 6739
email: pwebster-at-hei.org

} ----------
} From: Bentley, Karen
} Sent: Thursday, June 10, 2004 7:20 AM
} To: 'microscopy-at-msa.microscopy.com'
} Subject: [Microscopy] Gold Distance from Antigen
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Michael:
}
} I have a an excellent book entitled "Electron Microscopic
} Immuncytochemistry" edited by Julia Polak and John Priestley, Oxford
} University Press, 1991. They state on page 74 of Chapter 3 entitled
} "Post-embedding Electron Microscopic Immunocytochemistry":
}
} "The minimum theorectical lateral resolution (i.e. distance between the
} centre of the gold particle and the epitope recognized by the primary
} antibody) that can be achieved with the protein-A gold technique is about 16
} nm, using a colloidal gold particle of 3 nm. Using the immunoglobulin-gold
} technique with a gold particle of 10 nm the lateral resolution is
} approximately 21 nm. It is clear that the bigger the gold particle, the
} less satisfactory is the lateral resolution of the technique."
}
} Hope this answers your question.
}
} Karen Bentley
}
} Karen L. Bentley, M.S.
} Associate Scientist & Manager}
} Electron Microscope Research Core
} University of Rochester Medical Center
} Rochester, NY 14642
} 585-275-1954
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 16:12:30 2004

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Does anyone know if special precautions are required before inserting a
high-tension cable back into the oil tank of a TEM. We have a TEM that
was shipped with the transformer separate from the instrument. I want
to finish installing the instrument, but wanted to inquire as to
whether there were any special precautions to follow.
Thanks in advance,
Robert

Dr. Robert Kyle Pope
Indiana University South Bend
Department of Biology
1700 Mishawaka Avenue
South Bend, IN 46615-1408
Email: ropope-at-iusb.edu
Fax: 574-237-6589
Tele: 574-237-4411

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 16:57:34 2004

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Roth (1982 The protein A-gold technique..... pp 107-133 in Techniques in
Immunocytochemistry vol. 1, eds GR Bullock and P Perutz) also discusses size
of antibodies, and estimates that they are about 8 nm in diameter. So if
both primary and secondary antibodies are lying flat on your section,
there's a maximum ~16 nm between antigen and gold particle.

As Paul notes, this is a maximum distance, the gold can be stacked directly
on top of the antigen. In immunoFESEM work on microtubules, for example
(Vesk et al. 1994 Imaging of plant microtubules with high resolution
scanning electron microscopy. Protoplasma 182: 71-74), using primary
anti-tubulin and gold-labelled secondary, you see a single or occasionally a
double blob on the microtubule with the gold on top. The tissue has been
dried, of course, so I guess the antibodies and gold are more likely to
appear this way.
cheers,
Rosemary

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

} From: "Webster, Paul" {PWebster-at-hei.org}
} Date: Thu, 10 Jun 2004 11:09:55 -0700
} To: "MSA listserver submission (E-mail)" {Microscopy-at-MSA.Microscopy.Com}
} Subject: [Microscopy] RE: Gold Distance from Antigen
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Hi Karen,
}
} The statment in the Polak & Priestley book makes an assumption that when the
} specimen is dried, the antibodies and gold probe fall to one side (presumably
} in a random direction).
}
} As there is no evidence to support the statement, other than it was published
} in a book, may I propose the possibility that the gold particles have an
} equally good chance (or better) of drying on top of the antibodies. This would
} mean that the lateral resolution in practice is much better than predicted by
} what is expected theoretically. The resolution in three dimensions may not be
} so good in that the gold will end up above the antigen but this should not
} concern us when we examine the sections in the TEM
}
} The theoretical resolution predicted in the Polak and Priestley book, assumes
} the gold particles will be bound to the far end of the antibody molecule, when
} in fact the particles are more likely to bind closer to the hinge region
} (Baschong & Wrigley 1989 small colloidal gold conjugated to FAB fragments or
} to immunoglobulin G as high resolution labels for electron microscopy. A
} technical overview. J. Electron Microsc. Tech. 14:313-323), thus reducing the
} theorectical resolution predicted by Polak & Priestley.
}
} Anyone who performs immuno-EM on a routine basis will tell you that gold
} particles are very often much closer to the antigen site than could be
} expected if the gold was "falling off the pile of protein". Quite often the
} gold is located in precisely the location predicted.
}
} A good demonstration of how precise immunolabeling can be is seen in the study
} by Sodeik et al (1997 Microtuble-mediated transport of incoming Herpes simplex
} virus 1 capsids to the nucleus. J. Cell Biol 136:1007-1021). An antibody to
} dynein (which attaches the capsid to microtubules) labels exactly 40 - 50 nm
} away from the virus, where the antigen is predicted to be. If the
} immunolabeling were to be as poor resolution as predicted by theorectical
} considerations, the technicnique could not be used for such high resolution
} studies as it has been applied.
}
} Obviously we need more experimentation, and thus more data, to continue this
} discussion and to provide Michael with the answer he wants.
}
} Regards,
}
} Paul Webster.
}
}
}
}
}
}
}
} Paul Webster, Ph.D.
} House Ear Institute
} 2100 West Third Street
} Los Angeles
} CA 90057
} phone (213) 273 8026
} fax (213) 413 6739
} email: pwebster-at-hei.org
}
}
} } ----------
} } From: Bentley, Karen
} } Sent: Thursday, June 10, 2004 7:20 AM
} } To: 'microscopy-at-msa.microscopy.com'
} } Subject: [Microscopy] Gold Distance from Antigen
} }
} }
} }
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } Michael:
} }
} } I have a an excellent book entitled "Electron Microscopic
} } Immuncytochemistry" edited by Julia Polak and John Priestley, Oxford
} } University Press, 1991. They state on page 74 of Chapter 3 entitled
} } "Post-embedding Electron Microscopic Immunocytochemistry":
} }
} } "The minimum theorectical lateral resolution (i.e. distance between the
} } centre of the gold particle and the epitope recognized by the primary
} } antibody) that can be achieved with the protein-A gold technique is about 16
} } nm, using a colloidal gold particle of 3 nm. Using the immunoglobulin-gold
} } technique with a gold particle of 10 nm the lateral resolution is
} } approximately 21 nm. It is clear that the bigger the gold particle, the
} } less satisfactory is the lateral resolution of the technique."
} }
} } Hope this answers your question.
} }
} } Karen Bentley
} }
} } Karen L. Bentley, M.S.
} } Associate Scientist & Manager}
} } Electron Microscope Research Core
} } University of Rochester Medical Center
} } Rochester, NY 14642
} } 585-275-1954
} }
} }
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 10 17:37:42 2004

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Dear Colleagues

} } } } } Imaging and Microscopy CD-ROM (Vol 2) { { { { {

This message invites you to contribute to the next on a series of CD-ROM
published by our laboratory. To date, we have distributed over 50,000
copies of 9 CD-ROMs --- 8 in cytometry and 1 in imaging and microscopy.
The second volume of our imaging and microscopy CD-ROM with 5000 copy
distribution is imminent. We have 2-3 weeks to complete this next
electronic publication. You may see the others at
http://www.cyto.purdue.edu/flowcyt/cdroms/newcd6.htm

We invite you contribute your unpublished materials - images, movies,
protocols, lectures, etc. You retain all copyrights to all materials
published. This is an opportunity to publish quality materials in a
well recognized series of CD-ROMs that will receive worldwide distribution.

This particular CD-ROM will be distributed initially at the MSA meeting
in Savannah, and then at a number of meetings around the world. As with
all of the Purdue CD-ROMs, it is free to those attending meetings, or if
obtained from one of the sponsoring companies. The disc is produced by
our staff at Purdue University Cytometry Laboratories and is done so as
part of our "Cytomics Initiatives in Education" program.

You may contribute an entire section on your work, a small section
describing an image or series of images, animations or videos or other
materials. Book reviews, manual evaluations, protocols, technical
support information, software routines, macros and instrument setup
materials are welcome and useful. You must verify that you own the
copyright by submitting the form at

http://tinyurl.com/3bmgn

and provide permission to us to place this material onto the CD-ROM. You
retain all ownership rights. If the materials are already published, you
may require permission of the publisher to place the materials onto this
CD-ROM by using the form which is found at

http://tinyurl.com/2sw6o

All of the above information is somewhere on our website starting here
http://www.cyto.purdue.edu/flowcyt/cdroms/newcd6.htm

Time is short, but this means that the materials published are very
recent. You have 21 days left to contribute!!

You may submit materials directly to us at cd2-at-flowcyt.cyto.purdue.edu
or to my personal email address. Instructions for FTP of large files are
on the webpage above.

If you are a company and wish to participate in sponsorship which is
still available, please contact us directly.

Kind Regards

J. Paul Robinson & Bartek Rajwa
Purdue University Cytometry Laboratories

------------------
J.Paul Robinson, PhD
Professor of Immunopharmacology
Professor of Biomedical Engineering

Bartlomiej Rajwa, PhD
Purdue University Cytometry Laboratories
Hansen Research Bld, B050
West Lafayette, 47907 IN
tel. (765) 494 0757

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 02:02:52 2004

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Hi

Lets see if I can help? I assume this is an oil filled tank, its heavy?

Keep the air in the room as still as possible and make sure that there is
the minimum amount of dust in the air. Make sure the cable end is absolutely
clean and clean round the top of the high voltage tank before opening the
tank itself. Use a cleaning media/cloth that does not leave a dust behind.
Some instruments have an insulating grease on the connection, these cables
have a taper fit.

The cable end will probably have a locating pin so that it only fits in one
position. Gently lower it into place and try to feel it settling in the
contact area, do not force it!

Once in place clamp or bolt it down and you are ready to go! Run the high
voltage up slowly to give time for any trapped air to be flushed out.

Good luck

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0)7711 606967
www.emcourses.com

----- Original Message -----
} From: "Dr. Robert K. Pope" {ropope-at-iusb.edu}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, June 10, 2004 10:30 PM

Hi Listers,

I just wanted to thank all who replied to my question with a nod of my head
;-).

I was trying all the suggestions and nothing was working. I left the bits
alone for a night came back put all the screws and widgets back together.
Withthe exception of putting the tightening screw on the top instead of the
bottom all was the same--except this time it worked.

Now I can go back and thick section Wah, oh, I mean Yippee!

Thanks again all!

No more nodding off in Norolk,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 10:25:31 2004

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We are trying to label silica particles with rhodamine B-ITC. The
first time we tried using a standard bead labeling protocol it seemed
to work, but now we can't repeat it. The thing I find wierd is that
the pellet of particles is clearly pink by eye, so I would think that
would mean they are labeled. Yet in the microscope, very few are
fluorescent. I suppose it could be the small number of labeled ones
generating the color, but I wondered if anyone had any alternative
ideas as to why they might not look fluorescent even though colored.
Thanks- Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 10:43:30 2004

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List,

My lab is looking into purchasing a new coater for our FESEM sample
preparation. We have been extremely satisfied with our current system, a
BOC Edwards Xenosput (Dynavac), for Pt coating. Unfortunately Edwards no
longer sells this particular technology. At present we are considering an
Osmium coater or Ion beam system. I would appreciate frank opinions from
experienced users of these, or other, viable candidates for this type of
coating. Specifically, we are interested in sample through put, routine
maintenance, overall reliability, cost of consumables, limitations on sample
size and ease of use. Thanks in advance, jr

FYI Generally speaking we operate at {2kv and magnifications up to ~150K.

John A. Robson
Boehringer Ingelheim Pharmaceuticals, Inc.
PO Box 368
900 Ridgebury Rd
Ridgefield, CT 06877

Phone (203)798-5640
Fax (203)798-5698
e-mail jrobson-at-RDG.boehringer-ingelheim.com

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 12:03:27 2004

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Colleagues,

BAL-TEC AG and Boeckeler Instruments / RMC Products, Inc. Cordially invite you to the First U.S. Users' Group Meeting for High Pressure Freezing during the M&M Meeting in Savannah, Georgia. Current users and potential users are invited to the meeting.

When: Sunday, August 1, 2004, 12:00 noon - 5:00 pm.

Where: Grand Ballroom F, Westin Savannah Harbor Golf Resort and Spa, Savannah, Georgia.

A buffet lunch will be provided.

Presenters are being invited from current users of the HPM 010 High Pressure Freezer.

Attendance is limited to 50 persons, so please RSVP at your earliest convenience.

If you have questions, wish to RSVP, or have already made travel arrangements, please contact Boeckeler Instruments for assistance at 800.552.2262 or 502.745.0001 and ask for Ms. Kim Megaw. You can also e-mail Kim at { {kim-at-boeckeler.com} } .

Thank you. We look forward to seeing you in Savannah!

Bob Chiovetti, Ph.D.
Senior Product Specialist
RMC Products
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 13:09:46 2004

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Hello,

We have been experiencing a problem using Aclar for
flatembedding lately: After polimerization, it is very
difficult to peel it off the tissue. Often it rips out
pieces of tissue as it comes off. This problem started when
we opened a new order from EMS, while samples with the old
Aclar batch (and processed parallelly with the new batch),
worked fine. We tried new orders from EMS and Ted Pella...
without much improvement. Aclar also feels more rigid and
thicker than we used in the past, even though it is the
same catalog number and thickness. We use EMbed 812,
polimerized for 1-2 days at 60 degrees C.

Has anybody experienced a similar problem? Can you
recommend alternative material for flatembedding?

Alev

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Alev Erisir
University of Virginia
Department of Psychology
102 Gilmer Hall, PO Box 400400
Charlottesville, VA 22904-4400

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 14:26:41 2004

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We're making metal plates to raise the Olympus IX71 microscope stage by
12mm to accommodate a piezo focusing device.

Does anybody know the screw size for holding the stage in place so that we
can order the appropriate replacement screws?

Thanks.
____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 15:38:24 2004

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We need to put an extension ring 12 mm high between the objective and the
nosepiece.

Does anybody out there have such rings or know where we could purchase them?

An alternative would be to have the machine shop here make a few. Would
somebody please post the thread size in case we have to do this.

Thanks!

____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 11 16:28:13 2004

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On Jun 11, 2004, at 8:44 AM, David Knecht wrote:

} We are trying to label silica particles with rhodamine B-ITC. The
} first time we tried using a standard bead labeling protocol it seemed
} to work, but now we can't repeat it. The thing I find wierd is that
} the pellet of particles is clearly pink by eye, so I would think that
} would mean they are labeled. Yet in the microscope, very few are
} fluorescent. I suppose it could be the small number of labeled ones
} generating the color, but I wondered if anyone had any alternative
} ideas as to why they might not look fluorescent even though colored.
} Thanks-

Dear David,
Are you sure that all the particles have exactly the same composition?
One reason that a dye can absorb light--to generate color--but not
fluoresce is if there are non-radiative decay processes, which in
general are strongly affected by the environment of the dye. So the
dye molecules could be bound to some of the particles in one way, where
they fluoresce, and in another way on others of the particles (if some
particles have a different surface environment, for example) where they
do not. In either case, there would likely be absorption of light,
although the spectrum could be shifted, so the particles would appear
colored. Not only is this possible if there are two different
compositions, surface treatments, etc. for the particles, but some
subtle effects where different crystal faces predominate on the
surfaces of some of the particles will also affect fluorescence. I
have had no experience either with rhodomine B-ITC or silica particles,
so if the real experts disagree, go with their advice.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 13 00:30:03 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Alev Erisir wrote:
============================================================================
============
We have been experiencing a problem using Aclar for flatembedding lately:
After polimerization, it is very difficult to peel it off the tissue. Often
it rips out pieces of tissue as it comes off. This problem started when we
opened a new order from EMS, while samples with the old Aclar batch (and
processed parallelly with the new batch), worked fine. We tried new orders
from EMS and Ted Pella... without much improvement. Aclar also feels more
rigid and thicker than we used in the past, even though it is the same
catalog number and thickness. We use EMbed 812, polimerized for 1-2 days at
60 degrees C.

Has anybody experienced a similar problem? Can you recommend alternative
material for flatembedding?
============================================================================
=============
We have offered Aclar film, specifically Aclar 33c, since it seemed to be
the one with the most attractive properties for applications in microscopy
and histology. It is not "sticky" either before or after resin curing. See
URL
http://www.2spi.com/catalog/photo/aclar-film.shtml for additional
information.

Chuck

============================================

Charles A. Garber, Ph. D. Ph: 1-610-436-5400
President 1-800-2424-SPI
SPI SUPPLIES FAX: 1-610-436-5755
PO BOX 656 e-mail:cgarber-at-2spi.com
West Chester, PA 19381-0656 USA
Cust.Service: spi2spi-at-2spi.com

Look for us!
########################
WWW: http://www.2spi.com
########################
============================================

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 13 10:07:02 2004

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The 30th Annual Nikon 2004 Small World Photomicrography Competition

Celebrating its 30th year, the annual Nikon International Small World Competition was founded in 1975 to recognize excellence in photography through the microscope. The competition's reputation has grown throughout the years and is regarded as the leading forum for recognizing the beauty and complexity of life as seen through the light microscope. The 2004 deadline for entries is Wednesday June 30, 2004.

Astonishing displays of color and remarkable subject matter are among the highlights in the annual Nikon International Small World Photomicrography contest. These award-winning photographs merge the techniques of scientific inquiry with aesthetic beauty to create vibrant and dynamic images reflective of the intriguing world of microscopy. Hailed as the worldâ€™s leading forum for photographic excellence in the art and science of photomicrography, images submitted to the contest capture the mysterious and often unseen universe viewed through a light microscope.

Microscopists from all areas are encouraged to enter the contest and can upload their images from www.nikonsmallworld.com . Submissions may include up to three 35mm photographs or digital images of any subject matter viewed using a light microscopy technique. The first and second of twenty prizewinners receive a selection of Nikon products and equipment worth $3,000 and $2,000 respectively. Use of a Nikon microscope or camera is not required. Participants can enter online by uploading their images or sending in 35mm transparencies to Nikon's headquarters in Melville, New York.

The deadline for entries is June 30, 2004.

For complete contest information and to enter online, go to
www.nikonsmallworld.com . You can also call Nikon at 631-547-8569.

} From Stan at Nikon

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 13 20:19:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (charles-at-3dcircuits.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, June 11, 2004 at 12:51:05
---------------------------------------------------------------------------

Email: charles-at-3dcircuits.com
Name: charles

Title-Subject: [Microscopy] [Filtered] MListserver: EDX Restoring Image Calibration File for Noran Voyager V3.7

Question: We are attempting to restore the "image calibration file" on a Noran Voyager (V3.7 software). The loss of this file occurred after the Voyager 3.7 software was installed (from scratch) on a new computer. We do not have a backup or copy of this file, however, we do have a printout of the calibration constants from the previous setup. According to Thermo, this file is entitled "wima.column1.cal", and cannot be easily "created" except by the field engineer. Does anyone know how to create this file, or could a correct calibration file be created with a "template" and filling in the calibration constants that we have in hardcopy.

Thanks for any suggestions.
Charles

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 13 23:51:58 2004

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Hi All

I have a cressington turbo 208 carbon coater with the metal evaporator
accessory.

I use it regularly for carbon coating, but am only just starting to use
it for metal coating.

I would like to use gold wire, but am not sure how thick the wire should
be, or the length of gold wire I require to obtain a suitable coat.

I have tried using 4cm of 0.25mm gold wire for 20 seconds at 20mA, but
am not seeing a 'charge-free' coat. (I don't want to coat too thickly
but am not sure how much gold per sample I should be using.)

Can anyone give me some ideas? Does anyone who has this coater already
have some settings I could try?

thanks

Samantha Taylor
TDG Experimental Officer
Alcoa World Alumina
XRD, Microscopy and Thermal Analysis
Phone:(08) 9410 3588
Fax: (08) 9410 3167
Email: Samantha.Taylor-at-Alcoa.com.au

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 05:51:52 2004

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Colleagues...

The Ask-the-Experts session at the M&M 2004 meeting in Savannah takes on a different format this year to provide programming closer to the time of the annual Microscopy and Microanalysis (M&M) meeting, and to better address the needs of the meeting attendees.

Rather than listing topics in the Call for Papers, which must be produced nearly a year before the meeting, an on-line Form is now available for you to suggest topics for this informal session.

You can find a link to this form in the News section of the Meeting Home Page. :

http://mm2004.microscopy.org

This link will allow meeting participants to submit questions, and/or as appropriate suggest name(s) of experts to whom the question might be directed.

The Ask-the- Experts organizers will then seek to schedule a time to address topics of significant interest during the meeting.

The schedule of topics will be announced and posted to the meeting website a couple of weeks before the early registration deadline, so that potential M&M 2004 attendees can schedule in the topics of interest to them. Please plan to participate both in the topic selection and the sessions, so that we can gauge whether this change of format is beneficial!

Ask-The-Experts Organizers.

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 07:39:27 2004

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Our SEM (JEOL 6360 LV w/tungsten filament) is likely being relocated along
with the rest of our lab to a second-floor location (the room is on a
concrete slab) in the general vicinity of a mainframe computer, an
elevator, a men's room and a large outside air conditioning unit. I have
asked to give an expert opinion on the feasibility of this move from a
noise (electromagnetic and vibration) standpoint. The proposed room is ~
40 feet from the mainframe (as the crow flies, across the hall with
multiple walls in between), ~ 40 feet from the elevator (same side of the
hallway, four walls between), next door to the men's room (but the stalls
are on the opposite wall) and ~ 20 feet from the outside A/C unit. The
scope is on a JEOL-supplied air table, and I typically image at less than
5,000x magnification (usually no higher than 1,000x). My samples are
predominantly organic in nature (cloths, polymers, hair).

I have proposed to have the room assessed for the various types of noise
(~$3,500), but have been greeted with resistance by management, who
expected about $300 (and have no expertise in microscopy). So I ask those
on the ListServer who have encounted a similar noise concern for an SEM
lab relocation, should I expect to have issues with electromagnetic or
vibrational noise due to any of the mainframe, elevator, men's room or A/C
unit (or even second-floor on concrete location)?

I thank you in advance for any assistance.

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 09:06:31 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Once upon a time our sem was moved to a second floor location adjacent to
the MTS Lab (fatigue/tensile testing lab). That lasted a month of so before
management was convinced that the system was nearly useless in the new
location. Images had the "jiggles" at a few thousand x and higher. The lab
was re-relocated back.

You can take your chances or measure the environmental conditions. You
*may* have sufficient EMI isolation, given the distances. Vibration
isolation is very dependent on the building construction and source levels
and more difficult to guess/estimate.

} From your description, there are no high current wiring or switchboxes
nearby. I would be most concerned about mechanical vibrations with EMI
concerns secondary.

The question is: How expensive is a vibration survey vs. moving the sem and
finding it will not do your work?

Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Brian.Kirkmeyer-at-iff.com [mailto:Brian.Kirkmeyer-at-iff.com]
Sent: Monday, June 14, 2004 9:04 AM
To: Microscopy-at-MSA.Microscopy.Com

Our SEM (JEOL 6360 LV w/tungsten filament) is likely being relocated along
with the rest of our lab to a second-floor location (the room is on a
concrete slab) in the general vicinity of a mainframe computer, an
elevator, a men's room and a large outside air conditioning unit. I have
asked to give an expert opinion on the feasibility of this move from a
noise (electromagnetic and vibration) standpoint. The proposed room is ~
40 feet from the mainframe (as the crow flies, across the hall with
multiple walls in between), ~ 40 feet from the elevator (same side of the
hallway, four walls between), next door to the men's room (but the stalls
are on the opposite wall) and ~ 20 feet from the outside A/C unit. The
scope is on a JEOL-supplied air table, and I typically image at less than
5,000x magnification (usually no higher than 1,000x). My samples are
predominantly organic in nature (cloths, polymers, hair).

I have proposed to have the room assessed for the various types of noise
(~$3,500), but have been greeted with resistance by management, who
expected about $300 (and have no expertise in microscopy). So I ask those
on the ListServer who have encounted a similar noise concern for an SEM
lab relocation, should I expect to have issues with electromagnetic or
vibrational noise due to any of the mainframe, elevator, men's room or A/C
unit (or even second-floor on concrete location)?

I thank you in advance for any assistance.

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 10:00:54 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have a 305FE Schottky field emitter gun
that is decommissioned. It is eight months
old and was working fine when pulled off.
I'm toying with the idea of documenting
the reverse engineering of this gun, unless
someone can make good use of it. I also
have the separate FE support box that contains
the ion pump power supplies. This is probably
just useful as a boat anchor.

It seems interesting to see what is inside
a current production thermal FE gun. There
would be pix and dimensions on my Web site
if I do this.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 10:34:00 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I am writing today to try and answer a question with the help of
knowledgeable experts in the field of microscopy. I am a MBA graduate
student here at Texas A&M University working with them in collaboration
and development of new and existing patents. Recently, I was tasked
with trying to determine whether there is currently in the market a
device which can measure the forces BETWEEN cells in the pico newton
range. From the responses of industry and academic contacts so far it
is evident that there are quite a number of companies which can measure
the forces between cells and OTHER objects such as those to measure cell
adhesion and cell surface tension by way of optical tweezers and AFM's.
I have also found many devices (such as those from Cell Robotics) which
can easily manipulate or surgically cut away portions of cellular
material. But I have as of yet found no device which is used for the
explicit measurement of forces between cells in the tens of pico
newtons.

I really wish that I could be more specific in my explanation of what
it the customer is seeking. It is my belief that because of possible
patent disclosure I am not allowed to have a wider scope for the
intended use of this device.

I would gladly welcome any responses through either the list server or
to the phone number below at NASA. Please remember that I am not an
expert in the field of microscopy and therefore simplicity in
explanation is requested because of my ignorance. Thank you in advance
for taking the time to read this and respond. Gig 'em!

Ryan M Lee
NASA Technology Transfer Center
Texas Engineering Extension System
Texas A&M University System
979-862-8603

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 13:11:29 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi, all,

The 2 small fluorescent tubes, which are situated just above where the knife and boat sit, both "blew" last week. The person using the ultramicrotome at the time told me that the bulbs were no longer working. I installed 2 new tubes today, and still can't get overhead illumination. I am now suspecting a blown fuse might be the cause, but I don't know where to look for this fuse - there is not much explanation in the manual about these overhead lights.

Could anyone please point me in the right direction?

Thanks in advance for any help.

Regards,

Paula.

Paula M. Allan-Wojtas
Research Scientist - Food Microstructure/chercheur scientique - microstructure des aliments
Food Safety and Quality team/ Salubrité et qualité des aliments
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 902-679-5566
Facsimile/Télécopieur: 902-679-2311
32 Main Street/ 32, rue Main
Kentville, Nova Scotia/ Kentville (Nouvelle-Écosse)
B4N 1J5

allanwojtasp-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 13:11:07 2004

Contents Retrieved from Microscopy Listserver Archives
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Does anyone out there have the service manual/circuit diagrams for a
Cambridge Stereoscan 90 SEM, or can you tell me where I can purchase them?
I'd also just like to know who else has this microscope. I have some spares
(e.g., turbo pump, camera system) available for barter. I also have
documentation for a Stereoscan 150 if anybody wants it.

Paul Grover
Dept. of Biological Sciences
Purdue University

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 13:33:55 2004

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Woody,
Last year I moved one FESEM and three TEMs into a new lab. I did the site
check with a $200 EMF meter/probe, available from several vendors on-line,
and about 20mls of clean mercury in a well sealed 60ml poly bottle (wider
is better). The required EMF meter readings are available in the equipment
installation manual. I placed the bottle of mercury on the floor where the
EM was to go, removed the cap (very carefully) and peeked down through the
bottle neck at the surface of the liquid. With no vibrations I would see a
smooth mirror. If rings are visible in the mercury's surface than the floor
is vibrating. Low EMF and no 'jiggles' here. All of my scopes are running
at spec.

Disclaimer:
I am not responsible for your results or any mercury spills due to operator
error. There are many variables to consider. Vibrations may vary over the
course of time (trains, intermittent local equipment operation). Audio
noise and air flow patterns can not be detected using the above methods.

Good luck.
Jim

} From: "White, Woody N." {nwwhite-at-bwxt.com}
} To: "'Brian.Kirkmeyer-at-iff.com'" {Brian.Kirkmeyer-at-iff.com} ,
} Microscopy-at-msa.microscopy.com
} Subject: [Microscopy] RE: SEM site assessment
} Date: Mon, 14 Jun 2004 09:25:42 -0500
} MIME-Version: 1.0
} X-UConn-MailScanner-Information: Contact UConn Help Desk 860-486-4357 for
} more information.
} X-UConn-MailScanner: Found to be clean
} X-UConn-MailScanner-SpamCheck:
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

James S. Romanow
The University of Connecticut
Physiology and Neurobiology Department
Electron Microscopy Facility
Unit 3242
BSP Building, Room G06
91 North Eagleville Road
Storrs, CT 06269-3242

860 486-2914 voice
860 486-6369 fax
james.romanow-at-uconn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 14:09:58 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Kirk,
Last year I moved one FESEM and three TEMs into a new lab. I did the site
check with a $200 EMF meter/probe, available from several vendors on-line,
and about 20mls of clean mercury in a well sealed 60ml poly bottle (wider
is better). The required EMF meter readings are available in the equipment
installation manual. I placed the bottle of mercury on the floor where the
EM was to go, removed the cap (very carefully) and peeked down through the
bottle neck at the surface of the liquid. With no vibrations I would see a
smooth mirror. If rings are visible in the mercury's surface than the floor
is vibrating. Low EMF and no 'jiggles' here. All of my scopes are running
at spec.

Disclaimer:
I am not responsible for your results or any mercury spills due to operator
error.

Good luck.
Jim

} From: "White, Woody N." {nwwhite-at-bwxt.com}
} To: "'Brian.Kirkmeyer-at-iff.com'" {Brian.Kirkmeyer-at-iff.com} ,
} Microscopy-at-msa.microscopy.com
} Subject: [Microscopy] RE: SEM site assessment
} Date: Mon, 14 Jun 2004 09:25:42 -0500
} MIME-Version: 1.0
} X-UConn-MailScanner-Information: Contact UConn Help Desk 860-486-4357 for
} more information.
} X-UConn-MailScanner: Found to be clean
} X-UConn-MailScanner-SpamCheck:
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

James S. Romanow
The University of Connecticut
Physiology and Neurobiology Department
Electron Microscopy Facility
Unit 3242
BSP Building, Room G06
91 North Eagleville Road
Storrs, CT 06269-3242

860 486-2914 voice
860 486-6369 fax
james.romanow-at-uconn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 14:16:51 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Listees,

We're loosing our Hitachi 3500 SEM due to a split in the EM facility here
at Clemson University. Is there anything out there available, comparable
on a used basis. We're looking for equipment and a price. Thanks in
advance for any information.

Darryl Krueger, RA
BioScience Dept.
Clemson University

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 15:39:17 2004

Contents Retrieved from Microscopy Listserver Archives
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For cheap vibration detection, I've used a large (40 cm diameter) dish of
water, placed on whatever surface you're testing, no a/c on, turn overhead
lights off, shine a lamp onto the water surface at a low angle from the side
while standing perfectly still and observe the reflections on adjacent wall
- this is quite sensitive - can pick up vibrations from folk walking down
the hall outside. But perhaps a denser liquid, like mercury, picks up a
different vibration spectrum, or responds differently?

I used this demonstration to get a proper anti-vibration table for one of
our light microscopes....

cheers,
Rosemary

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

} From: Jim Romanow {bsgphy3-at-uconnvm.uconn.edu}
} Date: Mon, 14 Jun 2004 14:55:49 -0400
} To: microscopy-at-SPARC5.microscopy.com
} Subject: [Microscopy] RE: SEM site assessment
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Woody,
} Last year I moved one FESEM and three TEMs into a new lab. I did the site
} check with a $200 EMF meter/probe, available from several vendors on-line,
} and about 20mls of clean mercury in a well sealed 60ml poly bottle (wider
} is better). The required EMF meter readings are available in the equipment
} installation manual. I placed the bottle of mercury on the floor where the
} EM was to go, removed the cap (very carefully) and peeked down through the
} bottle neck at the surface of the liquid. With no vibrations I would see a
} smooth mirror. If rings are visible in the mercury's surface than the floor
} is vibrating. Low EMF and no 'jiggles' here. All of my scopes are running
} at spec.
}
} Disclaimer:
} I am not responsible for your results or any mercury spills due to operator
} error. There are many variables to consider. Vibrations may vary over the
} course of time (trains, intermittent local equipment operation). Audio
} noise and air flow patterns can not be detected using the above methods.
}
} Good luck.
} Jim
}
}
}
} } From: "White, Woody N." {nwwhite-at-bwxt.com}
} } To: "'Brian.Kirkmeyer-at-iff.com'" {Brian.Kirkmeyer-at-iff.com} ,
} } Microscopy-at-msa.microscopy.com
} } Subject: [Microscopy] RE: SEM site assessment
} } Date: Mon, 14 Jun 2004 09:25:42 -0500
} } MIME-Version: 1.0
} } X-UConn-MailScanner-Information: Contact UConn Help Desk 860-486-4357 for
} } more information.
} } X-UConn-MailScanner: Found to be clean
} } X-UConn-MailScanner-SpamCheck:
} }
} }
} }
} }
-----------------------------------------------------------------------------} }
-
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } Once upon a time our sem was moved to a second floor location adjacent to
} } the MTS Lab (fatigue/tensile testing lab). That lasted a month of so before
} } management was convinced that the system was nearly useless in the new
} } location. Images had the "jiggles" at a few thousand x and higher. The lab
} } was re-relocated back.
} }
} } You can take your chances or measure the environmental conditions. You
} } *may* have sufficient EMI isolation, given the distances. Vibration
} } isolation is very dependent on the building construction and source levels
} } and more difficult to guess/estimate.
} }
} } } From your description, there are no high current wiring or switchboxes
} } nearby. I would be most concerned about mechanical vibrations with EMI
} } concerns secondary.
} }
} } The question is: How expensive is a vibration survey vs. moving the sem and
} } finding it will not do your work?
} }
} } Woody
} }
} }
} }
} } Woody White
} } BWXT Services:
} } http://www.bwxt.com/bwxt.html
} } My Site:
} } http://woody.white.home.att.net
} }
} } -----Original Message-----
} } } From: Brian.Kirkmeyer-at-iff.com [mailto:Brian.Kirkmeyer-at-iff.com]
} } Sent: Monday, June 14, 2004 9:04 AM
} } To: Microscopy-at-MSA.Microscopy.Com
} } Subject: [Microscopy] SEM site assessment
} }
} }
} }
} } ----------------------------------------------------------------------------
} } --
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------------
} } ---
} }
} } Our SEM (JEOL 6360 LV w/tungsten filament) is likely being relocated along
} } with the rest of our lab to a second-floor location (the room is on a
} } concrete slab) in the general vicinity of a mainframe computer, an
} } elevator, a men's room and a large outside air conditioning unit. I have
} } asked to give an expert opinion on the feasibility of this move from a
} } noise (electromagnetic and vibration) standpoint. The proposed room is ~
} } 40 feet from the mainframe (as the crow flies, across the hall with
} } multiple walls in between), ~ 40 feet from the elevator (same side of the
} } hallway, four walls between), next door to the men's room (but the stalls
} } are on the opposite wall) and ~ 20 feet from the outside A/C unit. The
} } scope is on a JEOL-supplied air table, and I typically image at less than
} } 5,000x magnification (usually no higher than 1,000x). My samples are
} } predominantly organic in nature (cloths, polymers, hair).
} }
} } I have proposed to have the room assessed for the various types of noise
} } (~$3,500), but have been greeted with resistance by management, who
} } expected about $300 (and have no expertise in microscopy). So I ask those
} } on the ListServer who have encounted a similar noise concern for an SEM
} } lab relocation, should I expect to have issues with electromagnetic or
} } vibrational noise due to any of the mainframe, elevator, men's room or A/C
} } unit (or even second-floor on concrete location)?
} }
} } I thank you in advance for any assistance.
} }
} } Kirk
} }
} } Brian (Kirk) Kirkmeyer, Ph.D.
} } Research Scientist, Microscopy
} } International Flavors and Fragrances
} } 1515 State Highway 36
} } Union Beach, NJ 07735-3542
} } 732-335-2426 / 732-335-2350 FAX
} } brian.kirkmeyer-at-iff.com
} }
}
} James S. Romanow
} The University of Connecticut
} Physiology and Neurobiology Department
} Electron Microscopy Facility
} Unit 3242
} BSP Building, Room G06
} 91 North Eagleville Road
} Storrs, CT 06269-3242
}
} 860 486-2914 voice
} 860 486-6369 fax
} james.romanow-at-uconn.edu
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 14 21:23:27 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (muchphoto-at-Earthlink.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Monday, June 14, 2004 at 14:11:43
---------------------------------------------------------------------------

Email: muchphoto-at-Earthlink.net
Name: Michael Reese Much

Education: Undergraduate College

Location: Bethlehem, PA USA

Question: I am photographing protozoa and am looking for a way to slow them down or even kill them for digital photomicroscopy. I am using methyl cellulose to slow them down but I'd like to find a way to incapacitate them without their cellular structure disintegrating.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 01:10:02 2004

Contents Retrieved from Microscopy Listserver Archives
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muchphoto-at-Earthlink.net (by way of Ask-A-Microscopist) wrote:
} } } ------------------------------------------------------------------------------} The Microscopy ListServer -- Sponsor: The Microscopy Society of America} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html} -------------------------------------------------------------------------------} } Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (muchphoto-at-Earthlink.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Monday, June 14, 2004 at 14:11:43} ---------------------------------------------------------------------------} } Email: muchphoto-at-Earthlink.net } Name: Michael Reese Much} } Education: Undergraduate College} } Location: Bethlehem, PA USA} } Question: I am photographing protozoa and am looking for a way to slow them down or even kill them for digital photomicroscopy. I am using methyl cellulose to slow them down but I'd like to find a way to incapacitate them without their cellular structure disintegrating.} } ---------------------------------------------------------------------------Dear Michael Much: What kind of microscopy are you using for digital photomicroscopy of protozoa? Your post doesn't specify what kind, but I'm presuming that you're using light microscopy in conjunction with digital photography. I'm hardly an expert on protozoa in general, but I did some work on ciliates while I was working on my M.A. thesis about 4 years ago. Methyl cellulose should indeed slow down protozoa (and definitely on ciliates), but apparently it's affecting the cell's cellular structure. I'm not sure what other chemicals could slow down protozoa other than methyl cellulose, but I do know of various methods in light microscopy that can kill protozoa. For example, if you're working in a lab that uses traditional electron microscopy techniques, then you might have access to toxic but effective chemicals like osmium tetroxide (OsO4). The vapors from that chemical!
are usually sufficient to kill protozoa. Alternatively, you could pursue using a small amount of, say, glutaraldehyde or some other kind of fixative. I'm guessing that adding a small amount, and then diluting it alot by repeated washes might result in a clean enough slide for photomicrography. Good luck with your assignment. Nelson Conti

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 03:31:00 2004

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Below are some articles from Miscape that address slowing down
protozoa and vital staining of live protozoa. Many of the classic
formula for slowing various wee creatures call for narcotics that we
considered difficult to get. I have found that most are not if you
know a doctor well enough that he trusts you to use the substance
for what you say you are going to use it for and don't live in an
area the US Drug Enforcement is making an example of at the time.
The last time I needed chloroform I got a prescription from a
veterinarian. My doctor had no problems with a small bottle of coral
hydrate already diluted and if I wanted cocaine I would talk to my
eye doctor and as for an amount so small that it would be worthless
as a stimulant and dilute it on the spot. A compounding pharmacy
will have cocaine as well but when it gets to class 3 narcotics that
have to be written on the DEA pad most doctors are pretty careful
not write any that look odd.

CO2 bubbled in the media slows and kills many organisms. Physical
compression in thick media also helps. If you can't find a
compressing cell I have been looking for and excuse to make some for
my own use and this might get me off high center.

Matching the chemical to the desired action generaly relaxation at
death or as the processes slow is what is desired and sometimes can
be achieved by using weaker slower acting solution of the chemical.
If you can find a proven protocol and the chemical it is far better
to use it than to water time developing you own.

Far better to walk on the shoulders of giants than to wander then
wilderness alone doing the same work over and over again.

On slowing and killing protozoa
http://www.microscopy-uk.org.uk/mag/indexmag.html?http://www.microscopy-uk.org.uk/mag/artmay02/rhmicrotech.html

Vital staining
http://www.microscopy-uk.org.uk/mag/indexmag.html?http://www.microscopy-uk.org.uk/mag/artfeb00/rhvital.html

Good luck
Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

----- Original Message -----
} From: "by way of Ask-A-Microscopist" {muchphoto-at-Earthlink.net}
To: {microscopy-at-microscopy.com}
Sent: Monday, June 14, 2004 9:46 PM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (R.H.Olley-at-reading.ac.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, June 14, 2004 at 12:51:52
---------------------------------------------------------------------------

Email: R.H.Olley-at-reading.ac.uk
Name: Robert H. Olley

Organization: Reading University

Title-Subject: [Microscopy] [Filtered] Shadow direction in EM and planetary exploration

Question: I have recently seen some planetary exploration photographs which remind me of features seen in polymers under SEM / TEM. If you look at the following two

(a) Olympus Mons Caldera on Mars:

http://nssdc.gsfc.nasa.gov/imgcat/html/object_page/vo1_890a68.html

(b) Craters on Phoebe from Cassini:

http://antwrp.gsfc.nasa.gov/apod/ap040614.html

Don't you think they've got the shadow direction wrongly oriented? The Phoebe craters look like tents and the caldera appears to be sticking up. Not the sort of mistake an electron microscopist would make!?

* * * * * * * * * * * * * * * * * *

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 07:47:42 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (R.H.Olley-at-reading.ac.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, June 15, 2004 at 03:05:19
---------------------------------------------------------------------------

Email: R.H.Olley-at-reading.ac.uk
Name: Robert H. Olley

Organization: Reading University

Title-Subject: [Microscopy] [Filtered] Slowing down protozoa

Question: to: Michael Reese Much

I remember my biology teacher telling us that one used menthol to kill amoeba. Most agents are so aggressive that the amoeba withdraws its pseudopods and goes into a lump, but menthol kills the amoeba so gently that "it doesn't know what's happening to it". That way, one can get static amoeba with pseudopods extended.

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 07:47:49 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (romano-at-mpie.de) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, June 15, 2004 at 03:30:45
---------------------------------------------------------------------------

Email: romano-at-mpie.de
Name: Patricia Romano

Organization: Max Planck Institut

Education: Graduate College

Location: D¸sseldorf, Nord-Rhein Westfalia, Germany

Question: Dear Sir or Madam,
Currently I am trying to use SEM and LOM to see the structure of crustacean shells. I was looking on the net for information related to preparation of the samples. I was wondering if it would be possible to get some information related to this. Could you please give me any hints about how
to prepare the samples?, or where should I look to get a deeper knowledge of biological
tissues?. Could you recommend some literature related to it?.
Thank you very much in advance.
Best regards.

Patricia Romano

Dr. Patricia Romano Triguero
Max-Planck-Institut fuer Eisenforschung
Abteilung - Mikrostrukturphysik und Umformtechnik
Max-Planck-Str. 1
40237 Duesseldorf
Deutschland

Tel +49 (0)211-6792-663
Fax +49 (0)211-6792-333
Email romano-at-mpie.de

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 10:30:40 2004

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Getting ready for new SEM, I find the following
odd items if someone can use them:

2ea FEI 13423 LaB6 cathodes, appear to be new
1ea FEI 12629 LaB6 cathode
1ea FEI 18570 Schottky FE cathode, appears new
1ea Denka M1-EM {100} 90 degrees 15uR LaB6 cathode, new
1ea box with 5 large Mo apertures 13-1 200234, new
10ea Topcon filaments AW030WET(?) new in box
Strange looking LeMont Scientific Quad solid state BSE
preamp with diodes. Square 4-hole mounting flange
with O-ring. Diode plate swings out and back manually.

If anyone knows what these are for and can use them,
let me know. Otherwise, they go to trash.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 10:36:42 2004

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Rosemary,
Back in 1980 I would put the Hg in a 10 cm petri dish to check for
vibration. It 'got the job done' but I like your idea better.

Regards,
Jim

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 12:52:04 2004

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Unfortunately for images like these too often interpretation is
complicated.
But the outline of shadows tells us that we have impressions, not
plateaus.
For example, smaller round caldera on the top has a long sharp shadow
that
definitely looks like shadow from the rim and not shadow formed by the
rounded
top of the plateau. If you rotate this image 90 degrees left, so that
brightest
rim will be on the bottom, you'll get image more familiar for our eyes
(illuminated from the top) and caldera definitely will be seen as
depression
with smaller calderas as even deeper depressions.

Vladimir

} -----Original Message-----
} From: by way of MicroscopyListserver [mailto:R.H.Olley-at-reading.ac.uk]
} Sent: Tuesday, June 15, 2004 8:08 AM
} To: microscopy-at-microscopy.com
} Subject: [Microscopy] viaWWW: Shadow direction in EM and
} planetary exploration
}
}
}
}
} --------------------------------------------------------------
} ----------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} --------------------------------------------------------------
} -----------------
}
} Below is the result of your feedback form (NJZFM-ultra-55).
} It was submitted by (R.H.Olley-at-reading.ac.uk) from
} http://microscopy.com/MicroscopyListserver/MLFormMail.html on
} Monday, June 14, 2004 at 12:51:52
} --------------------------------------------------------------
} -------------
}
} Email: R.H.Olley-at-reading.ac.uk
} Name: Robert H. Olley
}
} Organization: Reading University
}
} Title-Subject: [Microscopy] [Filtered] Shadow direction in EM
} and planetary exploration
}
} Question: I have recently seen some planetary exploration
} photographs which remind me of features seen in polymers
} under SEM / TEM. If you look at the following two
}
} (a) Olympus Mons Caldera on Mars:
}
} http://nssdc.gsfc.nasa.gov/imgcat/html/object_page/vo1_890a68.html
}
} (b) Craters on Phoebe from Cassini:
}
} http://antwrp.gsfc.nasa.gov/apod/ap040614.html
}
} Don't you think they've got the shadow direction wrongly
} oriented? The Phoebe craters look like tents and the caldera
} appears to be sticking up. Not the sort of mistake an
} electron microscopist would make!?
}
} * * * * * * * * * * * * * * * * * *
}
} --------------------------------------------------------------
} -------------
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 13:54:20 2004

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On Jun 15, 2004, at 6:07 AM, by way of MicroscopyListserver wrote:

} Title-Subject: [Microscopy] [Filtered] Shadow direction in EM and
} planetary exploration
}
} Question: I have recently seen some planetary exploration photographs
} which remind me of features seen in polymers under SEM / TEM. If you
} look at the following two
}
} (a) Olympus Mons Caldera on Mars:
}
} http://nssdc.gsfc.nasa.gov/imgcat/html/object_page/vo1_890a68.html
}
} (b) Craters on Phoebe from Cassini:
}
} http://antwrp.gsfc.nasa.gov/apod/ap040614.html
}
} Don't you think they've got the shadow direction wrongly oriented?
} The Phoebe craters look like tents and the caldera appears to be
} sticking up. Not the sort of mistake an electron microscopist would
} make!?
}
Dear Robert,
You are quite correct that the direction of the shadow changes the
perception of height so that depressions appear raised and mounds
appear as craters; this is a fairly well-known visual phenomenon. The
advantage of a laptop is that one can hold the screen upside down and
see the proper perspective. As to whether "they've got the shadow
direction wrongly oriented", one disadvantage of ultramacroscopy is
that the lighting conditions are fixed, and, until we can figure out
how either to move the sun or provide a new one, we have to take what
is given. Of course, the images could be rotated by 180 degrees before
they're posted, but that would interchange the north and south poles,
which goes against astronomical convention.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 14:21:17 2004

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Darryl,

Don't know anything about the company......but perhaps you might look into
SEMTech Solutions. They offer service for AMRAY SEMs, and also offer
Re-manufactured Pre-owned Scanning Electron Microscopes.

http://www.semtechsolutions.com/

Kelly A. Ramos
Metallurgical Engineer / Supervisor
Argo-Tech Materials Laboratories
23555 Euclid Avenue
Cleveland, OH 44117
216-692-5904 or 216-692-5446
(fax) 216-692-5816
http://www.atclabs.com

darryl krueger
{dkruege-at-CLEMS To: Microscopy-at-MSA.Microscopy.com
ON.EDU} cc:
Subject: [Microscopy] Looking to buy SEM
06/14/04 03:30
PM

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Dear Listees,

We're loosing our Hitachi 3500 SEM due to a split in the EM facility here
at Clemson University. Is there anything out there available, comparable
on a used basis. We're looking for equipment and a price. Thanks in
advance for any information.

Darryl Krueger, RA
BioScience Dept.
Clemson University

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 15:06:43 2004

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More odd items.

Two bags of Pella 16292 100ea 15mmx10mm
specimen mounts and four Pella 1666
mount grabbing tweezers. If these
fit your SEM and you can use them,
first $15 for UPS shipping gets all.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 20:53:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (muchphoto-at-Earthlink.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, June 15, 2004 at 10:50:50
---------------------------------------------------------------------------

Email: muchphoto-at-Earthlink.net
Name: Michael Much

Education: Undergraduate College

Location: Bethlehem, PA, USA

Question: Thanks to everybody for your replies regarding slowing down protozoa. The diversity of answers was quite interesting. I really liked the link to vital staining of protozoa--something I have been experimenting with.
I called my veterinarian regarding the suggestion of lidocaine and she felt it would most likely destroy any cellular organisms.
Some of you asked what type of scope I'm using--it's a light microscope--a trinocular and I have fabricated my own camera mounts for the third tube to accept film cameras, digital cameras and video cameras.
I am not a student but rather an amateur microscopist who is doing his own experimentation in shooting microscopic invertebrates.

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 15 21:55:22 2004

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To researchers out there in cyberspace. We are very intereted in localising
types of collagen by immunocytochemistry on paraffin or resin sections of
human tympanic membranes. If anyone has any suggestions on where to buy
collagen antibodies that will work on the above please contact us.

Many thanks

Terry

Dr Terry Robertson (PhD)
Senior Research Fellow and Acting Manager
School of Surgery and Pathology
First Floor M Block, QE2 Medical Centre
Mailbag M504
University of Western Australia
Nedlands, Australia 6907
Phone 61 8 93462935
Fax 61 8 93462891
Mobile 0403025440
email terryr-at-cyllene.uwa.edu.au

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 06:30:10 2004

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Thank you to everyone who provided me with input! It has been a ton of
help.

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy
International Flavors and Fragrances
1515 State Highway 36
Union Beach, NJ 07735-3542
732-335-2426 / 732-335-2350 FAX
brian.kirkmeyer-at-iff.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 10:16:45 2004

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Fellow Microscopists,

If you haven't already taken a look at the new online microscopy journal
www.modernmicroscopy.com, we suggest that you do, as it is becoming a
great microscopy resource. This peer reviewed journal features
articles, reviews, and tutorials about microscopy by some of the most
experienced microscopists in the field, and access is free. As the main
sponsor of the site, The McCrone Group staff has contributed a number of
articles to get the site started. We are actively looking for new
topics and ideas from the entire microscopy community. Submission
information can be found on the site, and contributions are always
welcome. The success of the site is determined by the participation
from and the benefits provided to the microscopy community.

Thank you, on behalf of the McCrone Group,

Elaine Schumacher
Senior Research Scientist
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539 USA
630-887-7100 (tel)
630-887-7417 (fax)
E-mail: eschumacher-at-mccrone.com
Web Site: www.mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 11:26:24 2004

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Hello, all,

Join your colleagues this October in Cork, Ireland for the Conference on Food Structure and Food Quality. Sponsored by the Food Structure & Functionality Forum Division and the European Section of the AOCS.

This three-day symposium will hold a comprehensive technical program in addition to three intensive short courses.

The conference will also feature the winner of the 2004 Food Structure & Functionality Division Lifetime Achievement Award, Professor Anne-Marie Hermansson, SIK, The Swedish Institute for Food and Biotechnology, Gothenburg, Sweden.

Organizers are still accepting abstracts for oral and poster presentations through 30 June. Visit :
http://www.aocs.org/meetings/fsq/call.asp for more information, including online registration and the complete technical program.

Register by 3 September to receive the early registration rate.

Paula M. Allan-Wojtas, Past Chair, Food Structure and Functionality Forum, a division of AOCS.

Research Scientist - Food Microstructure/chercheur scientique - microstructure des aliments
Food Safety and Quality team/ Salubrité et qualité des aliments
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 902-679-5566
Facsimile/Télécopieur: 902-679-2311
32 Main Street/ 32, rue Main
Kentville, Nova Scotia/ Kentville (Nouvelle-Écosse)
B4N 1J5

allanwojtasp-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 12:11:22 2004

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Contributions about FIB are certainly welcome. Articles related to any
aspect of optical and electron microscopy, related techniques and
instrumentation will be considered for publication. We invite you to
take a look at the site, and help us to expand range of subjects that
you find there.

Regards,

Elaine

Elaine Schumacher
Senior Research Scientist
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539 USA
630-887-7100 (tel)
630-887-7417 (fax)
E-mail: eschumacher-at-mccrone.com
Web Site: www.mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 15:39:20 2004

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A recent question has come up around our labs, and that is, "What effect
do wireless laptop computers employing 802.11 B\A\G, Wireless Access
Points, Cell Phones, Cordless Phones and other hand held wireless deices
have on the performance of SEMs, TEMs, EELS spectrometers, and EDX
Spectrometers". We are going to try to formulate some test methods to
evaluate this, but I was hoping that maybe someone out there in the
Microscopy World has had some experience with this subject, or has some
Words of Wisdom on the subject.

John Mardinly
Intel

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 17:33:17 2004

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Colleagues,

BAL-TEC AG and Boeckeler Instruments/RMC Products cordially invite you to the
Bal-Tec Tutorial on SEM-Controlled Broad Ion Beam Sample Preparation,
presented by Dr. Wolfgang Gruenewald.

**When**:
Tuesday, August 3, 5:00 - 6:00 pm.

**Where**:
M&M 2004 (Savannah, Georgia), Exhibition Hall, Booth #606

**Info**:
Learn about Bal-Tec's new SEM-controlled Broad Ion Beam Milling System for
site specific EM specimen preparation.

Attendance is limited; sign up at the MSA Education Booth after you register
for the meeting.

For individual demonstrations, sign up at Booth #606 or contact Barbara at
Bal-Tec: barbara.etlinger-at-bal-tec.com.

See you in Savannah!

Bob Chiovetti
Senior Product Specialist
RMC Products/Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 16 18:20:20 2004

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(6/16/04 14:01) Mardinly, John {john.mardinly-at-intel.com} wrote:

} A recent question has come up around our labs, and that is, "What effect
} do wireless laptop computers employing 802.11 B\A\G, Wireless Access
} Points, Cell Phones, Cordless Phones and other hand held wireless deices
} have on the performance of SEMs, TEMs, EELS spectrometers, and EDX
} Spectrometers". We are going to try to formulate some test methods to
} evaluate this, but I was hoping that maybe someone out there in the
} Microscopy World has had some experience with this subject, or has some
} Words of Wisdom on the subject.
}
} John Mardinly
} Intel

John,

802.11 uses the 2.4 GHz band. If there is an effect, I'd expect you'd be able to detect it with a Fourier transform on the resulting image (much like you can find 60 Hz noise from the E field of power lines). If you were trying to design an experiment, I'd use a directional WiFi antenna at a known angle across the sample. My sense of the orders of magnitude makes me think that the SEM would not show any effect except at perhaps the highest possible magnifications, but the math on that is pretty easy to work out.

Cell phones use different bands, depending on the carrier and the service type. Those numbers are available online, but if memory serves. Most phones use 900, 1800 or 1900MHz bands. I think that US cell phones primarily use 900 and 1900 MHz.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 05:55:21 2004

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Bob

FYI, Tutorial Announcement at the M&M 2004 meeting are done by the
Education Committee. A single announcement is made annually.
I appreciate your enthusiasm to let people know about your
tutorial, however, can you in the future please coordinate with me and/or
the education committee with respect to Education Committee
functions. It is preferrable to do a one time posting rather
than lots of individual ones.

Thanks in advance

Nestor

At 6:55 PM -0400 6/16/04, RCHIOVETTI-at-aol.com wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 07:53:15 2004

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I've received a reply to yesterday's posting indicating that there's a
problem with getting past the main page of the modernmicroscopy.com site
and accessing the articles. I tried it myself this morning both through
the link that I provided and through Internet Explorer, and found the
site to be locked up at present. I checked with one of our IT staff,
and found that this has been an intermittent problem since the site was
set up. The problem is with the internet service provided, and they
haven't been able to resolve it yet, but I've been told that it seems to
clear up on its own, and the site becomes accessible again. I had
replies yesterday that indicated that people had been able to use the
link in my posting to get to the journal articles.

Of the many times that I've gone to the journal in the past several
months, this is the first time that I've encountered this problem. I
guess it's Murphy's Law in action, to have the glitch occur just when I
send out an invitation to the listserver community to visit the site!
I'm sorry for any frustration that this may have caused, and urge you to
try again at a later time. I'll check the site periodically myself. If
you continue to have access problems, please let me know.

Regards,

Elaine

Elaine Schumacher
Senior Research Scientist
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539 USA
630-887-7100 (tel)
630-887-7417 (fax)
E-mail: eschumacher-at-mccrone.com
Web Site: www.mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 09:21:22 2004

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Dear Microscopists,

An major update of the list of meetings for microscopists in the year
2005 has been finished at the Petr's Microscopy Resources at the

http://www.petr.isibrno.cz/microscopy/meetings.php#2005

Your submission of other meetings will be very appreciated (submission
form is accessible from the page mentioned, the direct link is
http://www.petr.isibrno.cz/microscopy/PMRform.php).

Petr Schauer

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 10:16:17 2004

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Greetings, listers,

A customer of mine is trying to view osteoblasts grown on a peptide layer
on titanium disks. In both her conventional SEM and my ESEM, she has seen
patches of cellular adhesive on the peptide layer, but the cells are
missing (she knows from other procedures that the cells have been growing
well on the disks).

Do you have any suggestions for specimen preparation (other than
glutaraldehyde fixation) that would keep the osteoblasts intact for SEM?

Thanks!

Leslie Eibest
SEM lab
Dept. of Biology
Duke University

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 11:34:39 2004

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Dear Microscopists

We have started long-term live cell experiments (} 24 hours) and
although I have followed basic instructions learned over the years,
there are still problems with our setup.

If anyone is interested in the details, we have a fair-sized
plexiglass incubator housing the microscope stage into which I have put
a water-filled flask through which CO2 is bubbled, we have a heater
stage, a blower providing warm air and an extra container of water for
humidity. Still, after several hours, when the temperature should have
stabilized, we see drift in focus, condensation on the inside of the lid
of the cell culture dish and inadequate humidity. CO2 is not regulated
accurately.

Does anyone know of any webiste or other literature - with lots of
pictures - to see how others have designed and used live cell setups.

Thank you in advance
Judy

Judy Trogadis
Bio-Imaging Coordinator
St. Michael's Hospital, 7Queen
30 Bond St.
Toronto, ON M5B 1W8
Canada
ph: 416-864-6060 x6337
pager: 416-685-9219
fax: 416-864-6043
trogadisj-at-smh.toronto.on.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 11:48:22 2004

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Brent,

I am not sure how you would measure a GHz signal on an image. Even if you
acquire a 2kx2k image in 1 second, the sample frequency is a few MHz. That
means, that the highest frequency you can measure is of the same order
(Nyquist). If you can't measure it, it will not show up in FFTs either.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Brent Neal [mailto:brent-at-reindeergraphics.com]
Sent: Wednesday, June 16, 2004 17:42
To: Mardinly, John
Cc: Microscopy-at-MSA.Microscopy.Com

All items have new homes.

Thanks for the replies.

gary g.

At 08:51 AM 6/15/2004, I wrote:

} Getting ready for new SEM, I find the following
} odd items if someone can use them:
}
} 2ea FEI 13423 LaB6 cathodes, appear to be new
} 1ea FEI 12629 LaB6 cathode
} 1ea FEI 18570 Schottky FE cathode, appears new
} 1ea Denka M1-EM {100} 90 degrees 15uR LaB6 cathode, new
} 1ea box with 5 large Mo apertures 13-1 200234, new
} 10ea Topcon filaments AW030WET(?) new in box
} Strange looking LeMont Scientific Quad solid state BSE
} preamp with diodes. Square 4-hole mounting flange
} with O-ring. Diode plate swings out and back manually.
}
} If anyone knows what these are for and can use them,
} let me know. Otherwise, they go to trash.
}
} gary g.
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 12:52:48 2004

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These have a new home.

Thanks for the replies.

gary g.

At 01:27 PM 6/15/2004, I wrote:

} More odd items.
}
} Two bags of Pella 16292 100ea 15mmx10mm
} specimen mounts and four Pella 1666
} mount grabbing tweezers. If these
} fit your SEM and you can use them,
} first $15 for UPS shipping gets all.
}
} gary g.
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 13:08:13 2004

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Thanks to all for your responses and suggestions regarding the current
problem in accessing the ModernMicroscopy site. We appreciate the
feedback, and are working with our internet service provider to correct
the problem. I'll post an update when the issues are resolved, and
again, I apologize for the frustration that this may have caused to
anyone trying to access the site.

Regards,

Elaine

Elaine Schumacher
Senior Research Scientist
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539 USA
630-887-7100 (tel)
630-887-7417 (fax)
E-mail: eschumacher-at-mccrone.com
Web Site: www.mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 13:21:54 2004

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Listers -

Has anyone out there looked at shark (OK, dogfish) vertebrae in an
SEM? A colleague from down the hall in the fisheries department has some
vertebrae (sectioned and unsectioned) that he'd like to look at in order to
count the rings (kind of like the rings in a tree stump). The rings are just
too close together to clearly differentiate in a binocular scope, but I was
thinking in order for them to show up in an SEM there has to be a density or
textural difference between "ring" and "inter-ring" areas. Would etching of
sectioned ones with something help? (These vertebrae are not true bone of
course, but a sort of calcified cartilage, so I suppose an acid might do
something usefull......)
I'm open to all ideas......

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 13:49:48 2004

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Howdie!

I don't think that the GHz signal is going to affect the electron
beam inside the column, it's all about skin depth.
The most common way for disturbances of this kind is through
cables between equipment, power lines and tracks on circuit
boards. Any non linear electronics will create overtones, and
if you have a signal in your system it will also create modulation
products that is added as noise. Since all electronic circuits are
nonlinear it will add noise, then it is up to the system design to
compensate and filter out any noise.
If you modulate (turning on and off) the GHz signal with a
slower frequency you should get a detectable signal in the
picture of more or less sharp features.
Since most of the devices you named in the first letter is using
time division multiplexing this should be simple to set up.
In the most basic way you could use a cellular phone and just
make a call. The duty cycle in a cellular system is in the order
of 1/8th active and have a repetition frequency of around a
couple of hundred hertz.
For the exact numbers it depends on the phone system used
and local settings. But it shouldn't be hard to find out in a web
search or a call to the phone company.
If you adjust the scanning speed you could probably get a
striped picture as the signal is adding to the noise level in your
system.

For a quick demo of the effect try putting your cellular phone
near your computer monitor and make a call to see the effects.
You don't see the GHz signal but the added noise is affecting
circuits and you will see the time division.

I have never done any measurements like this since I just got
our TEM working after a year of repairs and renovation. Now
it's grounded again while we build a closed cooling system.
Last week we got an EDS so we have to put some work into
it again and get the system up and running.
http://www.home.neab.net/gandalf/EM-lab/TEM100CX/index.htm

What I have done is worked with micro wave equipment and
also designed electronic equipment with radios.

Btw, it's fully possible to sample a GHz signal at a couple of MHz.
You can't recreate the original signal (that's Nyquist) but you will
get a downconversion in the frequency band (folding distortion).
This is a trick used in software frontends in the mobile phone
system in the base stations.
But any right designed A/D sampler in a system should have a
filter in front of it to remove any signal above Nyquist, that's
why the signal shouldn't appear directly in the picture.

As a final disclaimer I'm not going to take any responsibility if
you damage your equipment. The signal levels from a mobile
could be really high and affect the electronics, especially older
equipment not designed for the wireless age. Start with a good
distance between the phone and the equipment before getting closer.

Regards, Göran

Mike Bode wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 13:50:04 2004

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(6/17/04 11:07) Mike Bode {mb-at-soft-imaging.com} wrote:

} Brent,
}
} I am not sure how you would measure a GHz signal on an image. Even if you
} acquire a 2kx2k image in 1 second, the sample frequency is a few MHz. That
} means, that the highest frequency you can measure is of the same order
} (Nyquist). If you can't measure it, it will not show up in FFTs either.
}
} mike

That was the point I was making exactly, and what I meant when I said "the math is straightforward."

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 14:09:25 2004

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Lets be careful what we play with at home.
http://www.biomedcentral.com/news/20040617/04

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 14:38:48 2004

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The lockup problem with modernmicroscopy.com has been resolved, and the
site is now accessible. We're not sure at this point if a high request
volume resulting from my initial posting was the cause of the problem,
but we'll continue to monitor the situation and work toward resolution
of any ongoing issues. Thanks again to all for your patience and your
feedback. As I said in my original message, please consider submitting
articles for publication. We look forward to your contributions.

Regards,

Elaine

Elaine Schumacher
Senior Research Scientist
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539 USA
630-887-7100 (tel)
630-887-7417 (fax)
E-mail: eschumacher-at-mccrone.com
Web Site: www.mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 15:02:35 2004

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} A customer of mine is trying to view osteoblasts grown on a peptide layer on
} titanium disks. In both her conventional SEM and my ESEM, she has seen
} patches of cellular adhesive on the peptide layer, but the cells are missing
} (she knows from other procedures that the cells have been growing
} well on the disks).
}
} Do you have any suggestions for specimen preparation
} (other than glutaraldehyde fixation) that would keep the osteoblasts
} intact for SEM?
}
} Leslie Eibest
} SEM lab, Dept. of Biology, Duke University
===========
Leslie,
Please let us know if the cells were Critical Point Dried, HMDS, etc.

There are some factors that apply to all preparations and some not.
If the cell side of the disc comes in contact with other surfaces
the cells can be mechanically knocked off. Were the discs secured in a holder?
There may be expansion/contraction factors in play because a metal was
used instead of glass or a plastic as a carrier for the peptide and cells.

Has any TEM shown the contact between the peptide and the osteoblasts?
Do they stuck together well or only in small patches? I assume that a
cross-section work-up was done to establish the fact that the cells do
adhere well to the peptide.

Pat Connelly
Univ. of Pennsylvania, Biology Dept.

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 16:30:39 2004

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Dear Goran,
I remember when Hitachi brought a FETEM to the Seattle ICEM meeting, the highest
resolution was affected when the security guards activated their walkie-talkies.
It just blurred the lattice they were showing a little. I think this is a much
lower frequency than the GHz that cordless phones use, but certainly the highest
resolution may be affected by radio interference affecting the electronics.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
tel: 604-822-5648
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Göran Axelsson" {axelsson-at-acc.umu.se}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, June 17, 2004 12:16 PM

Howdie!

I don't think that the GHz signal is going to affect the electron
beam inside the column, it's all about skin depth.
The most common way for disturbances of this kind is through
cables between equipment, power lines and tracks on circuit
boards. Any non linear electronics will create overtones, and
if you have a signal in your system it will also create modulation
products that is added as noise. Since all electronic circuits are
nonlinear it will add noise, then it is up to the system design to
compensate and filter out any noise.
If you modulate (turning on and off) the GHz signal with a
slower frequency you should get a detectable signal in the
picture of more or less sharp features.
Since most of the devices you named in the first letter is using
time division multiplexing this should be simple to set up.
In the most basic way you could use a cellular phone and just
make a call. The duty cycle in a cellular system is in the order
of 1/8th active and have a repetition frequency of around a
couple of hundred hertz.
For the exact numbers it depends on the phone system used
and local settings. But it shouldn't be hard to find out in a web
search or a call to the phone company.
If you adjust the scanning speed you could probably get a
striped picture as the signal is adding to the noise level in your
system.

For a quick demo of the effect try putting your cellular phone
near your computer monitor and make a call to see the effects.
You don't see the GHz signal but the added noise is affecting
circuits and you will see the time division.

I have never done any measurements like this since I just got
our TEM working after a year of repairs and renovation. Now
it's grounded again while we build a closed cooling system.
Last week we got an EDS so we have to put some work into
it again and get the system up and running.
http://www.home.neab.net/gandalf/EM-lab/TEM100CX/index.htm

What I have done is worked with micro wave equipment and
also designed electronic equipment with radios.

Btw, it's fully possible to sample a GHz signal at a couple of MHz.
You can't recreate the original signal (that's Nyquist) but you will
get a downconversion in the frequency band (folding distortion).
This is a trick used in software frontends in the mobile phone
system in the base stations.
But any right designed A/D sampler in a system should have a
filter in front of it to remove any signal above Nyquist, that's
why the signal shouldn't appear directly in the picture.

As a final disclaimer I'm not going to take any responsibility if
you damage your equipment. The signal levels from a mobile
could be really high and affect the electronics, especially older
equipment not designed for the wireless age. Start with a good
distance between the phone and the equipment before getting closer.

Regards, Göran

Mike Bode wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 20:41:44 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (dorit-at-burnham.org) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, June 17, 2004 at 12:12:40
---------------------------------------------------------------------------

Email: dorit-at-burnham.org
Name: Dorit Hanein

Organization: The Burnham Institute

Title-Subject: [Microscopy] [Filtered] Position Open: Electron Microscopist
Research Assistance

Question: Position Open: Electron Microscopist Research Assistance,
to start August, 2004. (http://www.burnham-inst.org).

Requirements include working knowledge of high resolution TEM and a
BA/BS or equivalent experience in biological or material science, or
bioengineering. Responsibilities include negative stain sample
preparation and electron microscopy, vitreous ice sample preparation
and electron cryo-microscopy, some microscope maintenance and
standard biochemical analyses.

Application should include a statement of career goals and addresses
for three references. Salary is competitive and commensurate with
experience. EOE.

Send applications to: Dr. Dorit Hanein, e-mail dorit-at-burnham.org

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 17 20:42:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (Wall1-at-LLNL.GOV) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, June 17, 2004 at 13:12:50
---------------------------------------------------------------------------

Email: Wall1-at-LLNL.GOV
Name: Mark A. Wall

Organization: Lawrence Livermore National Laboratory

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: The Characterization group in the Chemistry and
Materials Science Directorate at LLNL, Livermore, CA, has an opening
for a PhD. level candidate. The selected candidate will be
responsible for the daily operations of a new dual-beam FIB equiped
with EDS, OIM, CL, lift-out, injections gases, STEM, etc. The
selected candidate will supervise one dedicated technican who will
maintain and operate the instrument. In addition, the selected
candidate will be responsible for working with numerous staff
scientists for the application of FIB technology as well as
developing dual-beam experimentation, applications, etc. as required
for numerous materials programs at LLNL. Experience with hands-on FIB
techniques is required. Experience with TEM and other materials
characterzation techniques is highly desired.

Applications shall be submitted on-line at http://jobs.llnl.gov/prod_index.html

The job posting number is 001906.

Please refer questions to Mark A. Wall -at- wall1-at-LLNL.GOV

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From MicroscopyL-request-at-ns.microscopy.com Fri Jun 18 03:58:43 2004

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Frank,
Cartilage is nearly all protein. Have you considered tagging it with
fluorescent antibodies? There may be one available for use in a
non-shark ( bovine? human?) cartilage imaging application that would
bind well enough to shark. Some of genetic machinery (and the proteins
that result) which allowed early the chordates to flourish remains
essentially unchanged. Perhaps that optical scope will still be the
quick and easy solution.

Bob Carter
2000 Bayshore Road
Lopez Island, WA 98261

-----Original Message-----
} From: Thomas, Frank [mailto:FThomas-at-nrcan.gc.ca]
Sent: Thursday, June 17, 2004 11:44 AM
To: Microscopy-at-MSA.Microscopy.Com

Listers -

Has anyone out there looked at shark (OK, dogfish) vertebrae in
an SEM? A colleague from down the hall in the fisheries department has
some vertebrae (sectioned and unsectioned) that he'd like to look at in
order to count the rings (kind of like the rings in a tree stump). The
rings are just too close together to clearly differentiate in a
binocular scope, but I was thinking in order for them to show up in an
SEM there has to be a density or textural difference between "ring" and
"inter-ring" areas. Would etching of sectioned ones with something help?
(These vertebrae are not true bone of course, but a sort of calcified
cartilage, so I suppose an acid might do something usefull......)
I'm open to all ideas......

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography, P.O. Box
1006, Dartmouth, Nova Scotia B2Y 4A2 Ressources naturelles Canada,
l'Institut Oceanographique du Bedford, B.P. 1006, Dartmouth,
(Nouvelle-Ecosse) B2Y 4A2 Government of Canada/Gouvernement du Canada

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 18 07:32:13 2004

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Hi Pat,

Re: cell adhesion on titanium disks, you wrote:

} ===========
} Leslie,
} Please let us know if the cells were Critical Point Dried, HMDS, etc.

For her conventional SEM workup, the cells were dehydrated in ethanol, then
critical point dried and sputter coated. For ESEM work in my lab, we put
disks with cells directly in the scope, and viewed them wet at about 5 Torr
and 3 C.

} There are some factors that apply to all preparations and some not.
} If the cell side of the disc comes in contact with other surfaces
} the cells can be mechanically knocked off. Were the discs secured in a holder?

For ESEM work, since we didn't do any processing, I don't think the cells
contacted any other surfaces.

} There may be expansion/contraction factors in play because a metal was
} used instead of glass or a plastic as a carrier for the peptide and cells.

That could be, since the samples were chilled.

} Has any TEM shown the contact between the peptide and the osteoblasts?
} Do they stuck together well or only in small patches? I assume that a
} cross-section work-up was done to establish the fact that the cells do
} adhere well to the peptide.

She hasn't done any TEM that I'm aware of, but has been able to recover
growing cells from the disks. The fact that we could see where the cells
used to be attached gave us the impression that they had adhered to the
peptide layer. We don't know about cell distribution on the disk - that's
what she was trying to determine with the SEM.

Thanks for your help!

Leslie

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 18 07:55:39 2004

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hi leslie

i used to do a lot of work on bone/implant interface and osseointegration
including culture studies. i would grow long-term (2-6 months) osteogenic cells
(released from fetal mouse calvaria) on commercially pure titanium and titanium
alloy dics. i viewed specimens that i ran through CPD after glut fixation.
partly, i was looking for neural "contaminant" cells that were growing on top of
the osteogenic cells and they were fairly easy to see. the osteo cell lawn is
very difficult to see since the cells attach and flatten out much like epithelial
or fibroblast cells and form a thin layer on the surface. this was true even
before confluency and this was on uncoated titanium surfaces. adding a protein
coating will make the visualization even more difficult as i found using various
extracellular matrix protein coatings. if i used fine sandpaper to rough up the
surface, i could easily see the surface groves "through" the cell layer. in
short, don't expect the cells to look distinct especially after several days in
culture since they lay down their own matrix and adhesion proteins and are pretty
much part of the surface.

hope this helps.

tbudd

Pat Connelly wrote:

} ------------------------------------------------------------------------------
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}
} } A customer of mine is trying to view osteoblasts grown on a peptide layer on
} } titanium disks. In both her conventional SEM and my ESEM, she has seen
} } patches of cellular adhesive on the peptide layer, but the cells are missing
} } (she knows from other procedures that the cells have been growing
} } well on the disks).
} }
} } Do you have any suggestions for specimen preparation
} } (other than glutaraldehyde fixation) that would keep the osteoblasts
} } intact for SEM?
} }
} } Leslie Eibest
} } SEM lab, Dept. of Biology, Duke University
} ===========
} Leslie,
} Please let us know if the cells were Critical Point Dried, HMDS, etc.
}
} There are some factors that apply to all preparations and some not.
} If the cell side of the disc comes in contact with other surfaces
} the cells can be mechanically knocked off. Were the discs secured in a holder?
} There may be expansion/contraction factors in play because a metal was
} used instead of glass or a plastic as a carrier for the peptide and cells.
}
} Has any TEM shown the contact between the peptide and the osteoblasts?
} Do they stuck together well or only in small patches? I assume that a
} cross-section work-up was done to establish the fact that the cells do
} adhere well to the peptide.
}
} Pat Connelly
} Univ. of Pennsylvania, Biology Dept.

--
Dr. T. Budd
Professor and Chair of Biology
St. Lawrence University
Canton, NY 13617
Phone = 315-229-5640
Fax = 315-229-7429
E-mail = tbudd-at-stlawu.edu

This message is made of 100% recycled electrons!

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 18 08:10:34 2004

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John;

If you are using a cell phone for this test, be aware that the output
power the antenna provides is a function of what the cell base station
tells it to put out and that's a function of the power the base station
receives. You will unlikely have constant output power from a cell
phone. If this is a test you really need to do, you should simulate the
RF with a generator and the modulation scheme you wish to use, i.e.
CDMA, TDMA, GSM etc, You will also need an antenna and power
meter/spectrum analyzer to really know what power level you have at the
intended target, EM column/electronics?

Peter Tomic
Agere Systems

-----Original Message-----
} From: Brent Neal [mailto:brent-at-reindeergraphics.com]
Sent: Wednesday, June 16, 2004 7:42 PM
To: Mardinly, John
Cc: Microscopy-at-MSA.Microscopy.Com

(6/16/04 14:01) Mardinly, John {john.mardinly-at-intel.com} wrote:

} A recent question has come up around our labs, and that is, "What
} effect do wireless laptop computers employing 802.11 B\A\G, Wireless
} Access Points, Cell Phones, Cordless Phones and other hand held
} wireless deices have on the performance of SEMs, TEMs, EELS
} spectrometers, and EDX Spectrometers". We are going to try to formulate

} some test methods to evaluate this, but I was hoping that maybe someone

} out there in the Microscopy World has had some experience with this
} subject, or has some Words of Wisdom on the subject.
}
} John Mardinly
} Intel

John,

802.11 uses the 2.4 GHz band. If there is an effect, I'd expect you'd be
able to detect it with a Fourier transform on the resulting image (much
like you can find 60 Hz noise from the E field of power lines). If you
were trying to design an experiment, I'd use a directional WiFi antenna
at a known angle across the sample. My sense of the orders of magnitude
makes me think that the SEM would not show any effect except at perhaps
the highest possible magnifications, but the math on that is pretty easy
to work out.

Cell phones use different bands, depending on the carrier and the
service type. Those numbers are available online, but if memory serves.
Most phones use 900, 1800 or 1900MHz bands. I think that US cell phones
primarily use 900 and 1900 MHz.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 18 11:40:25 2004

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Cartilage has a lot of glycosamionglycans (hyaluronic acid and
various chondroitin sulfates) to go along with the proteins, cells and
fibers of various types. All of these components vary in propotion to
the type of cartilage, its location and (I would suspect) the species.
An LM stain like Alcian Blue or colloidal iron might be of use

Bob Carter wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
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From MicroscopyL-request-at-ns.microscopy.com Sat Jun 19 07:35:13 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (k.bustamante-at-surrey.ac.uk) from http://microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Friday, June 18, 2004 at 14:09:33
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Email: k.bustamante-at-surrey.ac.uk
Name: Karla Bustamatne

Organization: University of Surrey

Education: Graduate College

Location: Surrey, UK

Question: HI. I had taken histological samples on the locust ventral cord. I am taking neural recordings using penetrating electrodes. I was hoping to take the recordings and then remove the probe and be able to find track where the probe was positioned. I was unable to find any. Therefore i left one of the probes inside the tissue and proceed with the histology procedure. I found that close to the region where the probe was teh staining is poor. I was wondering if the probe which is make of silicon oxide and gold electrodes could have had an effect on the staining. I used bodian, cresyl fast violet and haemotoxily and eosin staining methods.
I am not an experience histologist.Actually my main degree is in electronics so apologize if i am asking something obvious.

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From MicroscopyL-request-at-ns.microscopy.com Sat Jun 19 20:53:23 2004

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HPH (Hello, and Please Help.) I have been trying to make
formvar support grids by methods that have always produced
good results in years past. Now, however, the formvar
refuses to leave the glass slides as I lower them into a
container of water. Has anyone experienced this? Can you
give ne a clue? My procedure now and in the past is to dip
clean slides in a solution (w/v) of 0.25% formvar in
dichloroethane, air dry, then scrape bottom and sides with
a razor blade. What do you think? Humidity? Phase of the
moon? Bad hands? Please advise. WJP

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 20 01:55:32 2004

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HHH (Hello, Here's help),
Yes, it is probably humidity, phase of the
moon, or the pollen. What I have found helps ever so much with
Formvar is to take a kimwipe (a brand of tissue paper--probably lens
paper would work too) and rub it vigorously over the surface of the
slide and then dip into the Formvar and cast as usual. I guess this
charges the surface with a little static electricity, but whatever
the mechanism this seems to work a treat.

Happy casting,
Tobias

}
}
} HPH (Hello, and Please Help.) I have been trying to make formvar
} support grids by methods that have always produced good results in
} years past. Now, however, the formvar refuses to leave the glass
} slides as I lower them into a container of water. Has anyone
} experienced this? Can you give ne a clue? My procedure now and in
} the past is to dip clean slides in a solution (w/v) of 0.25% formvar
} in dichloroethane, air dry, then scrape bottom and sides with a
} razor blade. What do you think? Humidity? Phase of the moon? Bad
} hands? Please advise. WJP

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 20 13:51:53 2004

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After scraping an outline of the film to be cast with a clean razor blade,
I breathe on the coated slide and the vapor of my breath makes the film
look frosty. Then I quickly dip the slide at a 45 degree angle into a bowl
of water and the film floats off. If you don't want to blow on the slide, I
have held the slide over a beaker of hot water (recently boiled) and the
water vapor likewise makes the film on the slide look frosty. As an aside,
I no longer use Formvar or Parlodian, but prefer Butvar which, in my hands,
makes very stable films even during the humidity of summer in Iowa. I don't
even bother to carbon coat my films which I routinely cast on 1X2 copper or
nickel slot grids.

Dean Abel
Biological Sciences 143 BB
University of Iowa
Iowa City IA 52242-1324

At 09:15 PM 6/19/2004 -0500, you wrote:
} HPH (Hello, and Please Help.) I have been trying to make formvar support
} grids by methods that have always produced good results in years past.
} Now, however, the formvar refuses to leave the glass slides as I lower
} them into a container of water. Has anyone experienced this? Can you give
} ne a clue? My procedure now and in the past is to dip clean slides in a
} solution (w/v) of 0.25% formvar in dichloroethane, air dry, then scrape
} bottom and sides with a razor blade. What do you think? Humidity? Phase of
} the moon? Bad hands? Please advise. WJP

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 20 14:58:19 2004

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I am working on a project to examine the optical crystallography of fossil
bones and teeth in thin section. There are abundant publications with SEM
images of fossil teeth (particularly enamel) that have been etched to show
the orientation of the apatite crystallites. Similar studies of bone
materials appear to be sparse (!). Since I'm a bit out of my area here,
could anyone on the list direct me to a site, or publications, that might
supply me with some SEM images of fossil (or recent) bone that show the
microstructure in detail? Thanks for any help in this area.

Henry Barwood
Associate Professor of Science, Earth Science
Department of Math and Physics
MSCX 312G
Troy State University
Troy, Alabama 36082
hbarwood-at-troyst.edu

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 20 22:18:02 2004

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The problem is not one that can be blamed on, or cured with black magic, but simply to do with the glass surface interacting with the formvar film. Did you by any chance change the make of the slides you are using? Or perhaps you changed the way you clean the glass.

I use glass slides from VWR that are cleaned superficially by dipping in alcohol and then wiping clean with lens paper. The coating and floating always works if I keep things the same.

If I leave the slides in the alcohol for too long, the film reamins stuck to the glass. If I wipe with anything other than the lens tissue, the film sticks. If I use other glass slides, the film sticks. If I clean any glass surface too well (e.g. in chromic acid) the film always sticks. Interestingly, when I try to grow cells on super-cleaned glass coverslips, the cells avoid the glass surface completely.

I am always surprized when rational scientists who meet a problem with a technique are willing to blame it on some supernatural event. Look more closely at the details and the mystery will be explained (i.e. do some experiments).

I once had a problem with Lowicryl not polymerizing. Instead of blaming anyone or any thing, we figured out the problem. It turns out that plastic tubes with orange tops can be fabricated in two sorts of plastic. We had been using polypropylene tubes but accidentally switched to polystyrene without really noticing. Mix Lowicryl in polystyrene tubes and it will not polymerize! No magic there.

The answers are out there!

Regards,

Paul Webster.

-----Original Message-----
} From: Perreault,William [mailto:william.j.perreault-at-lawrence.edu]
Sent: Sat 6/19/2004 7:15 PM
To: Microscopy-at-msa.microscopy.com
Cc: william.j.perreault-at-lawrence.edu

HPH (Hello, and Please Help.) I have been trying to make
formvar support grids by methods that have always produced
good results in years past. Now, however, the formvar
refuses to leave the glass slides as I lower them into a
container of water. Has anyone experienced this? Can you
give ne a clue? My procedure now and in the past is to dip
clean slides in a solution (w/v) of 0.25% formvar in
dichloroethane, air dry, then scrape bottom and sides with
a razor blade. What do you think? Humidity? Phase of the
moon? Bad hands? Please advise. WJP

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 02:49:35 2004

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......... clean the glass slide under warm tap water with a bristle
brush and curd soap (no soap with smelling substances etc) rinse only
shortly with destilled or deionised water, let it dry at the air and
polish it with an absolute clean linnen cloth.
then go on as you always did but breath "slowly and heavily " on the
slide before immersing it extremely slowly at an 45 degree angle into
the water.
works with all glass slides (don't use superfrost slides for this
special purpose).

peter heimann

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 06:57:02 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (flechedorfr-at-netscape.net) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, June 21, 2004 at 05:59:47
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Email: flechedorfr-at-netscape.net
Name: flechedorfr

Title-Subject: [Microscopy] [Filtered] MListserver:TEM course

Question: Hello everyone
I am searching some internet courses on transmission electron microscopy. Can anyone please provide me to on-line websites?
Thanks in advance

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From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 07:42:10 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (akoorts-at-medic.up.ac.za) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Monday, June 21, 2004 at 01:13:51
---------------------------------------------------------------------------

Email: akoorts-at-medic.up.ac.za
Name: Alida Koorts

Organization: University of Pretoria

Education: Graduate College

Location: Pretoria, South Africa

Question: IN SITU HYBRIDIZATION for electron microscopy on core bone marrow biopsies. I need all the help I can get. First, the hybridization solution - damages the sections, I have found that two hours at 37 degrees celcius is perhaps the limit for hybridization incubation time but I get no labeling. I have tried 4 hours and 12 hours - perhaps a little labeling but the sections are damaged, difficult to distinguish the cells. I have used a probe concentration of 600 ng/ml - is this high or low? The probe that I use is about 250 bp long, PCR digoxygenin labeled. The hybridization solution contains 50% formamide, is this perhaps too stringent? Pretreatment of the sections - 10 ug/ml. Any other suggestions for pretreatment?
Regards
Alida

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From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 07:42:47 2004

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I had a similar sample last year - The researcher was looking at otoliths
from fish 'ears' and wanted to count the rings to age his sample - DIC in a
metallurgical (reflection) microscope worked well - growth rings were quite
visible, well differentiated and easy to count. Dogfish vertebrate are much
bigger than the otoliths though. Your colleague might have to slice them
thinner and perhaps cut into quarters to properly fit the stage of the
'scope

Richard Harris
Technical Manager
Imaging and Analysis
Department of Biology
University of Western Ontario
London Ontario CANADA
Ph. 519-661-2111 ext. 86780
Fax 519-661-3935

-----Original Message-----
} From: Thomas, Frank [mailto:FThomas-at-nrcan.gc.ca]
Sent: Thursday, June 17, 2004 2:44 PM
To: Microscopy-at-MSA.Microscopy.Com

Listers -

Has anyone out there looked at shark (OK, dogfish) vertebrae in an
SEM? A colleague from down the hall in the fisheries department has some
vertebrae (sectioned and unsectioned) that he'd like to look at in order to
count the rings (kind of like the rings in a tree stump). The rings are just
too close together to clearly differentiate in a binocular scope, but I was
thinking in order for them to show up in an SEM there has to be a density or
textural difference between "ring" and "inter-ring" areas. Would etching of
sectioned ones with something help? (These vertebrae are not true bone of
course, but a sort of calcified cartilage, so I suppose an acid might do
something usefull......)
I'm open to all ideas......

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 09:24:24 2004

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Hi William,
Our lab has experienced this problem in the past, too. We use slides
from Corning Glassworks and found when we switched from using double
frosted slides to plain, non-frosted slides, the Formvar stuck
relentlessly to the slides. Switching back to double frosted slides
cured the problem.
Shannan

Shannan Little
Research Technician
Electron Microscopy/ Image Analysis
Agriculture & Agri-Food Canada
Lethbridge, Alberta
http://res2.agr.ca/lethbridge/emia/index_e.htm

-----Original Message-----
} From: Perreault,William [mailto:william.j.perreault-at-lawrence.edu]
Sent: Saturday, June 19, 2004 8:16 PM
To: Microscopy-at-msa.microscopy.com
Cc: william.j.perreault-at-lawrence.edu

HPH (Hello, and Please Help.) I have been trying to make
formvar support grids by methods that have always produced
good results in years past. Now, however, the formvar
refuses to leave the glass slides as I lower them into a
container of water. Has anyone experienced this? Can you
give ne a clue? My procedure now and in the past is to dip
clean slides in a solution (w/v) of 0.25% formvar in
dichloroethane, air dry, then scrape bottom and sides with
a razor blade. What do you think? Humidity? Phase of the
moon? Bad hands? Please advise. WJP

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 11:17:25 2004

Contents Retrieved from Microscopy Listserver Archives
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Project MICRO is MSA's educational outreach program. The MICRO pages
on the MSA website (URL below) have just been updated (THANK YOU,
Nestor!) and are definitely worth a visit. The bibliography of
books, videos, CD-ROMs, and web links now has a powerful search
engine, which makes it easy to find items. And the quotes about
microscopy are always fun...

Caroline
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 14:05:03 2004

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These organisms, or spores, were found in large masses on the surface of cat feces, which had been in a moist environment for some time. The individual spores appear brown under a microscope, but the masses of spores are bright red. The spores are about 5 microns in diameter, and all the same size and distinctive shape. I considered the possibility that they might be a myxomycete, but have not been able to find any with spores resembling these. If anybody knows what species this is, or even is sure of what class of organisms it belongs to, please let me know. The spores can be seen at: http://www.msu.edu/~common/Unknown.jpg. Thanks.

Ralph Common

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 15:44:58 2004

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I study diffraction of 2 keV electrons from nano-fabricated gratings, and
I have three questions:

What is the lowest energy TEM available?

How small a voltage gives good results with TEM instruments (and samples)?

What is the lowest energy beam usually (or ever) used for e diffraction?

- Alex Cronin
Dept. of Physics
Univ. of Arizona
Tucson, AZ 85721
(520) 465-8459

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 15:48:17 2004

Contents Retrieved from Microscopy Listserver Archives
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I study diffraction of 2 keV electrons from nano-fabricated gratings, and
I have three questions:

What is the lowest energy TEM available?

How small a voltage gives good results with TEM instruments (and samples)?

What is the lowest energy beam usually (or ever) used for e diffraction?

- Alex Cronin
Dept. of Physics
Univ. of Arizona
Tucson, AZ 85721
(520) 465-8459

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 16:17:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mark.nathanson-at-umdnj.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, June 21, 2004 at 12:54:59
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Email: mark.nathanson-at-umdnj.edu
Name: Mark Nathanson

Organization: New Jersey Medical School

Title-Subject: [Microscopy] [Filtered] MListserver: EM- LKB Repair

Question: Does anyone know of a service facility or person for LKB Ultramicrotomes?

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From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 16:17:55 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jean-ross-at-uiowa.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, June 21, 2004 at 08:58:37
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Email: jean-ross-at-uiowa.edu
Name: Jean Ross

Organization: Central Microscopy Research Facility, Univ. of Iowa

Title-Subject: [Microscopy] [Filtered] Lynx processor

Question: Hello Everyone,

I would like the input of anyone who is a user of the Lynx EM processor. We have been having some mixed results in TEM processing of various tissues, resulting in soft blocks.

I have observed that the dehydrants are evaporating so that by the time the tissues reach those stations they are half their original volume. We have the unit in a fume hood. How do others handle possible evaporation and water uptake issues? We generally follow our normal protocols that we use for hand processing. Any tips or suggestions would be welcome.

Thanks,
Jean Ross

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From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 17:45:22 2004

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On Jun 19, 2004, at 7:15 PM, Perreault,William wrote:

} Now, however, the formvar refuses to leave the glass slides as I
} lower them into a container of water. Has anyone experienced this? Can
} you give ne a clue?

Dear William,
I had similar problems, not with plain formvar, but with holey
formvar, and the solution was to put a layer of Apiazon L onto the
slide. Two ways that worked were to put a small dab on the slide and
spread it with a finger and thumb on opposite sides of the slide or to
dissolve the Apiazon in a hydrocarbon solvent and dip the slide as one
would into the formvar. The former method has advantages for holey
films in that it causes the holes to line up in the direction that one
rubbed one's finger; the latter method should give a more uniform
film--although I never measured this--so is more suitable for plain
formvar films. I also dissolves 0.25 g of Alconox in 1 L water, heated
the solution to 50 C and used the warm solution to float off the
formvar. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 21 19:44:41 2004

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We are interested in electropolishing away some electroless nickel in
order to do TEM on some thin gold palladium plating on the electroless
nickel. Does anyone know of a good electrolyte for electropolishing the
electroless nickel? Thanks.

John Mardinly
Intel

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 01:21:48 2004

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Ralph,
They look like diatoms to me. Do you ever see anything that
look like hyphae in the cultures?

Just an off the cuff guess though, I don't know.

TB

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \
University of Massachusetts
/ / / \ \ \
Amherst, MA, 01003
/ / ___ / \ \__/ \ ____ Voice: 413 - 545 - 1533
Fax: 413 - 545 - 3243
http://www.bio.umass.edu/biology/baskin/

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 06:59:49 2004

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Hello Jean:

If your dehydrants are evaporating to half their volumn; the vials are not sealing correctly to the "Vial Sealing Assembly" which is attached to the processor lid. The only time vials are open to the air and subject to evaporation is when the processor is changing stations or the vial is being used. Whether or not the processor is in the fume hood really is not in play because the lid on the Lynx should be closed during process.

Chances are the "Seal Assembly" is defective due to age and exposure to solvents & resins. Other possibilities exsist but this is the most common cause.

Best Regards,

Al Coritz
Electron Microscopy Sciences
215-412-8400
www.emsdiasum.com

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 11:40:19 2004

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If you teach microscopy (at any educational level!) you'll be
interested in an article that has just appeared in the online journal
Cell Biology Education: "Microscopy images as interactive tools in
cell modeling and cell biology education", by a group in Brazil.
You'll find it at
http://www.cellbioed.org/articles/vol3no2/article.cfm?articleID=104
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 13:30:12 2004

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John,
I don't know if this will work for you, but for my Ph.D. work, I electropolished Ni emitters with a solution of HCl at room temperature using 5-10 V ac. I think that the solution was about 10%. The trick for Ni was that it didn't work well with fresh solution. What I did was put a pinch of NiCl in the solution to get the right slightly green color and it worked very nicely. I assume that this will work for you and probably be inert to the Au-Pd, but I can't be certain. I will check my dissertation to see if I have the recipe right. It has been a few years since then!

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Monday, June 21, 2004 9:10 PM
To: microscopy-at-msa.microscopy.com
Cc: Sim, Kian Sin

We are interested in electropolishing away some electroless nickel in
order to do TEM on some thin gold palladium plating on the electroless
nickel. Does anyone know of a good electrolyte for electropolishing the
electroless nickel? Thanks.

John Mardinly
Intel

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 17:13:48 2004

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Hello All,

Is there a simple test available for testing deionized
water quality? The building in which I work has a
couple of different water filtration systems. One is
the millique system, while the other is a 'homemade'
distillation system. I want to know if there is a
diference in water quality between the two. I have
used a simple water tester for a microbiology class I
took a couple of years ago. It had a grayish colored
grid pattern that estimates the number of microbes
present in the water. You add some water to the unit
and let it set for a set time period. After the
requisite time period, you check the grid pattern to
see if anything grew. This device may/may not be
appropriate for what I am looking for. Any suggestion
will be appreciated.
Sara Goldston

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 18:49:57 2004

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On Jun 22, 2004, at 3:39 PM, sara goldston wrote:

} Is there a simple test available for testing deionized
} water quality? The building in which I work has a
} couple of different water filtration systems. One is
} the millique system, while the other is a 'homemade'
} distillation system. I want to know if there is a
} diference in water quality between the two. I have
} used a simple water tester for a microbiology class I
} took a couple of years ago. It had a grayish colored
} grid pattern that estimates the number of microbes
} present in the water. You add some water to the unit
} and let it set for a set time period. After the
} requisite time period, you check the grid pattern to
} see if anything grew. This device may/may not be
} appropriate for what I am looking for. Any suggestion
} will be appreciated.
}
Dear Sara,
There are three concerns for water purity. The crudest is whether
anything is growing in it; since not a lot will grow in a saturated
NaCl solution, you can see that the microbe test isn't very stringent.
The presence of ions increases the conductivity, so having a
conductance meter will tell you how free of ions your water is. There
can be non-ionic solutes, however, that do not increase the
conductivity, so, while conductivity is the usual measure of water
purity, there can still be dissolved material. In fact, the output of
ion exchange resins--used in many water-purification systems--can
contain non-ionic material generated by the resin itself, so, for
really pure water, the output of the millique system can be distilled.
There may even then be impurities, but deionized, distilled water is
usually adequate. I don't know any test better than conductivity for
water purity.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 22 22:30:07 2004

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Dear Listers

I have some nanotubes which show structures in CCl4 or
chlorofrom. I wanted to scan them in TEM, What kind of
film can I use apart from Formvar or colloidin, Carbon
coating also did not help.
Any suggestions

Shashi Singh
CCMB
Hyderabad
INDIA

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From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 09:22:18 2004

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Hi listers,

Is there a way to make SEM pictures 3D? I know that tilting is involved,
what degree? Is it better to colorize and use the red/blue glasses or is
just tilting and using the stereo glasses best?

Any pointers about making a 3D pix would be greatly appreciated.

Tilting at windmills covered in algae,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 10:06:34 2004

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You might try Tek-Net in Lakewood, NJ. 732-905-5530.

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 10:24:20 2004

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We want to put a simple high resolution camera on our Zeiss Axiophot and
are considering a Nikon Coolpix 5000 or something similar. However, before
purchasing one, we would really like to see one attached to a computer in
use. This is for a multi-user facility and we want to see how simple it
really is to use and to what extent it can take low-light images.

Is there anyone in NYC or lower Westchester who has such a set up and a few
minutes to show me?

Thanks!

____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 11:05:33 2004

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Paula Sicurello asked

} Is there a way to make SEM pictures 3D?

Ah, at last, a subject where I can contribute. Yes. 3D SEM images are quite
possible.

I know that tilting is involved, what degree?

Do not tilt. You simply want horizontal displacement. If you tilt you will
introduce perspective errors.

} Any pointers about making a 3D pix would be greatly appreciated.

See if you can contact Dee Breger. She published a book of 3D SEM photos
("Through the Electronic Looking Glass: 3D Images from a Scanning Electron
Microscope," Cygnus Graphic, 1995). They were anaglyphs. Since SEM photos
are by nature monochromatic, an anaglyph is a very suitable means of
reproducing the image. If you plan on making false color images then you may
want to consider a more sophisticated method.

I believe Ms. Breger is now at Drexel with an email deebre-at-coe.drexel.edu.

Good luck,

Bruce Girrell

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 11:26:13 2004

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Hi Paula,

Here's the method that I've been taught.
Pick an area and take the photo normally
Tilt the subject/sample 6 degrees. If you're doing very high mag make sure
you can get pack to the exact original area.
We use a program called PCI Quartz which lets us process it under Stereo Pair.
Pick the color, match the photos. When your satisfied with the overlay and
have saved it rotate the photo 70 degrees.

Linda S. McCorkle
Ohio Aerospace Institute
Materials Division, Polymers Branch
NASA John H. Glenn Research Center at Lewis Field
21000 Brookpark Road
Cleveland, OH 44135

Tel.: (216) 433-3689
Fax: (216) 977-7132
e-mail: Linda.S.McCorkle-at-grc.nasa.gov

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 11:43:20 2004

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Please spread the word to interested qualified persons. (Please
don't respond to me, I have nothing to do with this position)

Histology/Electron Microscopy position

Children's Hospital and Health Center in San Diego has an immediate opening
for an Electron Microscopist with some histology experience. For more
details regarding salary, job responsibilties and job requirements please
contact Eric A. Breisch at ebreisch-at-chsd.org or Anne Peters at
apeters-at-chsd.org. Interested candidates may also apply online at the
Children's Hospital web site.
(http://www.chsd.org)

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 11:49:57 2004

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Hi Paula,

My .02:

The typical value of tilt difference for stereo shots is 6 degrees.

Although not critical, it has been my experience that the optimum value can
vary slightly, depending on magnification, the specimen elevation variation,
and the tilt starting value.

Good depth of focus helps keep the images sharp. This translates to a small
final aperture and a long working distance.

I almost exclusively use two images and a viewer. I ran across a web site
that offers a number of viewers. Mine is (similar to) the F71. Works
great, but pricy. I have no info about the site other than the address.
http://www.ascscientific.com/stereos.html

While the anaglyph method (red/blue) works, the perception (for me) was
never as crisp and dramatic as the two image/viewer method. Perhaps a
function of my less than perfect red/green vision...

With practice, some can perceive stereo without a viewer. I have no trouble
doing that, but the effect for me is less than with a good viewer.

To try without viewer: Use ~4x5 inch images held at "reading distance" and
separated by about the width of an image. Cross your eyes (hope no one hits
you in head :), defocus, and a third image should form in the empty space
between the two actual images. Concentrating on the center pseudo-image,
bring the eyes into focus and relax the crossed eyes. Voila, Stereo!

One more thing... Be sure to position the images correctly. Transposing
the images can invert the perceived "ups & downs". In most cases the tilt
of the "average" surface can be observed. "Down hill" should be in the same
direction as the actual tilt.

Have fun!
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Paula Sicurello [mailto:PSicurel-at-odu.edu]
Sent: Wednesday, June 23, 2004 10:48 AM
To: microscopy-at-msa.microscopy.com

Hi listers,

Is there a way to make SEM pictures 3D? I know that tilting is involved,
what degree? Is it better to colorize and use the red/blue glasses or is
just tilting and using the stereo glasses best?

Any pointers about making a 3D pix would be greatly appreciated.

Tilting at windmills covered in algae,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 12:15:10 2004

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John, according to ASTM E407, one of the less hazardous etchants (polishes
at high currents) you can use for Ni and high Ni alloys (EN would fall
into this category) is made up with 70%v of H3PO4 and the balance (30%v)
water. Use electrolytic at 5-10 V for etching. So I would presume, that
for polishing use at } = 10 V. I haven't tried this one and precautions
are: USE IN HOOK. DO NOT STORE. Mix (make-up) fresh.

Happy Polishing,
Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.

"Mardinly, John" {john.mardinly-at-intel.com}
06/21/04 09:10 PM

To
{microscopy-at-msa.microscopy.com}
cc
"Sim, Kian Sin" {kian.sin.sim-at-intel.com}
Subject
Electropolishing ELectroless nickel

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We are interested in electropolishing away some electroless nickel in
order to do TEM on some thin gold palladium plating on the electroless
nickel. Does anyone know of a good electrolyte for electropolishing the
electroless nickel? Thanks.

John Mardinly
Intel

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 12:22:30 2004

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Hello Paula,

the technique you are referring to is called "Stereo imaging" or similar
(see for example http://www.soft-imaging.com/rd/english/405.htm). Basically
you acquire 2 images with a specified tilt difference. What is best depends
on what you want to do with the images.

Display on a computer monitor: If you don't have a special monitor that
allows the use of polarized glasses, you have two options:

1) create an anaglyphic image (red/blue or green/blue), and use the
appropriate glasses. This will give you a good 3D display on the monitor,
although the image appears yellowish.

2) Switch between the two stereo images repeatedly. If done correctly, it
will also provide a sense of depth without using any glasses, but the image
is not fixed (seems to be oscillating).

The stereo angle for these types of images should be in the range of 6-10
degrees. If you go much beyond that, the brain cannot fuse the two images
anymore. This also depends on the 3-dimensionality of the sample.

For printing you can go the anaglyphic route (see 1 above), or you can mount
two prints at appropriate distances and use special 3D glasses for looking
at the prints. These glasses make sure that each eye sees only the print
that it is supposed to see, and you get again a 3D impression, which can
also be in color. The anaglyphic images have the advantage that they are
independent of distance from the print. The stereo glasses require a
specified geometric arrangement, which includes the distance from the
prints.

Finally, you can also use the stereo images to calculate a 3D surface
profile of your sample (see again the link above). Once you have done that,
you can use 3D display software to rotate and look at the 3D object and
actually measure in 3 dimensions.

In all cases you need to "adjust" the images, i.e., pick one point that is
at the identical position on both images. If you don't do that, there may be
a lateral shift between the images that can destroy the 3D appearance.

Hope that explains a few things.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Paula Sicurello [mailto:PSicurel-at-odu.edu]
Sent: Wednesday, June 23, 2004 08:48
To: microscopy-at-msa.microscopy.com

Hi listers,

Is there a way to make SEM pictures 3D? I know that tilting is involved,
what degree? Is it better to colorize and use the red/blue glasses or is
just tilting and using the stereo glasses best?

Any pointers about making a 3D pix would be greatly appreciated.

Tilting at windmills covered in algae,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 13:02:09 2004

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Sorry Bruce, but tilting is crucial to making an anaglyph (or enabling the
viewer to see a 3D image when using red/green or red/blue glasses) of SEM
images. In short what you are doing is mimicking what your two eyes do when
you look at an object. Your eyes are tilted at slight angles relative to
each other. The Image seen thorough both eyes are combined in your brain to
produce an image with 3D information. If you only have one eye than you
cannot see in 3D unless shadows help fool your brain in interpreting the
image.

You can do the same thing with an SEM image. You need to take two
images with one tilted relative to the other. The amount of tilt depends on
the degree of roughness of the sample which is in turn somewhat related to
magnification, but usually 7 degrees is a good starting point. What is
important is to keep the center of the image stable for both images. This
is easily done by putting a piece of transparent film (such as from a clear
sheet protector) on the viewing screen and using a grease pencil to mark
relevant features near the center of the image. Then move the stage to line
up the second image.

Any adjustment in focus should be done by adjusting working distance.
If you use your focus knob you will be changing the strength of your final
(objective) lens which in turn affects the rotational path of the electrons
in the beam.

Modern microscopes have software to easily overlay the images to create
a red/blue or red/green image which, when viewed thorough the appropriate
glasses, will give you your 3D image. You can also take the two images and
combine them in PhotoShop, as well as other programs, to make the final
anaglyph.

If you need more complete instructions then E-mail me. I can send the
article that appeared in Microscopy Today, Vol #99-1 (Jan. 1999). The book
by Bozzola & Russell also contains a discussion of making stereo images.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 6/23/04 11:33 AM, "Bruce Girrell" {bigirrell-at-microlinetc.com} wrote:

}
}
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-
}
} Paula Sicurello asked
}
} } Is there a way to make SEM pictures 3D?
}
} Ah, at last, a subject where I can contribute. Yes. 3D SEM images are quite
} possible.
}
} I know that tilting is involved, what degree?
}
} Do not tilt. You simply want horizontal displacement. If you tilt you will
} introduce perspective errors.
}
} } Any pointers about making a 3D pix would be greatly appreciated.
}
} See if you can contact Dee Breger. She published a book of 3D SEM photos
} ("Through the Electronic Looking Glass: 3D Images from a Scanning Electron
} Microscope," Cygnus Graphic, 1995). They were anaglyphs. Since SEM photos
} are by nature monochromatic, an anaglyph is a very suitable means of
} reproducing the image. If you plan on making false color images then you may
} want to consider a more sophisticated method.
}
} I believe Ms. Breger is now at Drexel with an email deebre-at-coe.drexel.edu.
}
} Good luck,
}
} Bruce Girrell
}
}
}

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Paula

Tilt angle of between 5 and 7 degrees gives best results.
Large tilt angles may give excessive impression of depth.

Vital ingredients of success are to register the two
images carefully, and to use height (z) adjustment
only to refocus.

Also turn off any raster rotation.

Take first picture.

Mark a prominent central feature at approx
mean height (z) on screen using a water soluble OHP pen, and
return the feature to that position after tilting.

After tilting focus using specimen height adjustment only.
(Do not focus using focus controls, which change image magnification).

Take second picture.

In most SEMs tilt in the horizontal image axis, so the images
must be rotated 90 degrees for viewing. If you do this Clockwise
then the left eye image (coloured red in anaglyph images) is the one with more
tilt, and the right eye image (coloured green or cyan)
image is the one with less tilt.

To make a cyan/red anaglyph
Open both images in Photoshop (or similar)
Change the right eye (cyan) image's Mode to RGB
Select All of the Left eye (red) image,
Copy and paste it into the
Red colour channel of the Right eye image.
Save as ...

View with cyan red glasses.

Chris

Quoting Paula Sicurello {PSicurel-at-odu.edu} :

}
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}
}
}
}
} Hi listers,
}
} Is there a way to make SEM pictures 3D? I know that tilting is involved,
} what degree? Is it better to colorize and use the red/blue glasses or is
} just tilting and using the stereo glasses best?
}
} Any pointers about making a 3D pix would be greatly appreciated.
}
} Tilting at windmills covered in algae,
}
} Paula :-)
}
} Paula Sicurello
} EM Lab
} 106 Mills Godwin Sciences Building
} Old Dominion University
} Norfolk, VA 23529
} USA
} 757-683-3822
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 15:05:25 2004

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Greetings,

This may be a long shot, but here goes. We are in dire need of an external
computer control kit for a JEOL JSM-5800 SEM,(MP-87010 (EXT)). If anyone
has one that they can part with, or have a retired 5800, please contact me
by phone or email. Thanks in advance. Folks on this list server are great
- Thanks Nestor.

Joseph

Joseph M. Oparowski
Center for Materials Science - Consulting and Failure Analysis
Bose Corporation Joseph_Oparowski-at-bose.com
The Mountain, M/S 415 Phone: (508) 766-1371
Framingham, MA 01701-9168 Fax: (508) 766-1313

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 15:11:25 2004

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}
} Paula Sicurello asked
}
} } Is there a way to make SEM pictures 3D?
}
} Ah, at last, a subject where I can contribute. Yes. 3D SEM
} images are quite possible.
}
} I know that tilting is involved, what degree?
}
} Do not tilt. You simply want horizontal displacement. If you
} tilt you will introduce perspective errors.

Unfortunately horizontal displacemen works only at really low mags.
Tilting involves no errors in calculation and for human eye at
tilt angle 6 degrees there will be nothing unusual in stereo images.
For pretty flat surfaces I used tilt angles as high as 16
degrees without any problems with observation (with tilt plus-minus
8 degrees).

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 23 16:24:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ssamuelsson-at-eyetk.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, June 23, 2004 at 16:08:14
---------------------------------------------------------------------------

Email: ssamuelsson-at-eyetk.com
Name: Steven Samuelsson

Organization: Eyetech Pharmaceuticals, Inc

Title-Subject: [Microscopy] [Filtered] MListserver: Imaging Specialist and Postdoc positions available

Question: Eyetech Pharmaceuticals Inc., located in Woburn, MA., is recruiting for a biological light microscopy/IA associate. This talented individual will provide hands-on support to facility investigators. Required expertise includes quantitative image analysis, computer science, light/laser microscopy. We are also recruiting for a postdoctoral fellow to investigate issues and mechanisms of retinal vascular leakage and therapies using morphology-based approaches. Minimum requirements include competence with light and electron microscopy instruments and advanced research techniques in cell and membrane biology. It is not necessary to have a background in eye research. Eyetech is an equal opportunity employer. US citizenship/permanent residency visa for USA required, as is fluency in English.

Please respond with a CV and career objective statement to:

Steven J. Samuelsson, Ph.D.
Head: Morphology; Cell Biologist
Eyetech Pharmaceuticals, Inc.
Eyetech Research Center
42 Cummings Park
Woburn, MA. 01801
Tel: 781 938-3937 x314
Fax: 781 935-9083
ssamuelsson-at-eyetk.com
www.eyetk.com

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From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 01:15:11 2004

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Dear friends,
in order to check some possible FRET between FITC and ALEXA 555, when
using bleaching of acceptor as method, we found that 543 nm bleached
FITC as well.
Did you ever experience such a behaviour?
Alby

------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 13:46:07 2004

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Listers,

Here is the July 2004 Microscopy Today table of contents. I will close the
subscription list for this issue on Tuesday 29 June 2004.
Microscopists in North America and MSA members anywhere can subscribe for
free. Anyone else may subscribe for US$35 per year (to PARTIALLY cover
postage). All subscriptions at http://www.microscopy-today.com Thank you.

Carmichael Right at Your Fingertips

Alden& Galvis On The Trail of the Fathers: The Serendipitous Santos

Sedgewick Advantages of Adobe Photoshop Elements 2.0 over the
full version of Photoshop

Boyes & Gai ETEM Issues and Opportunities for Dynamic In-situ
Experiments

Diebold Microscopical Evaluation of Glass Delamination in
Pharmaceutical Vials: A Look at Three Different Vial Manufacturers

Clarke Chromatic Aberration in Digital Photomicrographs from
Microscopes Requiring Compensating Eyepieces

Brooker, et al. The Structural and Chemical Analyser - A New Analytical
Technique for SEM

Walck Comments on the Use of Digital Filters

Julthongpiput, Fasolka & Amis Gradient Reference Specimens for Advanced
Scanned Probe Microscopy

Dunn & Hull Three-dimensional Volume Reconstructions Using Focused Ion
Beam Serial Sectioning

Miller Surveillance of Bioterrorism Agents: Considerations for EM
Laboratories

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 13:58:55 2004

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Hi All:
I have been asked to check into the following by one of our personnel:

For the JEOL 200CX, how much total power does TEM supposed to draw at
200KV without the ASID?
Our system draws 15A (210V) at 200KV with HT on. With beam current at
150uA, it draws roughly 17A.
Among 15A, 8A is for all the electronics and vacuum pump, and 7A is for
lens. Is this normal?

For the Tracor TN5520, we are looking for a computer interface (PC
board, software, OR the original Tracor hardware) that will enable us to
generate spectrum. The closer to free the better. Any donations would
be gladly accepted.

Thanks,
Michael Coviello
UT Arlington

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 14:10:36 2004

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Stereo image of the sample?
http://biology.berkeley.edu/EML/stereo.html

Tilting can be from anywhere from 2 - 8 degrees or so. It depends on the
sample. If the sample has a lot of protrusions which stick out, stay with
a small tilt angle.
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

On Wed, 23 Jun 2004, Paula Sicurello wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
}
}
}
} Hi listers,
}
} Is there a way to make SEM pictures 3D? I know that tilting is involved,
} what degree? Is it better to colorize and use the red/blue glasses or is
} just tilting and using the stereo glasses best?
}
} Any pointers about making a 3D pix would be greatly appreciated.
}
} Tilting at windmills covered in algae,
}
} Paula :-)
}
} Paula Sicurello
} EM Lab
} 106 Mills Godwin Sciences Building
} Old Dominion University
} Norfolk, VA 23529
} USA
} 757-683-3822
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 14:21:49 2004

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Hello everyone,

I have a 80 x 1 column vector of numbers that represents a PSF for a micro
CT scanner. These numbers approximately follow a Gaussian distribution. I
wish to expand this distribution into an multiple dimensional matrix, 80 x
80 for example, for processing through deconvolution. Does any one have any
idea how I would go about doing this???

Thank you in advance,

Thomas Sadowski
Southern Connecticut State University

_________________________________________________________________
FREE pop-up blocking with the new MSN Toolbar – get it now!
http://toolbar.msn.click-url.com/go/onm00200415ave/direct/01/

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 15:39:16 2004

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Hi all,
One of the researchers here has contacted me about doing an EM
autoradiography experiment using 14C isotope. I believe he wants to
look at the uptake and fate of carbon from labeled nanotubes that are
presented to cell mono layers. I have read that 90% of the 14C
radiation stays within 20um of its entry point in the emulsion. Does
anyone know what the resolution can be for this technique and in
particular the 14C isotope?

Greg

--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
(405)325-4391
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 16:16:42 2004

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Hi all,
One of the researchers here has contacted me about doing an EM
autoradiography experiment using 14C isotope. I believe he wants to
look at the uptake and fate of carbon from labeled nanotubes that are
presented to cell mono layers. I have read that 90% of the 14C
radiation stays within 20um of its entry point in the emulsion. Does
anyone know what the resolution can be for this technique and in
particular the 14C isotope?

Greg

--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
(405)325-4391
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 17:13:02 2004

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Workshop Announcement
University of California at Santa Barbara

The Department of Molecular, Cellular, and Developmental Biology and the
Neuroscience Research Institute are sponsoring an advance course on light
microscopy. This 5-day workshop will be offered from September 13 through
September 17, 2004 and will consist of lectures and laboratory exercises
that will run from 9 am to approximately 5 pm each day. The seminar/workshop
will be intensive enabling participants to develop theoretical and hands-on
expertise with light microscopes. Attendees will interact closely with the
instructors while using modern research grade microscopes, cameras, and
computers. The seminars and laboratories will cover basic optical theory and
how it pertains to increasing contrast (signal to noise ratio) in biological
samples. Fundamental techniques such as fluorescence, phase contrast,
Nomarski differential interference contrast, and darkfield imaging will be
taught and attendees will use microscopes equipped with these optical
enhancement accessories. In addition, the theory and practice of electronic
image acquisition (analog and digital) will be discussed and attendees will
work with low-light cameras, digital image processing computers, and
morphometric programs. There are five research grade microscopes, five
electronic imaging cameras, two computer workstations, and one confocal
microscope. With a maximum enrollment of 10 students, there will be ample
opportunity to work with all of the microscopes and cameras. For those so
interested, intensive hands-on instruction and guidance on the confocal
microscope will be provided.

For a fuller description of the workshop, please check the web address
below. Enrollment forms can be completed online and this workshop provides
an opportunity to have a working-vacation in Santa Barbara, California.

http://www.lifesci.ucsb.edu/mcdb/events/events.html

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 19:40:10 2004

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(6/23/04 11:50) Michael Cammer {cammer-at-aecom.yu.edu} wrote:

} -------------------------------------------------------------------------------
}
} We want to put a simple high resolution camera on our Zeiss Axiophot and
} are considering a Nikon Coolpix 5000 or something similar. However, before
} purchasing one, we would really like to see one attached to a computer in
} use. This is for a multi-user facility and we want to see how simple it
} really is to use and to what extent it can take low-light images.
}
} Is there anyone in NYC or lower Westchester who has such a set up and a few
} minutes to show me?

Michael,

I would be very careful about using a cheap digital camera. Most especially, I would recommend against the specific model you have mentioned (Nikon Coolpix 5000) for one simple reason: there is no raw output. The only scientifically useful data format that the Coolpix 5000 outputs is TIFF, and even that is not very useful since the TIFFs are only 8 bit. Of course, you'll remember from the Computer-Assisted Image Analysis course at NCSU that JPEG is worse than useless. (You probably won't remember me - I was the young guy in the back running the computers.) The specifications of many cameras can be easily found from sites such as DPReview {http://www.dpreview.com} . If you really want to use a 'prosumer' camera, I'd start looking at specs there first.

You've probably paid a good deal of money from your scope. You shouldn't cripple your instrument by putting a POS camera on it. This is especially the case since you've already thrown up a warning flag by talking about low light images. Most consumer or 'prosumer' digital cameras deal with low light conditions extremly poorly - you'll get noisy images.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Thu Jun 24 21:17:46 2004

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Not that I know anything much about this stuff, but the Canon Powershot G5 is listed on
that link you gave as having RAW as the uncompressed file format.

Does this make it OK?

cheers

rtch

Date sent: Thu, 24 Jun 2004 21:05:42 -0400
} From: Brent Neal {brent-at-reindeergraphics.com}

:
: (6/23/04 11:50) Michael Cammer {cammer-at-aecom.yu.edu} wrote:
:
:
:
} -------------------------------------------------------------------
------------
: }
: } We want to put a simple high resolution camera on our Zeiss
Axiophot and
: } are considering a Nikon Coolpix 5000 or something similar.
However, before
: } purchasing one, we would really like to see one attached to a
computer in
: } use. This is for a multi-user facility and we want to see how
simple it
: } really is to use and to what extent it can take low-light images.
: }
: } Is there anyone in NYC or lower Westchester who has such a set up
and a few
: } minutes to show me?
:
:
Michael,

There is no way to connect the CoolPix camera directly to the
computer you have to connect the camera to the USB port and power
cycle the camera or remove the flash card and read it. Nor is there
an easy way to control the camera with a computer. There is some
soft ware out there that does control the camera but it is not very
good. Also test the camera for artifacts. I have heard that some of
the newer Coolpix camera don't have the problems that 995 and early
4500 and 5000 cameras had I document here
http://www.couger.com/microscope/shootout/shootout.html.

If you can't get a camera free of ring artifacts a used Coolpix 950
for $100 to $175 is a lot less frustrating to use and won't have the
problems that antialiasing software causes in the later models that
infuriates some users and doesn't bother others much at all. Most
users find the 950 is good enough for kind of pictures you will get
from any of the consumer cameras all things considered.

No consumer camera gives you the kind of imaging you need for
professional work. They all process the image before recording it
and work poorly in low light conditions. That can be fixed with
software ticks but cameras designed for microscope use will give a
lot better account for them selves and should fit in the work flow
much better. They don't cost that much more and the cost will be
quickly repaid by the ware and tear on your nerves of who ever is
using it every day.

Good luck
Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 04:17:58 2004

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Brent writes ...

} I would be very careful about using a cheap digital camera. Most
} especially, I would recommend against the specific model you have
} mentioned (Nikon Coolpix 5000) for one simple reason: there is no
} raw output. ...

This is not true ... raw output from the CP5000 is possible with a
firmware update that's been available for a couple of years. I.E., our
CP5000 has raw output. I will agree with your concerns regarding low light
acquisition, but the original post asked that he see it for himself, as he
should. I'd imagine he'd have little problem in the NYC area ... with help
from his peers ... sorry I cannot help.

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 05:58:49 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (longli_tem-at-hotmail.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, June 24, 2004 at 08:57:38
---------------------------------------------------------------------------

Email: longli_tem-at-hotmail.com
Name: Long Li

Organization: University of Pittsburgh

Title-Subject: [Microscopy] [Filtered] MListserver: A post-doctoral position is available

Question: Dear All:

A post-doctoral position is available starting immediately on the characterization of nanoparticles by advanced scanning transmission electron microscopy methods, such as quantitative Z-contrast imaging, electron energy loss spectroscopy, as well as high resolution electron microscopy. Experience with VG-STEM and Z-contrast imaging is specially appreciated. This is part of a collaborative program with University of Illinois at Urbana-Champaign and Brookhaven National Labs, to predict and determine the 3-dimensional supported structure of nanoparticles utilized in heterogeneous catalysis either as model systems or for water purification for fundamental understanding of nano-catalytic reactions.

To apply for this position, please send a resume with the names and contact information for three references, or to obtain more information, please contact:

Professor Judith Yang
848 Benedum Hall
Materials Science & Engineering Dept.
University of Pittsburgh
Pittsburgh, PA 15261

jyang-at-engr.pitt.edu
(412) 624-8613

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From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 05:59:28 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (nancy_phillips-at-hp.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, June 24, 2004 at 13:15:24
---------------------------------------------------------------------------

Email: nancy_phillips-at-hp.com
Name: Nancy Phillips

Organization: Hewlett-Packard

Title-Subject: [Microscopy] [Filtered] MListserver: EDS Detector available for donation

Question: We have an older Oxford EDS detector from a decomissioned ESEM 2020 WITHOUT the computer/electronics that's available for donation (qualified group). It's model is 6807 10mm2 ATW1 with a retrograde angle of incline - specific to ESEM 2020. In working order when we pulled it off the tool ~ 2 years ago. Let me know offline if you are interested in it. Would need to pay shipping. Thanks.

Nancy Phillips
Hewlett-Packard
nancy_phillips-at-hp.com

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From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 06:00:03 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (juan-at-nanostellar.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, June 24, 2004 at 16:45:25
---------------------------------------------------------------------------

Email: juan-at-nanostellar.com
Name: Juan

Title-Subject: [Microscopy] [Filtered] software for nano-particle shape analysis

Question: Dear all,

We need to do shape-resolved nano-particle size analysis. For examples, TEM images show triangles, squares, pentagons..., and we would like to know if there is any software which can automatically recognize the shape and give the size of them.

Any suggestion would be appreciated. Thanks.

Juan

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From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 06:04:59 2004

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Hi for all !
I have big problem with this operation BINXFER in the qbasic for quantimet
570 color,

I have binary image, in the window "field measurement" we have a good data
for count,
when we have program in qbasic "test-c. qba" we need use image analysis
comand BINXFER with function "paralysis" to obtain a good data for count
I have problem with this function; you see now this program;
10 rem feature count test-c.qba
20 rem calibrate - pixel=1
30 cls
40 clearplane -1
50 mframe 31 61 450 450
60 iframe 0 0 512 512
70 display 0 0 3 6
80 loadbin 1 '1.bin'
90 binxfer 1 0 2 5 0 0 0 rem problem with paralysed not working !!
100 measfield 2
110 rfieldres fieldarray(1)
120 area=fieldarray(1)
130 perimeter=fieldarray(2)
140 count=fieldarray(5)
150 rem postext 5 10
160 print "area - " area
170 print "perimeter - " perimeter
180 print "count - " count
190 stop
200 end

when in the line 100 i give 100 measfield 1 program computing count for all
end !!!

How use this function BINXFER correct to obtain good data mesurements for
count ?

best regards

Chris Hübner

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 09:58:18 2004

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Hi,

Here's a question that goes back into the dim past. I need to make a
small front surface mirror. I have the blank glass, and I thought
that I would use my old em training and evaporate some chromium chips
onto the surface, in a Denton Vacuum Evaporator, model DV-515.
However, I can't find tungsten baskets anywhere in the lab. We do
have lots of carbon rods, and I am wondering if any of you have ever
used such rods to evaporate the chromium. I've done it with Pt, of
course.

Thanks,

Joel

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 11:32:38 2004

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Has anyone done, or has anyone seen done, microwave enhanced
immunohistochemistry on cell cultures using alkaline phosphatase secondary
antibody. So far I have been able to find only preliminary treatment with
microwave for antigen retrieval. Any info will be greatly appreciated.

Greg Erdos

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 12:53:32 2004

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I was asked to use ethylene glycol for TEM specimen preparation:
as a dehydration fluid, a fixative, in a boat of diamond knife, and
a solvent for stain. Any comments and advise are greatly
apprciated.

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 13:05:00 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (lbustillos-at-amalab.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, June 25, 2004 at 08:44:42
---------------------------------------------------------------------------

Email: lbustillos-at-amalab.com
Name: Luis Bustillos

Title-Subject: [Microscopy] [Filtered] MListserver: Microscope keeps shutting itself off.

Question: We are having a puzzling problem with our JEOL 100CX II. It shuts itself off sometimes after 1-2 hours but sometimes it will run a day or two before it will eventually shut itself off. We have checked all that we could think of that could be causing the problem. For example, the water circulation, air pressure, heating plates, fore pump sensors, exchanged the whole vacuum board, checked the input voltage but to no avail. I would really appreciate it if anybody has any suggestions.

Lou

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From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 13:05:52 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (satyam-at-iopb.res.in) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, June 25, 2004 at 09:28:08
---------------------------------------------------------------------------

Email: satyam-at-iopb.res.in
Name: P. V. Satyam

Organization: Institute of Physics, Bhubaneswar, India

Title-Subject: [Microscopy] [Filtered] MListserver: Thermostat for JEOL 2010 TEM

Question: Hello friends,
I need a help in finding out the following thermostat to get the for our recently purchased TEM machine (JEOL 2010, UHR).

THERMOSTAT
PART NO. - 440001765
50'C OFF AND 35'C ON
USED IN LENS PS CKT. BOARD.

At present I am in Japan. I will be going back to my Institute in India, where our machine requires this thermostat (on July 3rd). But, I can't purchase directly from JEOL due to their policies. We need the above item as soon as possible. I need to go back and import from them eventhough it is a small item!

I plan to visit Akihabara, Tokyo in another couple of days for this purpose. Please suggest.

I am willing to pay for these,If some one wants to ship them. We need very urgently.

What are the other sources where I can get the above thermostat?

Thanks in advance.

Satyam

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From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 14:30:44 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (stephanie.l.mccracken-at-medtronic.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, June 25, 2004 at 14:23:57
---------------------------------------------------------------------------

Email: stephanie.l.mccracken-at-medtronic.com
Name: Stephanie McCracken

Title-Subject: [Microscopy] [Filtered] BeCu X-section labs?

Question: Is anyone aware of contract labs that perform BeCu Cross-sections? I am interested in contracting this to avoid having to deal with the Health and Safety Issues.

Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 14:34:28 2004

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On Jun 25, 2004, at 11:19 AM, Dusevich, Vladimir wrote:

} I was asked to use ethylene glycol for TEM specimen preparation:
} as a dehydration fluid, a fixative, in a boat of diamond knife, and
} a solvent for stain. Any comments and advise are greatly
} apprciated.
}
Dear Vladimir,
I wouldn't use ethylene glycol either for a dehydrating agent--it is
completely miscible with water, so it wouldn't extract it--or a
fixative--it preserves many proteins as do other polyalcohols, e.g.
sucrose. On the other hand, it might work well as a fluid in the boat
of a diamond knife--I've never used it that way, but sections should
float and not be damaged--and it could be a good solvent for some
stains, although it is quite hydrophyllic.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jun 25 17:02:37 2004

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Free or low price. I only need parts.Any information
would be great help.
Thanks.

Tim

__________________________________________________
Do You Yahoo!?
Tired of spam? Yahoo! Mail has the best spam protection around
http://mail.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Sat Jun 26 17:29:06 2004

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Luis,
I would suggest you check the freon presure for EHT.

Long Li
____________________________________________________________________________
_________
Materials Science and Engineering Department
University of Pittsburgh
3700 O'Hara St., 848 Benedum Hall
Pittsburgh, PA 15261

Tel: (412) 624-9753
FAX: (412) 624-8069
e-mail: Lil2-at-pitt.edu
longli_tem-at-hotmail.com

----- Original Message -----
} From: "by way of MicroscopyListserver" {lbustillos-at-amalab.com}
To: {microscopy-at-microscopy.com}
Sent: Friday, June 25, 2004 2:31 PM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (innap-at-savion.huji.ac.il) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, June 27, 2004 at 03:02:29
---------------------------------------------------------------------------

Email: innap-at-savion.huji.ac.il
Name: Inna Popov

Organization: The Hebrew University of Jerusalem

Title-Subject: [Microscopy] [Filtered] MListserver: software for simulation of CBED

Question: Dear All,

I am trying to use Convergent Beam Electron Diffraction for precise measurement of lattice parameter. Do you know any (either commercial or free) software which construct CBED patterns (high order Laue zones patterns)?
I would also deeply appreciate any recommendation regarding Software for constucting crystalline shapes (3D polygons) based on know Miller indexes.
Best,
Inna

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From MicroscopyL-request-at-ns.microscopy.com Sun Jun 27 09:39:21 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (saram-at-duke.edu) from http://microscopy.org/MicroscopyListserver/MLFormMail.html on Sunday, June 27, 2004 at 09:37:05
---------------------------------------------------------------------------

Email: saram-at-duke.edu
Name: Sara E. Miller

Organization: Duke

Title-Subject: [Microscopy] [Filtered] MListserver: Electron Microscopy Technologist Job

Question:
Electron Microscopy Technologist Job

I have an electron microscopy technologist position open. We do all TEM--a
mixture of negative staining and thin sectioning; 75% is clinical (diagnosing
viral diseases by EM plus surgical pathology EM) and 25% is research. We have
5 EM tech positions that rotate and perform various duties.

Requirements for the position include a bachelorÇs degree and electron
microscopy training (a course or experience) or an associateÇs degree in EM. I
am looking for someone who is proficient in cutting thin sections and has
experience running an electron microscope. I would like to have someone who
has done some negative staining and examination of viruses.

I am looking for a person who enjoys challenging and interesting cases, is
dedicated to accuracy, and is willing occasionally to put in extra effort in
return for appropriate compensation. I am particularly looking for someone
who can manage several jobs at once while having a good time sharing
camaraderie with the rest of us, i.e., is not high strung. I know this special
person exists, since there are 4 lovely folks remaining (3 guys and 1 gal) with
these same qualifications. I will be happy to answer any questions you have by
phone or email.

Durham, NC, is a pleasant place in which to live and work--3 hrs from the
mountains or the beach, and has more entertainment than you could want with 3
major universities and their arts programs in close proximity. Durham is one
of the apexes of a triangle formed by it, Raleigh, and Chapel Hill, each only
20-30 min apart. In the center of the triangle are numerous businesses that
comprise the Research Triangle Park, a huge research center with close ties to
the various universities in the 3 cities. Duke Medical Center is composed of a
medical school and a tertiary care hospital. Many basic and applied research
projects are underway. The medical center is adjacent to the undergraduate
campus where it has been rumored that basketball competition is fierce.

If you are interested, please contact me directly, off line.
Sincerely,

Sara E. Miller, Ph. D.
Director, Electron Microscopy Laboratory
Department of Pathology, Box 3712
Duke University Medical Center
Durham NC 27710
Phone: (919) 684-3452
Fax: (919) 684-3265
saram-at-duke.edu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 27 15:51:19 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On my JEOL 840A I have used RS #228-2636 Industrial Thermostat, much cheaper
than the JEOL type although a different shape (I hold it in place with a spring that
wraps around the diff pump). This one opens at 50 deg, closes at 35 deg.

But I prefer to use the type which needs to be manually reset, to avoid temperature
recycling ---- if there's a problem which overheats the DP I want to know about it.

RS # 228-2513 is their lowest, it opens at 70 deg.

However, you have to watch out that you don't invalidate any guarantees by using
non-JEOL parts.

cheers

rtch

Question: Hello friends,
I need a help in finding out the following thermostat to get the for
our recently purchased TEM machine (JEOL 2010, UHR).

THERMOSTAT
PART NO. - 440001765
50'C OFF AND 35'C ON
USED IN LENS PS CKT. BOARD.

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Sun Jun 27 17:26:48 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (subramss-at-email.uc.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Sunday, June 27, 2004 at 14:45:04
---------------------------------------------------------------------------

Email: subramss-at-email.uc.edu
Name: Jimble

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] ESEM imaging gases: Methane

Question: I am trying to find out more about using Methane as an
imaging gas in the ESEM and would appreciate the input of any of you
who may have used alternate gases for imaging in the ESEM.

Regards,

Jimble

Srinivas Subramaniam
Advanced Materials Characterization Center
University of Cincinnati

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 01:41:26 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello Inna,
At the recent school on CBED http://www.zmn.tu-ilmenau.de/cat74.html this topic was covered in detailes.
The program mbfit from Dr. K.Tsuda allows advanced dynamical (Bloch waves) calculation of CBED patterns, and it was free at least for school participants. There was a program as well (one of many, I believe) called Winkiku for kynematical calculations. We also demonstrated there a multislice based code for CBED calculation including HOLZ lines, however it is not yet ready for external users. But if you are facing the problems of lines splitting and symmetry breaks on you patterns, multislice is the only way to go and we are opened for cooperation.
There was also a program based on modified Hough transformation for precise HOLZ line position measurement, which you may find usefull and which is freeware. You may contact Dr Ute Kaiser at ute.kaiser-at-tu-ilmenau.de to get one.

Hope this helps
Andrey

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
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} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (innap-at-savion.huji.ac.il) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, June 27, 2004 at 03:02:29
} ---------------------------------------------------------------------------
}
} Email: innap-at-savion.huji.ac.il
} Name: Inna Popov
}
} Organization: The Hebrew University of Jerusalem
}
} Title-Subject: [Microscopy] [Filtered] MListserver: software for simulation of CBED
}
} Question: Dear All,
}
} I am trying to use Convergent Beam Electron Diffraction for precise measurement of lattice parameter. Do you know any (either commercial or free) software which construct CBED patterns (high order Laue zones patterns)?
} I would also deeply appreciate any recommendation regarding Software for constucting crystalline shapes (3D polygons) based on know Miller indexes.
} Best,
} Inna
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 02:32:23 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Joel,

I am not sure that vacuum evaporation of chromium from carbon is a good
idea. I have never heard of that being done, even for such "macro"
applications as mirror coating.
Have you considered using aluminium metal instead for your
front-surfaced mirror? It might be easier in your case. For that you
would not need a tungsten basket, but simply a tungsten wire with a
v-notch kink in it. Perhaps you can find (or make) some of these?
The aluminium can be simply a small area of household foil which you can
hang over the v-kink and melt to a blob under vacuum beforehand,
although even this may be unnecessary. To prevent larger contaminant
particles from falling on the mirror surface you might be wise to
support it somehow so that it is not directly under the evaporation
source.
Good luck with your evaporation!

Jim

-----Original Message-----
} From: Joel Sheffield [mailto:jbs-at-temple.edu]
Sent: Friday, June 25, 2004 5:26 PM
To: Microscopy-at-MSA.Microscopy.Com

Hi,

Here's a question that goes back into the dim past. I need to make a
small front surface mirror. I have the blank glass, and I thought
that I would use my old em training and evaporate some chromium chips
onto the surface, in a Denton Vacuum Evaporator, model DV-515.
However, I can't find tungsten baskets anywhere in the lab. We do
have lots of carbon rods, and I am wondering if any of you have ever
used such rods to evaporate the chromium. I've done it with Pt, of
course.

Thanks,

Joel

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 06:21:32 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Jimble -

I'm afraid I can't help much with your question: in our ESEM we've
ever only used water vapour, or HV mode. But I'm curious - is there some
particular reason why you want to use methane? Would it have an advantage
over water vapour, or are you especially interested in observing a
particular reaction in a methane environment?
Also, of course, there's the small matter of a chamber full of
methane being exposed to a spark from, say, a stage drive motor. I suppose
once you had a partial pressure of only a couple torr of methane in there it
would be safe enough, but I'm wondering about the early evacuation stages,
when there could still be enough oxygen in the chamber to get a sudden and
highly unpleasant reaction going. (Maybe I'm a bit paranoid - here in Nova
Scotia we lost 26 coal miners in a methane explosion a few years back).
Anyway, good luck, but be careful with that stuff......

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: subramss-at-email.uc.edu [mailto:subramss-at-email.uc.edu]
Sent: Sunday, June 27, 2004 7:57 PM
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (subramss-at-email.uc.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Sunday, June 27, 2004 at 14:45:04
---------------------------------------------------------------------------

Email: subramss-at-email.uc.edu
Name: Jimble

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] ESEM imaging gases: Methane

Question: I am trying to find out more about using Methane as an
imaging gas in the ESEM and would appreciate the input of any of you
who may have used alternate gases for imaging in the ESEM.

Regards,

Jimble

Srinivas Subramaniam
Advanced Materials Characterization Center
University of Cincinnati

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 06:55:25 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

IF THIS ISN'T COMMERCIAL ADVERTISING
THEN WHAT IS, THIS KIND OF REPLY
SHOULD BE OFF LINE, WE'RE SURE HOPE IT
WAS INADVERTANT, NEVER THE LESS IT
IS ADVERTISING.
----- Original Message -----
} From: {ramos-at-argo-tech.com}
To: {Microscopy-at-MSA.Microscopy.com}
Sent: Tuesday, June 15, 2004 2:41 PM

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (tem_iopb-at-iopb.res.in) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday,
June 28, 2004 at 02:14:54
---------------------------------------------------------------------------

Email: tem_iopb-at-iopb.res.in
Name: P. V. Satyam

Organization: Institute of Physics

Title-Subject: [Microscopy] [Filtered] MListserver: Thermostat : JEOL Help

Question: Dear Friends,

I posted the following help message few days back:
} } Question: Hello friends,
} } I need a help in finding out the following thermostat to get the
} } for our recently purchased TEM machine (JEOL 2010, UHR).
} }
} } THERMOSTAT
} } PART NO. - 440001765
} } 50'C OFF AND 35'C ON
} } USED IN LENS PS CKT. BOARD.
} }

This message is to thank you all who gave their suggestions. Also, I
would like to thank Mr. Takebe, Regional Sale Manager in JEOL, Japan
who has going all the way to help me in getting the component. He has
promised me to hand deliver the components at me personally (at
present I am near Tokyo). Initially I was rather not that confident;
But this gesture from JEOL to help when it is badly needed is highly
appreciative from my side. I was worried that it will take more time
to get it if I go back India and place an order and hence posted for
faster ways to cricumvent and find some new methods to solve the
problems in using thermostat.

Please note that this is just my experience which I am sharing. No
commercial interests are involved in this.

Best regards
Satyam

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 08:20:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Inna,
I invite you to try the online CBED simulation routines at:
http://emaps.mrl.uiuc.edu. This site provides an online interface to a
collection of diffraction and imaging simulation routines written by Prof.
Zuo of the University of Illinois through a web based user interface written
by Dr. Jim Mabon. Both kinematic and full Bloch wave simulations of CBED
patterns can be performed.
For more information, please see:
http://cmm.mrl.uiuc.edu/EMAPS/WebEmapsInfo.htm

Cheers,

Ray D. Twesten, PhD.
Center for Microanalysis of Materials
Seitz Materials Research Laboratory
104 S. Goodwin Ave., Urbana, IL 61801
+1 217 244-6177 (Fax -2278)

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:innap-at-savion.cc.huji.ac.il]
Sent: Sunday, June 27, 2004 10:04 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (innap-at-savion.huji.ac.il) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, June
27, 2004 at 03:02:29
---------------------------------------------------------------------------

Email: innap-at-savion.huji.ac.il
Name: Inna Popov

Organization: The Hebrew University of Jerusalem

Title-Subject: [Microscopy] [Filtered] MListserver: software for simulation
of CBED

Question: Dear All,

I am trying to use Convergent Beam Electron Diffraction for precise
measurement of lattice parameter. Do you know any (either commercial or
free) software which construct CBED patterns (high order Laue zones
patterns)?
I would also deeply appreciate any recommendation regarding Software for
constucting crystalline shapes (3D polygons) based on know Miller indexes.
Best,
Inna

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 08:20:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Frank,
It's the dilution of methane and oxygen you have to worry about (Excluding
burning metals, fluorine gas and so forth)
The ratio called explosive limits determine the hazard. Too much methane
or too little methane no explosion. On the plus side, methane is slightly
lighter than air, so as you vent the system you would not have to worry
about heavy vapors collecting in low spots creating suffocation traps and
explosive concentrations.

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

"Thomas,
Frank" To: "'subramss-at-email.uc.edu'" {subramss-at-email.uc.edu} ,
{FThomas-at-NRCan microscopy-at-ns.microscopy.com
.gc.ca} cc:
Subject: [Microscopy] RE: viaWWW: ESEM imaging gases: Methane
06/28/2004
08:20 AM

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Jimble -

I'm afraid I can't help much with your question: in our ESEM
we've
ever only used water vapour, or HV mode. But I'm curious - is there some
particular reason why you want to use methane? Would it have an advantage
over water vapour, or are you especially interested in observing a
particular reaction in a methane environment?
Also, of course, there's the small matter of a chamber full of
methane being exposed to a spark from, say, a stage drive motor. I suppose
once you had a partial pressure of only a couple torr of methane in there
it
would be safe enough, but I'm wondering about the early evacuation stages,
when there could still be enough oxygen in the chamber to get a sudden and
highly unpleasant reaction going. (Maybe I'm a bit paranoid - here in Nova
Scotia we lost 26 coal miners in a methane explosion a few years back).
Anyway, good luck, but be careful with that stuff......

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: subramss-at-email.uc.edu [mailto:subramss-at-email.uc.edu]
Sent: Sunday, June 27, 2004 7:57 PM
To: microscopy-at-ns.microscopy.com

---

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (subramss-at-email.uc.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Sunday, June 27, 2004 at 14:45:04
---------------------------------------------------------------------------

Email: subramss-at-email.uc.edu
Name: Jimble

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] ESEM imaging gases: Methane

Question: I am trying to find out more about using Methane as an
imaging gas in the ESEM and would appreciate the input of any of you
who may have used alternate gases for imaging in the ESEM.

Regards,

Jimble

Srinivas Subramaniam
Advanced Materials Characterization Center
University of Cincinnati

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 08:47:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I DON'T THINK THAT THIS IS ADVERTISING. THE
CLEMSON UNIVERSITY PERSON ASKED FOR HELP IN
LOCATING A REPLACEMENT SEM. RAMOS OFFERED A
SUGGESTED SOURCE. ADVERTISEMENT WOULD BE IF
THE ACTUAL SOURCE POSTED TO THE LIST DIRECTLY. THEY
DID NOT. USERS, INCLUDING MYSELF, ARE ALWAYS
SEEKING SOURCES. NO ONE CAN KNOW ALL OF THEM.

IF IT IS ADVERTISING, I'M SURE NESTOR WOULD
LET US AND THE POSTER KNOW. OR NESTOR WOULD NOT HAVE
ALLOWED THE POSTING.

GARY G.

At 06:24 AM 6/28/2004, you wrote:

} IF THIS ISN'T COMMERCIAL ADVERTISING
} THEN WHAT IS, THIS KIND OF REPLY
} SHOULD BE OFF LINE, WE'RE SURE HOPE IT
} WAS INADVERTANT, NEVER THE LESS IT
} IS ADVERTISING.
} ----- Original Message -----
} } From: {ramos-at-argo-tech.com}
} To: {Microscopy-at-MSA.Microscopy.com}
} Sent: Tuesday, June 15, 2004 2:41 PM
} Subject: [Microscopy] Re: Looking to buy SEM
}
}
}
} }
} }
} } Darryl,
} }
} }
} } Don't know anything about the company......but perhaps you might look into
} } SEMTech Solutions. They offer service for AMRAY SEMs, and also offer
} } Re-manufactured Pre-owned Scanning Electron Microscopes.
} }
} } http://www.semtechsolutions.com/
} }
} }
} } Kelly A. Ramos
} } Metallurgical Engineer / Supervisor
} } Argo-Tech Materials Laboratories
} } 23555 Euclid Avenue
} } Cleveland, OH 44117
} } 216-692-5904 or 216-692-5446
} } (fax) 216-692-5816
} } http://www.atclabs.com
} }
} }
} }
} } darryl krueger
} } {dkruege-at-CLEMS To:
} Microscopy-at-MSA.Microscopy.com
} } ON.EDU} cc:
} } Subject: [Microscopy]
} Looking to buy SEM
} } 06/14/04 03:30
} } PM
} }
} } Dear Listees,
} }
} } We're loosing our Hitachi 3500 SEM due to a split in the EM facility here
} } at Clemson University. Is there anything out there available, comparable
} } on a used basis. We're looking for equipment and a price. Thanks in
} } advance for any information.
} }
} } Darryl Krueger, RA
} } BioScience Dept.
} } Clemson University
} }
} }
} }
} }
} }
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:01:30 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Frank writes ...

} ... But I'm curious - is there some particular reason
} why you want to use methane? Would it have an advantage over
} water vapour, or are you especially interested in observing a
} particular reaction in a methane environment?

It is curious to note the fact methane is used as a quenching gas in
ionization-type detectors (e.g., x-ray argon gas flow detectors). The
methane molecule redily supplies the ionized argon cation with the electron
it needs for being immediately available for ionization again. I don't know
the physical chemistry of it, ... but, in a context of specimen charging,
the phenomenon does beg the question Jimble asks.

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

} Name: Jimble
}
} Organization: University of Cincinnati
}
} Title-Subject: [Microscopy] [Filtered] ESEM imaging gases: Methane
}
} Question: I am trying to find out more about using Methane as an
} imaging gas in the ESEM and would appreciate the input of any of you
} who may have used alternate gases for imaging in the ESEM.
}
} Regards,
}
} Jimble
}
} Srinivas Subramaniam
} Advanced Materials Characterization Center
} University of Cincinnati
}
} ------------------------------------------------------------------
} ---------
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:27:40 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear All:

A post-doctoral position is available starting immediately on
the characterization of nanoparticles by advanced scanning
transmission electron microscopy methods, such as quantitative
Z-contrast imaging, electron energy loss spectroscopy, as well as
high resolution electron microscopy. Experience with VG-STEM and
Z-contrast imaging is specially appreciated. This is part of a
collaborative program with University of Illinois at Urbana-Champaign
and Brookhaven National Labs, to predict and determine the
3-dimensional supported structure of nanoparticles utilized in
heterogeneous catalysis either as model systems or for water
purification for fundamental understanding of nano-catalytic
reactions.

To apply for this position, please send a resume with the
names and contact information for three references, or to obtain more
information, please contact:

Professor Judith Yang
848 Benedum Hall
Materials Science & Engineering Dept.
University of Pittsburgh
Pittsburgh, PA 15261

jyang-at-engr.pitt.edu
(412) 624-8613

_________________________________________________________________
MSN Toolbar provides one-click access to Hotmail from any Web page – FREE
download! http://toolbar.msn.click-url.com/go/onm00200413ave/direct/01/

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:32:46 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Listers,

Here I am at my new job and I get to clean out the old chemicals. I've
already found 17 year old ether, an unmarked bottle of who know what and
various other old chemicals.

My question today regards the propylene oxide. Does it age? Can it still
be used as an intermediate solvent if it's 24 (bottle dated 9/1980) or 12
(bottle dated 9/1992) years old?

If not I will discard it, if it just ages like a fine wine we'll use it.

I've looked at the MSDS's and can't find anything about age, stability and
usefulness.

So if you know the answer to my question, please let me know.

Is it a tasty wine or a nasty vinegar?

Cheers,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:26:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mark.nathanson-at-umdnj.edu) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday,
June 28, 2004 at 09:07:49
---------------------------------------------------------------------------

Email: mark.nathanson-at-umdnj.edu
Name: Mark Nathanson

Organization: New Jersey Medical School

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am trying to recondition an LKB Nova Ultramicrotome, but
we have no documentation. Is there anyone in the Phila-New York area
with an instruction maual or repair manuals that thyey would be
willing to share?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:40:06 2004

Contents Retrieved from Microscopy Listserver Archives
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At the partial pressure you are talking about I would not worry about
possible explosion unless the methane build up in any cold traps or in
the pumping system. Purging the chamber should mean that there is
pretty much just methane in the chamber and therefore no oxygen for it
to combine with!

--
John Mansfield PhD MInstP
North Campus Electron Microbeam Analysis Laboratory
417 SRB, University of Michigan
2455 Hayward, Ann Arbor MI 48109-2143 USA
Phone: (734) 936-3352 FAX (734) 763-2282
Cell. Phone: (734) 834-3913
(Leaving a phone message at 936-3352 is preferable to 834-3913)
Email: jfmjfm-at-engin.umich.edu
URL: http://emalwww.engin.umich.edu/people/jfmjfm/jfmjfm.html
Location: Lat. 42° 16' 48" Long. 83° 43' 48"
AIM: thejfmjfm

Home address:
4304 Spring Lake Boulevard
Ann Arbor MI 48108-9657
Phone (734) 994-3096

On Jun 28, 2004, at 7:50 AM, Thomas, Frank wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Jimble -
}
} I'm afraid I can't help much with your question: in our ESEM we've
} ever only used water vapour, or HV mode. But I'm curious - is there
} some
} particular reason why you want to use methane? Would it have an
} advantage
} over water vapour, or are you especially interested in observing a
} particular reaction in a methane environment?
} Also, of course, there's the small matter of a chamber full of
} methane being exposed to a spark from, say, a stage drive motor. I
} suppose
} once you had a partial pressure of only a couple torr of methane in
} there it
} would be safe enough, but I'm wondering about the early evacuation
} stages,
} when there could still be enough oxygen in the chamber to get a sudden
} and
} highly unpleasant reaction going. (Maybe I'm a bit paranoid - here in
} Nova
} Scotia we lost 26 coal miners in a methane explosion a few years back).
} Anyway, good luck, but be careful with that stuff......
}
} F.C. Thomas
} FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
} GSC Atlantic
} Natural Resources Canada, Bedford Institute of Oceanography,
} P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
} Ressources naturelles Canada, l'Institut Oceanographique du Bedford,
} B.P.
} 1006, Dartmouth, (Nouvelle-Ecosse)
} B2Y 4A2
} Government of Canada/Gouvernement du Canada
}
}
} -----Original Message-----
} } From: subramss-at-email.uc.edu [mailto:subramss-at-email.uc.edu]
} Sent: Sunday, June 27, 2004 7:57 PM
} To: microscopy-at-ns.microscopy.com
} Subject: [Microscopy] viaWWW: ESEM imaging gases: Methane
}
}
}
}
} -----------------------------------------------------------------------
} -----
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
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} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (subramss-at-email.uc.edu) from
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} -----------------------------------------------------------------------
} ----
}
} Email: subramss-at-email.uc.edu
} Name: Jimble
}
} Organization: University of Cincinnati
}
} Title-Subject: [Microscopy] [Filtered] ESEM imaging gases: Methane
}
} Question: I am trying to find out more about using Methane as an
} imaging gas in the ESEM and would appreciate the input of any of you
} who may have used alternate gases for imaging in the ESEM.
}
} Regards,
}
} Jimble
}
} Srinivas Subramaniam
} Advanced Materials Characterization Center
} University of Cincinnati
}
} -----------------------------------------------------------------------
} ----
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:39:27 2004

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Dear All:
A post-doctoral position is available starting immediately on
the characterization of nanoparticles by advanced scanning
transmission electron microscopy methods, such as quantitative
Z-contrast imaging, electron energy loss spectroscopy, as well as
high resolution electron microscopy. Experience with VG-STEM and
Z-contrast imaging is specially appreciated. This is part of a
collaborative program with University of Illinois at Urbana-Champaign
and Brookhaven National Labs, to predict and determine the
3-dimensional supported structure of nanoparticles utilized in
heterogeneous catalysis either as model systems or for water
purification for fundamental understanding of nano-catalytic
reactions.
To apply for this position, please send a resume with the
names and contact information for three references, or to obtain more
information, please contact:
Professor Judith Yang
848 Benedum Hall
Materials Science & Engineering Dept.
University of Pittsburgh
Pittsburgh, PA 15261
jyang-at-engr.pitt.edu
(412) 624-8613

_________________________________________________________________
Make the most of your family vacation with tips from the MSN Family Travel
Guide! http://dollar.msn.com

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 09:56:12 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear All:

A post-doctoral position is available starting immediately on
the characterization of nanoparticles by advanced scanning
transmission electron microscopy methods, such as quantitative
Z-contrast imaging, electron energy loss spectroscopy, as well as
high resolution electron microscopy. Experience with VG-STEM and
Z-contrast imaging is specially appreciated. This is part of a
collaborative program with University of Illinois at Urbana-Champaign
and Brookhaven National Labs, to predict and determine the
3-dimensional supported structure of nanoparticles utilized in
heterogeneous catalysis either as model systems or for water
purification for fundamental understanding of nano-catalytic
reactions.

To apply for this position, please send a resume with the
names and contact information for three references, or to obtain more
information, please contact:

Professor Judith Yang
848 Benedum Hall
Materials Science & Engineering Dept.
University of Pittsburgh
Pittsburgh, PA 15261

jyang-at-engr.pitt.edu
(412) 624-8613

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 11:12:51 2004

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Hello,
We have just sent an Electroscan E3 ESEM to UC Berkeley's Salvage. UC
Berkeley people have first crack at it, then other UC people, and then
finally other organizations.

It was in a functioning state when decommissioned. You'll need a rotary
pump, and water chiller to make it fully functional I think.

For information about obtaining it, you'll need to contact UC Berkeley's
salvage department at:

http://www-propmgmt.bsrvm.berkeley.edu/excess/intro.htm

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

On Fri, 25 Jun 2004, jiahe xu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Free or low price. I only need parts.Any information
} would be great help.
} Thanks.
}
} Tim
}
}
} __________________________________________________
} Do You Yahoo!?
} Tired of spam? Yahoo! Mail has the best spam protection around
} http://mail.yahoo.com
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 14:03:39 2004

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Some reagents, unlike wine, undergo minimal change with time. Low MW
solvents (ethanol, acetone, propylene oxide) should be OK if they are
unopened and sealed tightly. About the only concern would be
evaporative loss which would lead to cooling and possible
condensation of water in the solvent. In that case, pass them along
to someone who could use them for cleaning purposes, etc.

We have even successfully used unopened, original Epon (yes, a truly
fine, 30 yr old vintage stored in a dark and cool environment) with
no problems. However, the additional components (DDSA, NMA, BDMA were
fresh reagents).

JB

} Here I am at my new job and I get to clean out the old chemicals. I've
} already found 17 year old ether, an unmarked bottle of who know what and
} various other old chemicals.
}
} My question today regards the propylene oxide. Does it age? Can it still
} be used as an intermediate solvent if it's 24 (bottle dated 9/1980) or 12
} (bottle dated 9/1992) years old?
}
} If not I will discard it, if it just ages like a fine wine we'll use it.
}
} I've looked at the MSDS's and can't find anything about age, stability and
} usefulness.
}
} So if you know the answer to my question, please let me know.
}
} Is it a tasty wine or a nasty vinegar?
}
}
} Cheers,
}
} Paula :-)
}
} Paula Sicurello
} EM Lab
} 106 Mills Godwin Sciences Building
} Old Dominion University
} Norfolk, VA 23529
} USA
} 757-683-3822

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 15:38:18 2004

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I disagree.

Kelly said he didn't know anything about the company, didn't he?

Mentioning a company name isn't advertising.

Let's not get so PC that we can't make recommendations to each other on the list.

cheers

rtch

ps Kelly also was polite in that he said who he is and where he's from, and that he didn't
shout

} From: "JERRY SMITH" {jsmit51-at-tampabay.rr.com}
To: {ramos-at-argo-tech.com} , {Microscopy-at-MSA.Microscopy.com}

Hi,

For those interested in microscopy education
and/or lattice fringe imaging, we've put together a
collection of web-explorable models* for general
access. The lion's share of those on the main menu
are for prospective nanoworld explorers to "do
detective work" with, e.g. to measure sizes, angles,
perhaps even Fourier analyze, and then practice
reporting on their results.

The visibilitymaps link, via "More here", leads
to a collection of research-relevant but similarly
interactive 3D maps** of visible lattice fringe
geometry for various specimen thicknesses and
microscope resolutions ala Ultramicroscopy 94
(2003) 245 and subsequent MSA papers***. We'll
eventually set up through webMathematica to host
user-requested plots.

Meanwhile, if you're contemplating analysis
of fringe images from a particular crystal type,
feel free to drop me a line (off the listserver,
specifying effective scope resolution and crystal
thickness as well) to see if we can manage to
post the model you'd like on request.

Cheers. /phil

* http://www.umsl.edu/~fraundor/nanowrld/live3Dmodels/default.htm
** http://www.umsl.edu/~fraundor/nanowrld/live3Dmodels/vmapframe.htm
*** http://www.umsl.edu/~fraundor/help/imagnxtl.htm

Phil Fraundorf
UM-StL Physics & Astronomy/CME
Washington U. Physics/MCSS
office: (314)516-5044
lab: (314)516-5024
http://www.umsl.edu/~fraundor

From MicroscopyL-request-at-ns.microscopy.com Mon Jun 28 19:12:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear All:

I am in the final evaluation process for the purchase of new optical
brightfield microscopes . They will be used for general biology,
embryology, and histology.

Can anyone give me their opinion off the server about the Zeiss Axiostar
Plus and the Nikon E200? Thank you for your assistance.

Ken
_______________________________________
Kenneth L. Tiekotter, Adjunct Professor
The University of Portland
Department of Biology
5000 N Willamette Blvd.
Portland, OR 97203 USA

Tel.: 503.493.8861

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 05:31:55 2004

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Paula,
I hope you're very careful with the old ether. As I understand it, the
stuff ages and becomes VERY unstable. I heard about a 5 gallon can that
was found in Woods Hole, MA. Required a bomb squad and resulted in a
big fine for the lab head.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

Paula Sicurello wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 05:49:19 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Lou,
I haven't seen any replies to your question, so I'll give it a shot.

I only work on SEMs, so I'm not familiar with the plumbing on the 100CX,
but on the JSM-840 and 6400, JEOL splits the water supply and sends one
feed the the Optics console and the other feed to the Electronics
console. When they exit their respective cooling loops they are
recombined so there is no way to tell if one or the other has a
restriction. A single flow meter may say the you have the correct flow,
but half of the system may be starved. This is sometimes caused by the
quick connect fittings getting old and the internal check valves closing
while the coupler is in the correct position.

What I have done on several systems is to put a flowmeter on each feed
and run half the water through each. If a blockage occurs on one leg,
it will be apparent on the respective flowmeter. One quick solution to
the blockage is to remove the check valve from the offending connector
until you can get a new connector.

Ken Converse
owner
Quality Images
third party SEM service
Delta, PA

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 06:44:58 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear MSA netters,

we need for an rather old Philips EM 420 the two-piece plate holders.
The format is 9.2cm x 11.2cm (eq. 3.6" x 4.4"). The insert is for the
8cm x 10cm (3.2" x 3.9") negative format. Please let me know if you
know anybody who has some of this holders in stock or wants to
get rid of his used ones.

Please contact me offline. Thank you in advance.

Andreas

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 06:52:37 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Listers,

Thanks to all who expressed concern over my 17 year old ether. It was in a
metal can and I called our Safety people as soon as I saw the age. The
safety person said that ether forms less peroxides in metal than in
glass-which is a good thing because I was moving that can all over the
place before I saw what it was. Then I had to move it again to try and
find a date on the can (the only label was an expiration date).

Let this be a reminder to all to put "date received" labels on all bottles
and cans of reagents and chemicals. Later down the line someone might need
to now the age of the stuff after inheriting it.

Once again Thanks for the concern-my ether did not go BOOM. Yippee!

I'll probably find some old really wet picric acid next.

Back to finding more old chemicals,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 07:50:11 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I had a similar problem with my old 100CXII. It's been a while, but I can
tell you a couple of things that went wrong towards the end. I seem to
remember that my mysterious shut-down was related to a big breaker in the HT
unit. If memory serves, this breaker is the main power switch for the HT
and is located on the left side facing the front of the unit. I replaced it
and the shut-downs stopped. My assumption is that over time the contacts
weakened and it would begin to get hot, then kick out. Another problem was
that the pneumatic valve blocks located under the left console began to
develop slow leaks. I fixed a couple of them, but eventually they all began
to fail. Replacement parts arrive 6 months after being ordered as they had
to come on special order from Japan, but by then I had replaced the
microscope.
Hope this helps

Dr Robert Simmons
Program Director
Biological Imaging Core Laboratory
Georgia State University
Atlanta, GA 30302-4010

404-651-3138
404-651-2509 FAX

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 08:27:20 2004

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Hi Darryl,

My job and EM lab were eliminated. My servicemen knew that my lab was
being eliminated, if I still wanted to work in EM, and knew the condition
of my TEM, SEM, image analyzer, and microtome. They knew I had them
rebuild the whole vacuum system within the last two years on the TEM and
the care it got over the years. Servicemen can be a networking resource
for you. Here's why.

Servicemen know who's lab is being closed or down sized, who's thinking of
upgrading their equipment, and who is actually upgrading. Even if the lab
also has some other manufacturer's equipment, they are usually told what is
happening with that total lab setup. Just ask them if they can help you in
your search.

Contact the salesmen with any manufacturer. If a customer knows the
salesman has a buyer for his used equipment being replaced, then the
salesman can use that to close a deal on a new piece of equipment from him.
The salesman wins, you win, the seller wins, and the manufacturer wins.
Be sure to ask the serviceman what the condition of the equipment is and
for some service reports for the last two years or so. Ask if the
equipment was serviced by factory people under a factory contract or under
insurance that used factory people.

Also, some industrial companies will donate their used equipment to a
university. If the thing is not any good, it will usually be dumpstered.
If it is still good equipment, they will try to donate it and take a tax
write-off. This 'free stuff' might be a bit too old for you. In that
case, you have to pay for something newer.

If a company does not want to fund an SEM lab anymore, you can make an
offer to take it off their hands as a donation. In exchange, you can offer
to let them use their old scope for a specified number of hours using their
own microscopist. This was done at a local university near me through the
serviceman. He got them together with a company I didn't even know had a
microscope.

There are a lot of options out there in addition to buying an SEM on the
open market. Hopefully, someone will read this and contact you about a
donation or a good SEM you can buy used.

Paul Beauregard
Senior Research Associate

} From: darryl krueger {dkruege-at-CLEMSON.EDU}
To: Microscopy-at-MSA.Microscopy.com
cc:

} Research Position in Characterization of Boron Carbide
}
}
}
} The primary aim of the project is to understand the root cause of
} the dramatic failure of B4C at pressures near 20GPa. The project
} will deal with carrying out thorough characterization of existing
} Boron Carbides and derivatives using analytical techniques such as
} high resolution transmission electron microscopy with electron
} energy loss spectroscopy, Raman spectroscopy, Nuclear Magnetic
} Resonance etc. in order to correlate the elastic modulus and
} hardness to the microstructure. In addition, the collapse of the
} crystal structure will be investigated theoretically using first
} principle calculations. Specifically, we will design a stable B4C
} crystal based on crystallographic and spectroscopic data available
} in the literature. The changes in the crystal structure will then be
} monitored while being subjected to various stresses below and above
} the threshold impact pressure of B4C. The calculations will provide
} a link from the atomistic level to the micro-structural level. The
} theoretical study could shed light on whether the poor ballistic
} performance above the threshold impact pressure is an intrinsic
} property of B4C.
}
}
}
} The successful candidate should have a strong background in
} characterization of materials using transmission electron
} microscopy. A thorough understanding of microstructure and
} crystallography of ceramic materials is essential. Applicants are
} requested to contact Prof. Manish Chhowalla, Rutgers University,
} Ceramic and Materials Engineering, 607 Taylor Road, Piscataway, NJ
} 08854. Email:
} {mailto:manish1-at-rci.rutgers.edu} manish1-at-rci.rutgers.edu. Phone:
} 732-445-5619

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 10:08:22 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

I agree with Robert. Our 100CX developed leaks in the gang of air pressure valves next to the HT tank. The JEOL service technician was able to rebuild them and that fixed the problem.

Randall Massey
Operations Manager
UW-Electron Microscope Facility
1300 University Ave.
Madison, WI 53706
voice (608)262-2993
Fax (608)262-7306

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 10:17:23 2004

Contents Retrieved from Microscopy Listserver Archives
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For any IC folks out there, I'm wondering if
anyone can explain what I believe is highly
amorphous ILD at vias in single and dual
damascene ICs? Relevant pix can be seen at:

http://www.microtechnics.com/ild1.jpg

http://www.microtechnics.com/ild2.jpg

Picture 2 shows cratering in the open areas
but both pix show massive opening at the via.
I attribute this to the ILD being more
amorphous at the via. But why? Or is
something else going on?

Etching is wet chemistry. Mag is about 60KX.

Thanks for any inputs.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 10:20:42 2004

Contents Retrieved from Microscopy Listserver Archives
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It's not the wet picric that should worry you. Picric
is explosive when dry! I perform monthly checks on my
picric acid to make sure it's hydrated.

Stu Smalinskas
Metallurgist
SKF USA
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Paula wrote:

Hi Listers,

Thanks to all who expressed concern over my 17 year
old ether. It was in a
metal can and I called our Safety people as soon as I
saw the age. The
safety person said that ether forms less peroxides in
metal than in
glass-which is a good thing because I was moving that
can all over the
place before I saw what it was. Then I had to move it
again to try and
find a date on the can (the only label was an
expiration date).

Let this be a reminder to all to put "date received"
labels on all bottles
and cans of reagents and chemicals. Later down the
line someone might need
to now the age of the stuff after inheriting it.

Once again Thanks for the concern-my ether did not go
BOOM. Yippee!

I'll probably find some old really wet picric acid
next.

Back to finding more old chemicals,

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

__________________________________
Do you Yahoo!?
Yahoo! Mail - 50x more storage than other providers!
http://promotions.yahoo.com/new_mail

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 10:28:33 2004

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Call me please. I am used to be a service engineer
for JEOL.

Tim
301-405-5244

--- Long Li {longli_tem-at-hotmail.com} wrote:
}
}
}
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} Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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}
-------------------------------------------------------------------------------
}
} Luis,
} I would suggest you check the freon presure for EHT.
}
}
}
}
}
} Long Li
}
____________________________________________________________________________
} _________
} Materials Science and Engineering Department
} University of Pittsburgh
} 3700 O'Hara St., 848 Benedum Hall
} Pittsburgh, PA 15261
}
} Tel: (412) 624-9753
} FAX: (412) 624-8069
} e-mail: Lil2-at-pitt.edu
} longli_tem-at-hotmail.com
}
}
}
}
} ----- Original Message -----
} } From: "by way of MicroscopyListserver"
} {lbustillos-at-amalab.com}
} To: {microscopy-at-microscopy.com}
} Sent: Friday, June 25, 2004 2:31 PM
} Subject: [Microscopy] viaWWW: Microscope keeps
} shutting itself off.
}
}
} }
} }
} }
}
--------------------------------------------------------------------------
} ----
} } The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
}
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} }
}
--------------------------------------------------------------------------
} -----
} }
} } Below is the result of your feedback form
} (NJZFM-ultra-55). It was
} submitted by (lbustillos-at-amalab.com) from
}
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html
} on
} Friday, June 25, 2004 at 08:44:42
} }
}
--------------------------------------------------------------------------
} -
} }
} } Email: lbustillos-at-amalab.com
} } Name: Luis Bustillos
} }
} } Title-Subject: [Microscopy] [Filtered]
} MListserver: Microscope keeps
} shutting itself off.
} }
} } Question: We are having a puzzling problem with
} our JEOL 100CX II. It
} shuts itself off sometimes after 1-2 hours but
} sometimes it will run a day
} or two before it will eventually shut itself off.
} We have checked all that
} we could think of that could be causing the problem.
} For example, the water
} circulation, air pressure, heating plates, fore pump
} sensors, exchanged the
} whole vacuum board, checked the input voltage but to
} no avail. I would
} really appreciate it if anybody has any suggestions.
} }
} } Lou
} }
} }
}
--------------------------------------------------------------------------
} -
} }
} }
}
}

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From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 10:41:28 2004

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Dear listers,

We will be studying changes in mitochondrial morphology after drug
application to cell monolayers. I have reviewed the listings in the
archives from few years ago regarding effects of osmolarity and choices of
buffer and fixative on muscle mitochondria. I would think that
mitochondria in cell monolayers would be particularly sensitive to these
factors.

I am condidering fixing the monolayers in 2.5 % glutaraldehyde in serum
free medium in an effort to maintain physiological conditions up to the
moment of fixation. Then, what about rinses before going into osmium?

Can anyone offer any pointers regarding preservation of mitochondrial
morphology in cell monolayers?

Thanks,
Dotty

Dorothy Sorenson
Microscopy and Image Analysis Laboratory
Department of Cell and Developmental Biology
University of Michigan Medical School
4643 Medical Science Building II
1301 Catherine
Ann Arbor, MI 48109-0616

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 12:43:05 2004

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When cells are cryo-fixed (metal mirror or high pressure freezing), the
mitochondria can have a very different morphology than after chemical
fixation. I remember an ancient paper from the 80's which looked at the
morphology of isolated mitochondria cryo-fixed before and after exposure to
an uncoupling agent. the uncoupled cryo-fixed mitochondria had an
appearance similar to chemically fixed ones while the coupled ones were
more compact and therefore denser. sorry I can't remember the actual
citation. but the bottom line is that I think any attempt to see subtle
drug effects on mitochondrial morphology after chemical fixation is suspect.

At 12:11 PM 06/29/04 -0400, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 14:27:52 2004

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Good afternoon,

I've been attempting to make gold-conjugated antibodies and I've had varying
degrees of success. I'm currently working with 1.4nm Nanogold, 2nm and 5nm
colloidal gold from various vendors. I believe each conjugate is made
correctly, but my methods for purifying and concentrating the 1.4nm and 2nm
products are not adequate. Depending upon the conjugate, the samples are
unrecoverable from the centricon or ultracentrifuge tube.

I'm figuring that my centrifuge conditions are not appropriate and that the
Nanogold may be binding irreversibly to the centricon membrane. The protocols
supplied by the colloidal gold vendors do not give sufficient details and my
efforts to extrapolate the speed at which to spin the 2nm conjugates have not
worked as of yet. I would appreciate any input or experience that one could
share. Feel free to contact me using the email address below.

Thanks in advance,
Henry

--
Henry C. Grisé
grise-at-bio.fsu.edu
Biology Graduate Student
Florida State University
Tallahassee, FL 32306

From MicroscopyL-request-at-ns.microscopy.com Tue Jun 29 16:06:25 2004

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I agree with Tom on this one. How will you know if all of the
mitochondria in one cell are doing the same thing at the same time (and
thus equally sensitive to the drug and giving you a valid measurement of
its effects) ? You won't! I think subtle changes would be better tracked
via biochemistry. Huge changes might be another matter but even then I
think you will need to do some stereology to validate what ever you see.

Geoff

Tom Phillips wrote:

} When cells are cryo-fixed (metal mirror or high pressure freezing),
} the mitochondria can have a very different morphology than after
} chemical fixation. I remember an ancient paper from the 80's which
} looked at the morphology of isolated mitochondria cryo-fixed before
} and after exposure to an uncoupling agent. the uncoupled cryo-fixed
} mitochondria had an appearance similar to chemically fixed ones while
} the coupled ones were more compact and therefore denser. sorry I
} can't remember the actual citation. but the bottom line is that I
} think any attempt to see subtle drug effects on mitochondrial
} morphology after chemical fixation is suspect.
}
} At 12:11 PM 06/29/04 -0400, you wrote:
}
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } Dear listers,
} }
} } We will be studying changes in mitochondrial morphology after drug
} } application to cell monolayers. I have reviewed the listings in the
} } archives from few years ago regarding effects of osmolarity and
} } choices of buffer and fixative on muscle mitochondria. I would think
} } that mitochondria in cell monolayers would be particularly sensitive
} } to these factors.
} }
} } I am condidering fixing the monolayers in 2.5 % glutaraldehyde in
} } serum free medium in an effort to maintain physiological conditions
} } up to the moment of fixation. Then, what about rinses before going
} } into osmium?
} }
} } Can anyone offer any pointers regarding preservation of mitochondrial
} } morphology in cell monolayers?
} }
} } Thanks,
} } Dotty
} }
} } Dorothy Sorenson
} } Microscopy and Image Analysis Laboratory
} } Department of Cell and Developmental Biology
} } University of Michigan Medical School
} } 4643 Medical Science Building II
} } 1301 Catherine
} } Ann Arbor, MI 48109-0616
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 02:23:30 2004

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Hi,
we are working up an animal model of allergic rhinitis and currently
favour the guinea-pig. Conventional toluidine blue works great on other
species but hardly demonstrates them at all in the g-p. The best I've
acheived is with a Luna's method, does any-one have any good working
methods tinctorial or IHC (we have not found an antibody to work yet)? It
has been suggested that I do some TEM but am loathe to go there as I
suspect the mast cell ultrastructure is also different to other species
(and hence the lack of histochemistry). This is making life extremely
difficult as the degranulation of mast cells is crucial

Histopathology Group
Asthma and Allergy Disease Biology
ri- CEDD.
GlaxoSmithKline Medicines Research Centre,
Gunnelswood Road,
STEVENAGE,
Hertfordshire.
SG1 2NY
tel. +44 (0)1438 764119
fax. +44 (0)1438 764782
email. gillian.2.brown-at-gsk.com

http://ukdiscovery.gsk.com/histopathology/default.htm

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 05:30:46 2004

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Hi

Are you working in wax or resin?

You could try periodic acid Schiff as a general starting point and then try
Alcian Blue (pH 2.5 and pH1.0) and also aldehyde fuchsin. Have you tried an
antibody to mast cell tryptase.

Gareth
Med vänliga hälsningar/With best regards

Gareth

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 08:36:21 2004

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Below is the result of your feedback form
(NJZFM-ultra-55). It was submitted by
(rpowell-at-nanoprobes.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html
on Tuesday, June 29, 2004 at 18:13:44
---------------------------------------------------------------------------

Email: rpowell-at-nanoprobes.com
Name: Rick Powell

Organization: Nanoprobes, Incorporated

Title-Subject: [Microscopy] [Filtered] MListserver: Re:
Gold conjugated IgG and Fab'

Question: (Vendor reply)

Hello Henry:

We manufacture NanogoldĆ conjugates, and often
begin the purification of IgG and Fab' fragments
by Centricon membrane centrifugation. The
conditions we usually use are a 30,000 MW cutoff
membrane ("Centricon-30"); the conjugate is
dissolved in reaction buffer, usually
phosphate-buffered saline at pH 6.5 or 7.5
depending on whcih type of Nanogold you used (one
to a few mL). We usually use a 6,000 g filtration
for 20 minutes, then invert, and extract into the
caps at 3,000 g for two minutes.

Some preps are more "sticky" than others; if this
is a problem (you can often tell because the
liquid does not filter through the membrane as
quickly as it should), then you can try vortexing
the tubes before inverting them, or adding a few
drops of dimethy lsulfoxide (DMSO) then vortexing
(make sure that total DMSO stays below 20% of
what's left above the membrane) - DMSO is highly
effective for dissolving Nanogold.

One consideration: we don't recommend doing this
as a purification method (i.e. multiple times),
but only to concentrate the samples before liquid
chromatography, which is our principal method for
separation. We recommend gel filtration liquid
chromatography to separate the Nanogold conjugate
from unbound excess Nanogold (Superose-12 is a
good resin for this).

The best method for separating colloidal gold
conjugates is widely held to be density gradient
ultracentrifugation over a 10 to 30% sucrose or
glycerol gradient. For 5 nm colloidal gold, the
literature procedure (see, for example, Slot and
Geuze, Immunolabeling for EM, 1984) consists of
an initial pelleting for 45 mins at 60,000 to
125,000 g; the loose part of the pellet is then
resuspended and recentrifuged over a 10 to 30%
gradient of sucrose or glycerol in 1% BSA-Tris
buffer, and centrifuged again for 45 minutes at
125,000 g (41,000 rpm on a Beckman SW41 rotor),
usually at 4C. The good stuff (the right size
and not aggregated) is usually about one-third to
half-way down. You can then remove the glycerol
by dialysis if necessary.

We usually can't pellet Nanogold, although we've
noticed that it occasionally precipitates rather
than pellets - for this or 2 nm gold you will
probably need to use a very high-g centrifuge
such as a Beckman Airfuge compressed-air
centrifuge.

Research Diagnostics, Inc. have a thorough set of
instructions for preparing colloidal gold
conjugates:

http://www.researchd.com/gold/gold8.htm

We include a section on our web site which
discusses what Nanogold is, how labeling works,
and how to optimize the labeling reaction and the
separation of conjugates:

http://www.nanoprobes.com/LGuide.html

We would also recommend double-checking the
conjugation reaction - particularly the pH and
(in the case of Nanogold) the stoichiometry, or
ratio of the amounts of Nanogold to protein.

Hope this helps,

Rick Powell
Nanoprobes, Incorporated
rpowell-at-nanoprobes.com
www.nanoprobes.com

__________________________________________________

Good afternoon,

I've been attempting to make gold-conjugated antibodies and I've had varying
degrees of success. I'm currently working with 1.4nm Nanogold, 2nm and 5nm
colloidal gold from various vendors. I believe each conjugate is made
correctly, but my methods for purifying and concentrating the 1.4nm and 2nm
products are not adequate. Depending upon the conjugate, the samples are
unrecoverable from the centricon or ultracentrifuge tube.

I'm figuring that my centrifuge conditions are not appropriate and that the
Nanogold may be binding irreversibly to the centricon membrane. The protocols
supplied by the colloidal gold vendors do not give sufficient details and my
efforts to extrapolate the speed at which to spin the 2nm conjugates have not
worked as of yet. I would appreciate any input or experience that one could
share. Feel free to contact me using the email address below.

Thanks in advance,
Henry

--
Henry C. GrisČ
grise-at-bio.fsu.edu
Biology Graduate Student
Florida State University
Tallahassee, FL 32306

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 09:39:21 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Listers,

Second try.
We're trying to cut a couple of Indium/Thallium alloys: 78 at. %
In/22 at. % Tl and 18 at. % In/82 at. % Tl.
We're actually trying to produce a good face for examination in a
reflecting metallographic (light) microscope, not produce sections. A
good SEM specimen would be nice. Grain structure at the LM level is
desired. The alloy is very soft, however, and isn't cooperating.
Tried:
Breaking in LN2. It bent.
Cutting with EMD. Pitted the face.
A diamond saw. Smeared the face.
Lapping. Embedded polishing compound in the face.
Electro-jet polishing, but the solutions tried didn't work. I don't
know what solutions were tried, though, any hints?
We're trying glass-knife microtomy, but I suspect we'll have smearing
problems. We don't have a materials science diamond knife, nor can we
buy one.
We're looking for a laser cutter or high-pressure water jet cutter.
Any other ideas? TIA

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 11:17:19 2004

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Hello Phil,

You have a challenge, no doubt! I have no experience with your particular
alloy, but have had limited success with soft metals using typical
metallographic grind/polish methods, followed by a long session in a
vibratory polisher with sub-micron alumina (C) or colloidal silica. Use a
light load, embedments *are* a problem...

Regards,
Woody
------------------

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Philip Oshel [mailto:peoshel-at-wisc.edu]
Sent: Wednesday, June 30, 2004 11:09 AM
To: Microscopy-at-microscopy.com

Listers,

Second try.
We're trying to cut a couple of Indium/Thallium alloys: 78 at. %
In/22 at. % Tl and 18 at. % In/82 at. % Tl.
We're actually trying to produce a good face for examination in a
reflecting metallographic (light) microscope, not produce sections. A
good SEM specimen would be nice. Grain structure at the LM level is
desired. The alloy is very soft, however, and isn't cooperating.
Tried:
Breaking in LN2. It bent.
Cutting with EMD. Pitted the face.
A diamond saw. Smeared the face.
Lapping. Embedded polishing compound in the face.
Electro-jet polishing, but the solutions tried didn't work. I don't
know what solutions were tried, though, any hints?
We're trying glass-knife microtomy, but I suspect we'll have smearing
problems. We don't have a materials science diamond knife, nor can we
buy one.
We're looking for a laser cutter or high-pressure water jet cutter.
Any other ideas? TIA

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 11:19:45 2004

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PS...

You probably already are aware, but Tl is rather toxic.

Woody

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 11:52:59 2004

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Phil:

One of the best methods for cutting soft materials is the wire saw.
There are 2 ways to use the wire saw - with diamond coated wire or with
an uncoated wire and an abrasive slurry. The method with an abrasive
slurry would be best for your application. I understand that you had
problems with embedding of abrasive grains during lapping, but the wire
sawing process is forcing the abrasive against the area you are cutting
away as opposed to towards the surface that will remain as in a lapping
process.

The wire saw will not smear the material as happens with a diamond wheel
saw. If you'd like, I'd be happy to cut a sample for you in our lab.
Please contact me off-line to make arrangements.

We also have a number of relevant application notes that you can
download from our website which deal with the wire saw as well as our
other materials processing equipment. Go to www.southbaytech.com and
navigate to "Applications Support". There are also links to FAQs and
Application Notes from the product pages. Type "Wire Saw" in the search
box at the upper right corner of the page to see our listing of 3 wire saws.

DISCLAIMER: South Bay Technology has been producing wire saws for more
than 40 years and, therefore, has a vested interest in promoting their use.

Best regards-

David

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

Philip Oshel wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Listers,
}
} Second try.
} We're trying to cut a couple of Indium/Thallium alloys: 78 at. % In/22
} at. % Tl and 18 at. % In/82 at. % Tl.
} We're actually trying to produce a good face for examination in a
} reflecting metallographic (light) microscope, not produce sections. A
} good SEM specimen would be nice. Grain structure at the LM level is
} desired. The alloy is very soft, however, and isn't cooperating.
} Tried:
} Breaking in LN2. It bent.
} Cutting with EMD. Pitted the face.
} A diamond saw. Smeared the face.
} Lapping. Embedded polishing compound in the face.
} Electro-jet polishing, but the solutions tried didn't work. I don't
} know what solutions were tried, though, any hints?
} We're trying glass-knife microtomy, but I suspect we'll have smearing
} problems. We don't have a materials science diamond knife, nor can we
} buy one.
} We're looking for a laser cutter or high-pressure water jet cutter.
} Any other ideas? TIA
}
} Phil

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 12:19:46 2004

Contents Retrieved from Microscopy Listserver Archives
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On Jun 30, 2004, at 8:08 AM, Philip Oshel wrote:

} Second try.
} We're trying to cut a couple of Indium/Thallium alloys: 78 at. % In/22
} at. % Tl and 18 at. % In/82 at. % Tl.
} We're actually trying to produce a good face for examination in a
} reflecting metallographic (light) microscope, not produce sections. A
} good SEM specimen would be nice. Grain structure at the LM level is
} desired. The alloy is very soft, however, and isn't cooperating.
} Tried:
} Breaking in LN2. It bent.
} Cutting with EMD. Pitted the face.
} A diamond saw. Smeared the face.
} Lapping. Embedded polishing compound in the face.
} Electro-jet polishing, but the solutions tried didn't work. I don't
} know what solutions were tried, though, any hints?
} We're trying glass-knife microtomy, but I suspect we'll have smearing
} problems. We don't have a materials science diamond knife, nor can we
} buy one.
} We're looking for a laser cutter or high-pressure water jet cutter.
} Any other ideas? TIA
}
Dear Phil,
Could you prepare a suitable face by pulling a "pre-scored" rod? By
this I mean to take a fairly thick cylinder of the alloy, cut into it
to make a fairly short length of very thin material (diameter to be
determined by what size face you need), then apply a short, intense
pull to separate the rod at its thinnest point, like breaking silly
putty.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 12:57:05 2004

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listers

does anyone have a foot switch and/or specimen holders for a leica 2800 frigocut-E
cryomicrotome in your spare parts inventory?? would be much appreciated as we set
up our latest "donation" to our lab.

thanks

tbudd

--
Dr. T. Budd
Professor and Chair of Biology
St. Lawrence University
Canton, NY 13617
Phone = 315-229-5640
Fax = 315-229-7429
E-mail = tbudd-at-stlawu.edu

This message is made of 100% recycled electrons!

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 13:52:57 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (parthara-at-ucmail.uc.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Wednesday, June 30, 2004 at 09:48:30
---------------------------------------------------------------------------

Email: parthara-at-ucmail.uc.edu
Name: Ranjani Parthasarathy

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello,

We are using permanox chamber slides (Nunc) to grow keratinocytes,
infect them with viruses and then perform immunofluorescence. We are
observing that under the microscope the cells do not look very clear.
Nunc says that glass slides are better then permanox for
immunofluorescence, as the permanox has minimal fluorescence and that
the nature of the plastic is that it has a slight cloudiness to it. I
have several chambers with cells treated and fixed and ready to be
stained. Is there any way to be able to use these chambers and not
have to redo the entire experiment?

Thanks for any suggestions
Ranjani
Research Associate
University of Cincinnati

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 14:18:58 2004

Contents Retrieved from Microscopy Listserver Archives
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We are looking for a darkfield system for an Olympus BH-2, used is
OK. Please contact me offline if you have any information. Thanks in
advance,

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370
fax +54 11 4982-4494
ramirez-at-macn.gov.ar

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 14:53:44 2004

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Phil,
To me it looks like your best bet is to cut it with whatever and then
polish it with polishing film to avoid embedding particles in the
sample. You will soil the film very fast and will need more fresh film
perhaps, but you will expose the substructure of the sample. The water
jet sounds promising, but it might smear the face too. Polishing in LN2?
Wet etching? This is one brain buster..

Philip Oshel wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Listers,
}
} Second try.
} We're trying to cut a couple of Indium/Thallium alloys: 78 at. % In/22
} at. % Tl and 18 at. % In/82 at. % Tl.
} We're actually trying to produce a good face for examination in a
} reflecting metallographic (light) microscope, not produce sections. A
} good SEM specimen would be nice. Grain structure at the LM level is
} desired. The alloy is very soft, however, and isn't cooperating.
} Tried:
} Breaking in LN2. It bent.
} Cutting with EMD. Pitted the face.
} A diamond saw. Smeared the face.
} Lapping. Embedded polishing compound in the face.
} Electro-jet polishing, but the solutions tried didn't work. I don't
} know what solutions were tried, though, any hints?
} We're trying glass-knife microtomy, but I suspect we'll have smearing
} problems. We don't have a materials science diamond knife, nor can we
} buy one.
} We're looking for a laser cutter or high-pressure water jet cutter.
} Any other ideas? TIA
}
} Phil

--
Milen Shishkov
Wellman Center for Photomedicine
Massachusetts General Hospital
Harvard Medical School

Address: MGH
BAR 712
50 Blossom St.
Boston, MA 02114
Phone: (617) 726 1589
Fax: (617) 726 4103

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 16:18:18 2004

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How are you looking at the slides? Have you removed the chamber and
coverslipped the cells or are you trying to look through the plastic
slide? If so, that is your problem. In addition, plastic can absorb a lot
of UV light so that can attenuate the signal. You might want to consider
putting small round (12 mm diameter) glass cover glasses into 24 well
trays. Seed your cells, infect them, and then mount cell side facing down
onto a glass slide. this works well. good luck. tom

At 02:22 PM 06/30/04 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 18:39:59 2004

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This is probably an FCC alloy with that much In in it and it makes sense that it smears and will not fracture at LN2 temp, it does not have a ductile-brittle transition. As you are finding out, soft materials are a problem to polish. Here are some suggestions:

1) Find an FIB and dry cut a small sample. No problems and you may even get enhanced optical imaging with playing with ion imaging the cut sample. Your sample size will be extremely small but still accessible unless the feature sizes are bigger than the sample size.

2) You don't say what the treatment of this alloy is. Are you interested in the phases and microstructure after some processing or deformation or what? If it is cast structure, why not recast it on a very smooth surface and then chemically etch the smooth surface when you remove it from that surface? You might try glass, mica, or something similar. That surface should be as clean as possible prior to casting the sample on it.

3) South Bay Technology also has a chemical wire saw system that drips an acid onto the wire cutting through the sample. I have never seen this system work, but I have seen it in their brochure. I would take Dave Henriks up on his offer of wire cutting the sample using a smooth wire and the boron carbide slurry mixture made with glycerin and water.

4) Use one of the other treatments that you have already tried followed by vibratome polishing. If you used EDM, you could put a coating of epoxy on surface to fill in the pits, cure it and then polish. Periodically redo the epoxy. You will have to chemically finish the sample to remove the "smeared" material. You could also try the vibratome route. You could also use a low angle ion mill to ion polish the surface after the mechanical cutting and polishing steps. On an EDM sample you might have to have in there for a while, but you would succeed. Also an option is to low angle ion mill the wire saw cut sample.

5) Check with Buehler, Struers, and other companies who have polishing equipment and who publish metallographic "how to" books. You want to look for examples of copper, lead, or solder alloys to see how they handle the smearing problem.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

Philip Oshel wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
}
} Listers,
}
} Second try.
} We're trying to cut a couple of Indium/Thallium alloys: 78 at. % In/22
} at. % Tl and 18 at. % In/82 at. % Tl.
} We're actually trying to produce a good face for examination in a
} reflecting metallographic (light) microscope, not produce sections. A
} good SEM specimen would be nice. Grain structure at the LM level is
} desired. The alloy is very soft, however, and isn't cooperating.
} Tried:
} Breaking in LN2. It bent.
} Cutting with EMD. Pitted the face.
} A diamond saw. Smeared the face.
} Lapping. Embedded polishing compound in the face.
} Electro-jet polishing, but the solutions tried didn't work. I don't
} know what solutions were tried, though, any hints?
} We're trying glass-knife microtomy, but I suspect we'll have smearing
} problems. We don't have a materials science diamond knife, nor can we
} buy one.
} We're looking for a laser cutter or high-pressure water jet cutter.
} Any other ideas? TIA
}
} Phil

--
Milen Shishkov
Wellman Center for Photomedicine
Massachusetts General Hospital
Harvard Medical School

Address: MGH
BAR 712
50 Blossom St.
Boston, MA 02114
Phone: (617) 726 1589
Fax: (617) 726 4103

From MicroscopyL-request-at-ns.microscopy.com Wed Jun 30 21:08:50 2004

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Ranjani, I agree with Tom that growing the cells in glass cover slips in
well plates get rid of most of such problems. Other possibility is you can
use, coverslip bottom chambers. If you wish you can get them from
http://www.nuncbrand.com/page.asp?ID=236&lang=GB If you wish to save the
current experiment where cells already grown and infected with virus in the
Permanox chambers you can remove the chamber completely including the small
silicon base which holds the plastic chamber on to the slides and coverslip
(glass) them with suitable antifade mountant, then find an inverted
fluorescence microscope and view them from through the cover slip side.
I hope this helps.
Shiv

Mayandi Sivaguru, Ph.D.,
Associate Director
Molecular Cytology Core Facility
Molecular Biology Program
2, Tucker Hall
University of Missouri
Columbia, MO 65211-7400
sivagurum-at-missouri.edu

Voice: 1-573-882-4895
Fax: 1-573-882-0123

www.biotech.missouri.edu/mcc/

At 02:22 PM 6/30/04, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Thu Jul 1 07:30:48 2004

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Dear Ephram,

Thanks. We have little control of
contrast mechanisms, and no easy way to
make the goniometer non-eucentric (if
only we were so lucky with real
microscopes), but beyond that and
memory/speed limitations, the size range
and diversity of structures we can
assemble for exploration is limited
mainly by our imaginations.

Perhaps for this community I should also
mention that fringe-visibility maps have a
layout similar to Kikuchi maps, except that
band widths depend on specimen thickness and
increase with d rather than the converse.
That means that quantitative/interactive Kikuchi
map models are also easily put together. I've
now posted 100kV Kikuchi maps for Gold and Si
by way of example.

Any other structures of interest or
suggestions? For example, a button to list
REL indices e.g. for planes seen horizontally
edge-on could be quickly implemented.

Cheers. /phil

*********** REPLY SEPARATOR ***********

On 6/28/2004 at 8:53 PM you? wrote:

} This site is a clear cut above other 3 dimensional sites I've seen, and
} the fact that it's microscopy-related is a real bonus.
}
} Well done.
}
} Ephram Shizgal
} Delong America Inc.
} www.lv-em.com
}
}
} -----Original Message-----
} From: Scanned Tip and Electron Image Lab Staff
} [mailto:staff-at-newton.umsl.edu]
} Sent: Monday, June 28, 2004 6:01 PM
} To: microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] interactive worlds & visibility maps
}
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 1 08:12:42 2004

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Micromavens,

Many thanks for all the replies and ideas. We have enough now that
some one or more of them must work. I'll pass on which one(s) end up
giving the needed results.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 1 08:18:41 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (marek-at-physics.mun.ca) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Tuesday, June 29, 2004 at 16:37:14
---------------------------------------------------------------------------

Email: marek-at-physics.mun.ca
Name: Marek Bromberek

Organization: Memorial Univ. of Newfoundland

Education: Graduate College

Location: St. John's, Canada

Question: I have two question which might be related:
1. How do I allign a polarizing microscope?
2. If I see double cross in the field of view, how do I get rid of it?

Thanks

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 1 08:19:17 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (manton-at-biol.uoa.gr) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Wednesday, June 30, 2004 at 05:23:16
---------------------------------------------------------------------------

Email: manton-at-biol.uoa.gr
Name: M. Antonelou

Organization: university of Athens

Education: Graduate College

Location: Athens, Greece

Question: Does anyone have any suggestions as to how I can polymerize
a pellet of mammalian cells (cell cultures) in unicryl resin by UV at
4oC without a final swelling of the cells?

I have had no serious swelling problems so far with a variety of
animal tissues in unicryl polymerization under the same conditions,
but when I started processing cultured cells I faced an unacceptable
(10x) increase in cell volume and a massing up of the ultrastructure
after resin polymerization (UV, 4oC, 15-20cm distance from the lamps).

So far, I have tried a high speed cell pellet, a low gelling
temperature agarose (3%) (in order to keep the pellet compact) and
polymerization at 4oC or 50oC, but they didn't work. A cell pellet in
10% gelatin works well in polymerization, but I had problem with
sectioning properties of the unicryl and furthermore, I don't like
the temperature that this procedure requires (possible loss of
antigenicity).

I would appreciate very much if someone who knows about unicryl could
propose a suggestion.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 1 09:02:12 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (ggallag-at-juno.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, July 1, 2004 at 08:58:42
---------------------------------------------------------------------------

Email: ggallag-at-juno.com
Name: Gregg Gallagher

Organization: ACMC

Title-Subject: [Microscopy] [Filtered] MListserver: Titanium Carbide

Question: What is the index of refraction for titanium carbide
powder? Should it appear "brighter" than silicon carbide using
reflective light?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 1 12:32:50 2004

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I'm thinking about changing the oil in my roughing pump on my TEM and I'm
looking for some advise. The TEM is a Phillips 400, and my interpretation
of the instructions is to break a union between the pump and the roughing
tank. I assume this is after venting the column. As a novice, I 'm
looking for advice on the best way to vent the column and I am reluctant to
undo any unions between the roughing tank and pump.

Any thoughts?

Thanks!!!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 2 09:37:37 2004

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Hi Listers,

You know what? I just started at this job and I have to leave it very
soon. There's nothing wrong with this job, the PI is a great guy and the
department is full of nice friendly people. It's just that I have to move
across the country ASAP.

Anyway here are the details:

Title: Research Specialist
though you will be an EM tech.

Experience with TEM and SEM (elemental analysis is helpful but not
neccessary) and all phases of those two things.
You will be helping teach an EM class in the spring semesters.

Location: Old Dominion University
Department of Biological Sciences
Norfolk, VA

Pay: It's not great but it's pretty cheap to live down here. Pay scale is
in pay band 4 and you will start at the lowest level, this is an exempt
position.

This job cannot be posted yet, due to HR protocols, but I am collecting
resumes from interested individuals and will pass them on to the PI.

Please send them as Word documents (you know .doc)

Looking forward to seeing who's interested.

Paula :-)

Paula Sicurello
EM Lab
106 Mills Godwin Sciences Building
Old Dominion University
Norfolk, VA 23529
USA
757-683-3822

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 2 15:27:00 2004

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Appended is a posting from a colleague. Please respond directly to him.

Smithsonian Institution/Jet Propulsion Laboratory - Postdoctoral position in Geochemistry

The National Museum of Natural History's Department of Mineral Sciences and the Jet Propulsion Laboratory are seeking applications for a postdoctoral fellowship in the field of geochemistry with applications to Astrobiology. The successful applicant will utilize state-of-art geochemical imaging and analysis tools including: submicron ion beam techniques (eg Time of Flight-Secondary Ion Mass Spectrometry) and electron beam methods (full-spectrum UV/VIS cathodoluminescence, and full-spectrum X-ray imaging and microanalysis). A Ph.D. in one of several fields including geochemistry, biogeosciences, or materials science is required. The position will be awarded initially for 1 year and is renewable for a second year contingent upon funding and performance. The position is immediately available to be filled (in Washington, DC) and carries a stipend of $45,000. Benefits include travel and research allowances, and health insurance. For further information contact: Dr. Ed Vicenzi, Dept. of Mineral Sciences, Smithsonian Institution, Washington, DC (vicenzi-at-volcano.si.edu), or Dr. Kim Kuhlman, Jet Propulsion Laboratory, California Institute of Technology, Pasadena, CA (kkuhlman-at-jpl.nasa.gov).

Scott Whittaker
Laboratories of Analytical Biology
Smithsonian Institution
National Museum of Natural History
PO Box 37012 MRC104
Washington DC 20013-7012
202-357-1651

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 2 21:11:14 2004

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Hi Listers,

After many inquiries, I realize I need to post the starting salary of the
job in Norfolk.

Now remember the cost of living in Norfolk is not high. For instance I
rent a large 2 bedroom townhouse in the more fancy part of town for
$650/month.

The starting annual salary is (drum roll please) $27,323

This is a hard money (and hard to get more money) position, you will be an
employee of the state of Virginia.

The work environment is more than relaxed, there is no real dress code
(except no open toed shoes in the lab)and you get your own office, phone
number and computer.

So if you are still interested drop me a line. I'll get back to you after
the 4th, actually the 5th.

See ya Tuesday,

Paula :-)

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 3 10:21:40 2004

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Hello Karl,
In regards to changing the mechanical pump oil in the EM400 it is not
necessary to vent the column.
Assuming you have a pumping service manual refer to page 636-5.2.3 also
fig. 828.
The pumps might not be attached with bolts and depending on the length of
the hose you might be able to turn this to get at the drain plugs to
change the oil.
Notice the sight glass and refill it about 3/4 full Edwards #19 oil.

Good Luck,
FG Technical Service ( X- FEI )
Brockton, MA.
508-580-1148
On Thu, 1 Jul 2004 14:00:43 -0400 Frank.Karl-at-degussa.com writes:
}
}
}
-------------------------------------------------------------------------
-----
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
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} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
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-------------------------------------------------------------------------
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}
} I'm thinking about changing the oil in my roughing pump on my TEM
} and I'm
} looking for some advise. The TEM is a Phillips 400, and my
} interpretation
} of the instructions is to break a union between the pump and the
} roughing
} tank. I assume this is after venting the column. As a novice, I
} 'm
} looking for advice on the best way to vent the column and I am
} reluctant to
} undo any unions between the roughing tank and pump.
}
} Any thoughts?
}
}
} Thanks!!!!
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 3 13:59:50 2004

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Colleagues...

The Microscopy and Microanalysis 2004 Program Search Engine
is now on-line at:

http://mm2004.microscopy.org

Cheers

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 3 14:50:26 2004

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Karl, please, don't vent the column, and don't do anything with the roughing tank.

Assuming the pump is working properly (pulls proper vacuum, does not make funny noises and smoke, doesn't leak oil), and does not
need cleaning:

1) Depress vacuum ON button (right control panel), hold it down for a minute or two, let the pump run and warm up.
2) Turn off TEM by pressing mains OFF button on left control panel.
3) Swing power supply cabinet open.

Quick oil change.

4) Disconnect pump intake hose and exhaust hose if present.
5) Carefully lift pump, rotate it so that drain plug is facing back of the TEM, and elevate pump by placing it upon a piece of wood
(4x4 works well), a brick, etc. Avoid stretching pump power cable. If cable is too short, unplug it from power supply after
un-screwing it's connector lock. Make sure pump is slightly tilted - drain plug down, motor-up.
6) Use oil pan (auto parts store), unscrew oil drain plug from the pump, drain oil, replace plug.
7) Make sure pump position is horizontal. Fill pump with fresh oil. Slowly, don't over-fill. Watch the sight glass.

Very quick-n-dirty oil change

4) Have a shallow dish and aluminum foil, plenty of paper towels, inspection mirror.
5) Bend aluminum foil as a U-channel, put it between drain plug and shallow dish.
6) Carefully unscrew drain plug, but don't remove it completely. Hold it at the drain hole and control oil flow, keep oil from
spilling over U-channel. Drain oil, replace plug.
7) Fill pump with fresh oil. Slowly, don't over-fill. Watch the sight glass with inspection mirror (you can't see it directly unless
pump is rotated).

Very quick-n-dirty oil change is not recommended as a standard practice. Old oil does not drain completely, and some oil will be
spilled.

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: {Frank.Karl-at-degussa.com}
To: {microscopy-at-msa.microscopy.com}
Sent: Thursday, July 01, 2004 2:00 PM

Colleagues

The June 2004 Microscopy Listserver Archives are now on-line at:

http://www.microscopy.com/MicroscopyListserver

Cheers....

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 5 01:36:14 2004

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Announcing the Royal Microscopy Society, IBMS accredited course:

Cell Imaging Techniques

Sep. 6-10th 2004

Oxford Brookes University
Oxford, UK

Course organisers: Chris Hawes and Susan Brooks

For more information and online registration:

http://www.rms.org.uk/cgi-bin/events_details.cgi?id=imm26825813

Cell imaging techniques are central to the life sciences and with the
dawn of the post-genomics era, techniques that permit the accurate
location of gene products within cells and tissues will be in ever
increasing demand. The rapidly developing field of cell imaging
techniques has contributed much towards our current understanding of
cell structure and function.

This popular five-day course is updated every year to take into account
new developments in cell imaging approaches and closely related
technologies. It will be of immense value to any life scientist or cell
biologist, from research or technical background, from hospitals,
research institutes, industry or academia and at any stage in their
career, who wishes to learn or update their knowledge of current cell
imaging techniques, either for routine purposes or for research. It
covers a wide range of applications in pathology, cell biology and the
plant sciences. It is structured towards a technical understanding of
immuno-affinity techniques, as once they are mastered they can be
applied to almost any cell system.

Course Structure:
The course is structured around hands-on practical workshops supported
by seminars led by a range of experts in the field. The approach is
interactive, friendly and participant-orientated and no previous
experience or knowledge is assumed. Course participants are led from the
basics through a range of state of the art techniques. The main emphasis
of the week will be to give participants sufficient practical knowledge
of immuno-labelling and other affinity labelling techniques to enable
them to carry out labelling and imaging experiments in their own
laboratories. In parallel, a series of more in-depth seminars by
specialist exponents in various areas of affinity labelling and related
techniques, will expose participants to more advanced areas of the
field. Full day practical workshops supported by seminars will focus on
three main topics: The first day is based around immuno-labelling for
light microscopy and includes an introduction to immunocytochemistry,
the concept of using different types of cell and tissue specimens and
the range of different labels for imaging cells, including fluorescent
markers. A second practical workshop day introduces participants to
state-of-the-art confocal microscopy, including immuno-labelling at the
confocal microscope level and imaging live cells using green fluorescent
protein (GFP). The other main practical workshop will focus on
techniques for immuno-labelling at the electron microscope level.
Supporting specialist seminars will be given on a range of subjects
including: in situ hybridisation, silver enhancement techniques,
fixation strategies, approaches to image analysis, multiple fluorescence
labelling techniques and the application of fluorescent proteins. There
will be a special guest lecture by Dr. Jim Haseloff from the Department
of Plant Sciences at the University of Cambridge.

For more information contact Lucy Haworth,
Telephone +44 (0) 1865 248768
Fax: +44 (0) 1865 791237
Email: lucy-at-rms.org.uk

Or me at the numbers below,

Cheers, John.

--

*********************************
C. John Runions, Ph.D.
School of Biological and Molecular Sciences
Oxford Brookes University
Oxford, UK
OX3 0BP

email: jrunions-at-brookes.ac.uk
phone: +44 (0) 1865 483 964

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 5 08:49:57 2004

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Question: HI. I had taken histological samples on the locust ventral
cord. I am taking neural recordings using penetrating electrodes. The
probe was left inside the tissue and proceeded with the histology
procedure.
I found that close to the region where the probe was, the staining is
poor. I was wondering if the probe which is make of silicon oxide and
gold electrodes could have had an effect on the staining???
I used bodian, cresyl fast violet and haemotoxily and eosin staining
methods.

Many thanks,

K Bustamante

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 5 11:09:07 2004

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I think the problem is more likely that you have damaged some of the cells
during penetration and they are dead. If you burst a cell, its contents
will leak out and that region will subsequently stain poorly. This is not
uncommon in my experience near points of dissection. In some cases, dead
cells are very sticky and can take up more stain than normal.

At 03:21 PM 07/05/04 +0100, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 5 11:25:54 2004

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POSTDOCTORAL POSITION IN INTERFACE PHYSICS

DEPARTMENT OF CHEMICAL ENGINEERING AND MATERIALS SCIENCE
UNIVERSITY OF CALIFORNIA-DAVIS

A postdoctoral position is available in the Interface Physics Group at
the University of California-Davis (UCD). Research in the Interface
Physics Group focuses on the use of atomic resolution imaging and
analytical techniques in electron microscopy, coupled with theoretical
simulations, to determine the structure-property relationships at
internal interfaces on the fundamental atomic scale. Current research
programs involve catalysts, ferroelectrics, high-Tc superconductors and
optoelectronic/high-power semiconducting materials and devices. The
position that is currently available is to oversee the installation of a
new JEOL 2500SE at UC-Davis and develop collaborative programs with
faculty working on various projects within the campus nanoscale
initiative. Successful candidates will be recent Ph.D. graduates in
physics, metallurgy, or materials science with a sound background in the
relevant materials issues and an ambition to be part of a developing
program pushing at the frontiers of interface physics. Please send a
resume and publication list to Professor Nigel D. Browning at the
address below. Prior experience in STEM or TEM is essential. However,
consideration will be based on the candidates overall potential for
success in the field and applicants with prior experience in related
fields are encouraged to apply. Positions are for one year initially,
normally renewed for a second year with possibilities existing for
further years. Salary is commensurate with experience.

Nigel D. Browning

Department of Chemical Engineering and Materials Science
University of California-Davis
One Shields Ave
Davis, CA 95616

AND

National Center for Electron Microscopy, MS 72-150
Lawrence Berkeley National Laboratory
Berkeley, CA 94720

Tel: 530-754-5358 (Davis)
510-486-4612 (NCEM)
Fax: 530-752-9554 (Davis)
510-486-5888 (NCEM)
e-mail: nbrowning-at-ucdavis.edu
ndbrowning-at-lbl.gov

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 6 14:11:43 2004

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Colleagues

I'm just tesing for bad addresses in the database. Please ignore/trash
this message.

Nestor
YourFriendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 6 15:27:11 2004

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Hello,
We recently inherited an XL 30 ESEM TMP, W. It is from
FEI/Philips/Electroscan. I was wondering if there are any other users out
there that may have some advice or tips for us. Please contact me at my
email address above/below.

To get it running, we had to replace the high tension supply/gun supply
unit. I noticed through the service records that this was done before, so
in 3 years of operation, it has had three power supplies. Anyone else
noticed similar problems on their XL ESEMS?
Thanks for your help.
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 6 20:47:07 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (camiller-at-anatomy.iupui.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 6, 2004 at 12:35:23
---------------------------------------------------------------------------

Email: camiller-at-anatomy.iupui.edu
Name: Caroline Miller

Organization: Indiana University

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I run a core service facility with a fee schedule. How much do other facilities charge for immuno staining and how are charges handled for attempts that are unsuccessfull? How much do facilities charge for scope time, independent vs. full service? This facility is not subsidized by the unversity.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 6 20:48:14 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (antuni-at-aol.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 6, 2004 at 19:42:54
---------------------------------------------------------------------------

Email: antuni-at-aol.com
Name: Anthony J. Ribaudo

Organization: NYPD

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: When we turn up the tungsten filament on our ARMAY 1830 SEM
the red LED goes out indicating current is running through the filament. However, the emission meter LEDs all light up across the whole range of the meter in a sweeping motion, we don't see a specific value of microamps e.g. say 30 or 40 microamps. Consequently, we cannot perform a beam alignment because we have no reference level.
The filament was installed as follows: After bringing the filament level with the Wehnolt aperture, we back off the filament 3 1/2 notches as recommended in the manual,
each notch is 25 micrometers. The instrument has an ion pump (gun chamber)and diffusion pump. Is the problem with the filament or the meteror some other problem ?
Suggestions are welcome.

Anthony Ribaudo
NYPD Forensic Lab

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 04:05:23 2004

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Hello

To make better products for imaging software we need more information about
the users. Therefore, you can help us to improve the usability of software!
For this reason, it would be very helpful if you could fill out the survey:

http://www.imaging.ergosystems.de

You can win 10 gift certificates from AMAZON each 50? worth!

Kind Regards
Daniel Mauch
(Usability Engineer)

ErgoSystems
Laimer Platz 1
D-80689 Munich
Germany

Email: info-at-ergosystems.de
Web: www.ergosystems.de (German)

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 07:46:09 2004

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Colleagues

As you all know Commerical Survey's using the Microscopy Listserver
are prohibited by our Rules.

http://www.microscopy.com/MicroscopyListserver/FAQ.html

This particular request was denied several weeks ago, at which time
I explained the rules, to the requestor. However I see
that the individual has proceeded nevertheless, which makes
the posting even more aggregious.

I have remove the individual from the subscriber listing and
blocked further postings.

Nestor
Your Annoyed Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 08:03:48 2004

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Dear all,
You may be aware that operating an EELS spectrometer is affected by the
proximity of a chair containing parts made out of ferromagnetic steel,
as in most office swivel chairs. We are interested in getting hold of a
non-magnetic chair to minimise this interaction. I have seen that one
IKEA chair, "Procent", appears not to contain steel apart from a small
amount in the castors (at least according to the IKEA website). Does
anyone have any experience with this chair?

Does anyone have an alternative suggestion for a non-magnetic chair
suitable for microscopy? It would be preferable if this chair was
available in the UK.

Best wishes

--
Ian MacLaren
Department of Physics and Astronomy
University of Glasgow
Glasgow G12 8QQ
Scotland
http://www.physics.gla.ac.uk/~maclariz/

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 09:03:08 2004

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Anthony,

Turn the filament another two clicks, for a total of 5 1/2 notches, or
about 125 to 130 microns. This is according to the service engineer from
Amray who serviced our 1830 for years. He is probably the person who
installed your instrument, if it is the one at the academy.

FYI, as you are bringing it up, there is a balancing act between the
filament current setting, and the bias voltage setting. Increasing the
bias will decrease the emission current. These settings help control the
spot size and beam current, according to your requirements. (Just in case
you were unaware of this...)

Let me know if this works.
Darrell

antuni-at-aol.com (by way of MicroscopyListserver) wrote on 07/06/2004
09:47:43 PM:

}
}
}
------------------------------------------------------------------------------

} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.
} com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------

}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (antuni-at-aol.com) from http://microscopy.
} com/MicroscopyListserver/MLFormMail.html on Tuesday, July 6, 2004 at
19:42:54
}
---------------------------------------------------------------------------
}
} Email: antuni-at-aol.com
} Name: Anthony J. Ribaudo
}
} Organization: NYPD
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: When we turn up the tungsten filament on our ARMAY 1830 SEM
} the red LED goes out indicating current is running through the
} filament. However, the emission meter LEDs all light up across the
} whole range of the meter in a sweeping motion, we don't see a
} specific value of microamps e.g. say 30 or 40 microamps.
} Consequently, we cannot perform a beam alignment because we have no
} reference level.
} The filament was installed as follows: After bringing the filament
} level with the Wehnolt aperture, we back off the filament 3 1/2
} notches as recommended in the manual,
} each notch is 25 micrometers. The instrument has an ion pump (gun
} chamber)and diffusion pump. Is the problem with the filament or the
} meteror some other problem ?
} Suggestions are welcome.
}
}
}
} Anthony Ribaudo
} NYPD Forensic Lab
}
}
}
}
}
---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 10:09:10 2004

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We have used a wooden swivel stool, much like a short bar stool.
These are easy to hold of. However, it didn't last too long. We have
also used plain wooden chairs that don't swivel, but they are harder
on your back.
Ciao for now,
Ken

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 12:02:49 2004

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Traditionally, how have stage micrometers (used in light microscopy)
been produced? I know that an etching process is involved, but was
wondering how such precision rulings were produced well in advance of
lasers and electron beam lithography. How, too, are the diffraction
grating masters produced that are used in TEM to generate the
replicas of the master grating? A reference, or words from a
"micro-guru," would be very much appreciated.

John B.
--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 12:40:14 2004

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Dear Ian,
I had the same problem with our(P)EELS. I asked Siemens Medical Solutions in
Erlangen/Germany (look at my signature to see why) whether they have any
solutions or suggestions for this: They have non-magnetic chairs for their
magnetic resonance imaging devices (MRI) and I got for free an older prototype
of a kneeling chair they designed for the surgon to work "in situ" (you do not
sit on these chairs but kneel: it becomes a little bit uncomfortable after 3
or 4 hours). Maybe there is a department of this or a similar factory around
and perhaps they want to get rid of an old one, too ...
Hope this helps.
Best regards
Gerhard Frank

Ian MacLaren schrieb:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Dear all,
} You may be aware that operating an EELS spectrometer is affected by the
} proximity of a chair containing parts made out of ferromagnetic steel,
} as in most office swivel chairs. We are interested in getting hold of a
} non-magnetic chair to minimise this interaction. I have seen that one
} IKEA chair, "Procent", appears not to contain steel apart from a small
} amount in the castors (at least according to the IKEA website). Does
} anyone have any experience with this chair?
}
} Does anyone have an alternative suggestion for a non-magnetic chair
} suitable for microscopy? It would be preferable if this chair was
} available in the UK.
}
} Best wishes
}

--
Gerhard Frank
UNIVERSITAET ERLANGEN-NUERNBERG Phone: +49 9131 85 28606
Institut fuer Werkstoffwissenschaften VII Fax: +49 9131 85 28602
Cauerstr. 6, D-91058 Erlangen, Germany Gerhard.Frank-at-ww.uni-erlangen.de

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 12:49:15 2004

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G'day Folks,

Can anyone tell me who, what, where the people are who market and/or sell parts for the Anatech Ltd./ Hummer
line of sputter coaters?

Many thanks in advance.

JohnA

******************************************************

John G. Aghajanian, Ph.D.
University of Connecticut Health Center
Central Electron Microscopy Facility
MC1610
263 Farmington Avenue
Farmington, CT 06030-1610

phone: 860 679-2395
fax: 860 679-4078

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 14:23:33 2004

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Fellow Listmembers,

Our Mini-Workshop Series on "Cryoultramicrotomy for Materials Sciences" is
coming to Los Angeles, California!

The next session will be held at the University of Southern California
(University Park Campus). Details are given below.

**When**:
Wednesday, August 18 through Thursday, August 19, 2004, 9:00am-4:00pm

**Where**:
University of Southern California
Center for Electron Microscopy and Microanalysis
CEM Building, Room 101
814 West 36th Place
Los Angeles, CA 90089-0101

**Local contact for parking, directions, etc.**:
Alicia Thompson
CEMMA / CEM Bldg., Room 100
Tel. 213-740-1991
Fax 213-821-0458
{athompso-at-usc.edu}

**What**:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair
probes), glass knife making, evaluation of glass knives, care and cleaning of
diamond knives and operation of the cryoultramicrotome.

If you wish to bring specimens, please let us know the nature of your
specimens when you
RSVP and reserve a place in the workshop (see below).

**Background**:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing"at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

**Important Info**:
There is no charge for this workshop.

Meals and refreshments will be served!

Attendance is open to everyone for the presentations and demonstrations on
the first day. However, attendance is limited for the cryoultramicrotomy
hands-on sessions on the second day.

**RSVPs and Reservations**:
To RSVP and to reserve a spot for the hands-on sessions, please contact Kim
Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262).

**Sponsors and Organizers**:
University of Southern California
Center for Electron Microscopy and Microanalysis
RMC Products Group, Boeckeler Instruments, Inc.

See you in Los Angeles!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 15:14:13 2004

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Hi Anthony,

A full scale emission current reading may mean one of a number of things!

1. The bias control is set at a low level allowing the full emission
rather than a controlled emission from the gun. SOLUTION turn the bias
control clockwise to reduce the emission by increasing the bias field (I do
not remember if the so called bias control is a true bias control, hence my
earlier explanation, or it may be an emission level control, in which case
you will need to turn the control anticlockwise to reduce the emission
current)

2. The filament is shorting out against the cathode cap thus removing the
bias system from the circuit. SOLUTION check that there are no whiskers
between the cathode cap and filament, clean the cathode cap.

3. The bias circuit has broken down. SOLUTION call in a service
technician.

I truly hope it is (1) or (2) best of luck

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0)7711 606967
www.emcourses.com

----- Original Message -----
} From: "by way of MicroscopyListserver" {antuni-at-aol.com}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, July 07, 2004 2:47 AM

John,

We have purchased parts/targets for our Hummer II through Anatech LTD.
www.anatechltd.com

good luck

scott

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

G'day Folks,

Can anyone tell me who, what, where the people are who market and/or sell
parts for the Anatech Ltd./ Hummer
line of sputter coaters?

Many thanks in advance.

JohnA

******************************************************

John G. Aghajanian, Ph.D.
University of Connecticut Health Center
Central Electron Microscopy Facility
MC1610
263 Farmington Avenue
Farmington, CT 06030-1610

phone: 860 679-2395
fax: 860 679-4078

"Dwell not upon thy weariness,
thy strength shall be according
to the measure of thy desire."
-Proverb

************************************************

Scott Payne
Assistant Director
NDSU Electron Microscopy Center
1307 N. 18th St.
Northern Crops Science Laboratory
North Dakota State University
Fargo, North Dakota, 58105

e-mail - scott.payne-at-ndsu.nodak.edu

Telephone - 701-231-8435

************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 15:32:41 2004

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John, They are Anatech Ltd., location unknown (I think that they're on the
west coast now - Union City, CA). Try these #s: (800) 752-7629 or (800)
390-4449.

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.
Waterbury, CT 06702

"Aghajanian,John" {aghajanian-at-nso1.uchc.edu}
07/07/04 01:48 PM

To
{microscopy-at-microscopy.com}
cc

Subject
Anatech/Hummer

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

G'day Folks,

Can anyone tell me who, what, where the people are who market and/or sell
parts for the Anatech Ltd./ Hummer
line of sputter coaters?

Many thanks in advance.

JohnA

******************************************************

John G. Aghajanian, Ph.D.
University of Connecticut Health Center
Central Electron Microscopy Facility
MC1610
263 Farmington Avenue
Farmington, CT 06030-1610

phone: 860 679-2395
fax: 860 679-4078

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 18:42:07 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Dotty,

I would start with a correlative study. The time has past when one can
attempt to deduce physiologic effects from structure alone. The only
way by which one can follow electrons around is to have a fast detection
system. Even with the best 'stopping' methods for ultrastructural
studies, there are variables that are missed and/or smudged by temporal
(if you will!) diffusion during specimen prep. Thus, as one example of
what I mean, without dealing with the question of the merit of the paper
itself, I offer the following link:

http://www2.iq.usp.br/bioquimica/confocal/Mitochon&Cytoskel.pdf

As an additional note - and in your defense, the problem here, as I view
the question, is that you are asking the correct question when the P.I.
should already have done so. I found what I wanted, a correlative
study, as a confirmation of an experimental suspicion with 3 minutes of
searching in Google ( {mitochondrial confocal pdf} ).

There is plenty of ultrastructure to be described under varying
experimental conditions, but one does not normally decide to use the
electron microscope to view a physiologic process - especially with
organelles whose behavior is as yet not completely charted. Ten or
fifteen years ago, one might have been able to use just the EM for the
use you mention, but I don't believe that is true anymore, now that the
LM is back in the real business of dynamic organellar biology. It seems
to me that your study should begin with confocal microscopy and quickly
migrate to multiphoton microscopy. It is now possible to trap, and
move, individual cells, and it certainly would be possible/probable to
get some information on the effects of various 'fixation' regimens on
live systems by using the confocal LM to watch it occur - even DIC
images would help to set the parameters for a 'least-offensive' method
of fixation. 3D before fixation and 3D after.

My apology for being so blunt, but sometimes one does more good with
unabashed brevity. Also, such a harangue might prompt a
more-knowledgeable investigator to lash me for my temerity, and there
always some mystical fun in that!

Regards,

Fred Monson

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SSS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: Dorothy Sorenson [mailto:dsoren-at-umich.edu]
Sent: Tuesday, June 29, 2004 12:11 PM
To: microscopy-at-msa.microscopy.com

Dear listers,

We will be studying changes in mitochondrial morphology after drug
application to cell monolayers. I have reviewed the listings in the
archives from few years ago regarding effects of osmolarity and choices
of
buffer and fixative on muscle mitochondria. I would think that
mitochondria in cell monolayers would be particularly sensitive to these

factors.

I am condidering fixing the monolayers in 2.5 % glutaraldehyde in serum
free medium in an effort to maintain physiological conditions up to the
moment of fixation. Then, what about rinses before going into osmium?

Can anyone offer any pointers regarding preservation of mitochondrial
morphology in cell monolayers?

Thanks,
Dotty

Dorothy Sorenson
Microscopy and Image Analysis Laboratory
Department of Cell and Developmental Biology
University of Michigan Medical School
4643 Medical Science Building II
1301 Catherine
Ann Arbor, MI 48109-0616

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 7 18:50:02 2004

Contents Retrieved from Microscopy Listserver Archives
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} Hi,
}
} I am imaging DNA with fluorescence microscopy.
}
} Does anybody know a nucleic acid stain having an excitation wavelenght
} higher than 500 nm and that is not an intercalator?
}
} Thank you,
}
} Anne-Laure
}
}
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} Le Ny Anne-Laure
} Grad Student Chemical engineering
} University of Southern California
} PCE 310
} Tel: 213-740-1320
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 8 08:16:37 2004

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Here in the US there are $10 molded plastic lawn chairs available at
just about any hardware, gardening, and certain grocery stores. They
come in a variety of ugly colors and shapes, are reasonably sturdy, and
have no metal whatsoever. If these are available in the UK, it might be
a reasonable solution.

I suspect that any chair with castors will at the least have some metal
in the axles and bearings, unfortunately.

-- Kevin Ryan
kevin-at-mediacy.com
Media Cybernetics, Inc.

} ----------------------------------------------------------------------
} --------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
}
} Dear all,
} You may be aware that operating an EELS spectrometer is affected by
} the proximity of a chair containing parts made out of ferromagnetic
} steel, as in most office swivel chairs. We are interested in getting
} hold of a non-magnetic chair to minimise this interaction. I have
} seen that one IKEA chair, "Procent", appears not to contain steel
} apart from a small amount in the castors (at least according to the
} IKEA website). Does anyone have any experience with this chair?
}
} Does anyone have an alternative suggestion for a non-magnetic chair
} suitable for microscopy? It would be preferable if this chair was
} available in the UK.

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 8 08:32:40 2004

Contents Retrieved from Microscopy Listserver Archives
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Short Course and Workshop Announcement
University of Missouri - Columbia

The Electron Microscopy Core Facility is hosting a 3-day Short Course
and Workshop on Computer-Assisted Image Analysis and Measurement
taught by Dr. John C. Russ on August 16 through August 18, 2004. This
popular course is intended to familiarize users of image analysis
equipment with the fundamental principles and methods available to
obtain meaningful results, and to educate laboratory supervisors or
research professionals seeking to learn how to use such methods in
their applications. The techniques are applicable to fields ranging
from materials, geological and biological/medical research to food
technology and manufacturing quality control.

The course relies heavily on tightly coupled lectures and hands-on
experience with the various techniques. The laboratory includes a
wide variety of image analysis methods designed to cover the range of
approaches and tools, and a detailed set of practical instructions to
enable their use with a minimal learning curve. No specific
background is assumed, although users should already be familiar with
microscopy or other imaging technology, and the techniques required
to obtain the images to be measured. Many of the examples used in the
course involve light or electron microscope images, but students are
invited to bring their own most interesting images (TIFF files) for
discussion and analysis.

Image analysis and measurement methods are used in a broad range of
applications and are usually concerned with extracting a few
numerical values, such as the number, size, shape or location of
objects from the image. In other cases, global structural parameters
such as measures of the volume and surface of structures present are
of interest. These measurements may require image processing to
correct defects, feature enhancement, comparison of multiple images,
object recognition, or other steps. Ultimately, the image is reduced
to just the features of interest. Measurements on these individual
features, or on the image as a whole, must then be obtained and
interpreted in a proper stereological context to obtain useful data
about the objects. Statistical interpretation of the data allows
comparisons of different populations, understanding of distribution
plots, and other inferences about the original objects. Structural
modeling and geometric probability can be used to develop models for
this interpretation.

The course will have an enrollment limit of 20. More information
including a registration form can be found at
http://www.emc.missouri.edu, or by contacting Lou Ross at
573.882.4777 or rosslm-at-missouri.edu.

Lou Ross
Senior Electron Microscope Specialist
Electron Microscopy Core Facility
W136 Veterinary Medicine
University of Missouri
Columbia, MO 65211-5120
(573) 882-4777, fax 884=5414
email: rosslm-at-missouri.edu
http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 8 08:45:18 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have a Reichert CSM binocular scope equipped for phase
contrast, which while I don't use it a lot, is a joy to work
with. Also have the invoices for it, dated Dec 1 and 13, 1950,
as well as original instruction manual (which contains nothing
on phase), and what especially intrigues me is a 5 page hand
typed carbon on Reichert stationery, dated Vienna 18th April
1950: "BRIEF INSTRUCTIONS FOR USING PHASE CONTRAST EQUIPMENT."
I know phase only came into widespread commercial use after WW2,
but the thing makes me wonder more about details. Does anyone
have information as to when Reichert first marketed their phase
equipment, and how early an example this one would be?

The CSM body is s/n 213429, phase condenser s/n 9978.

Thanks in advance for any info.
Larry Weissmann

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 8 10:11:41 2004

Contents Retrieved from Microscopy Listserver Archives
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John,

Ladd Research provides system, targets, parts and accessories for the
Hummers.

John Arnott

Disclaimer: Ladd Research sells microscopy supplies and equipment

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: sales-at-laddresearch.com

----- Original Message -----
} From: "Aghajanian,John" {aghajanian-at-nso1.uchc.edu}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, July 07, 2004 1:48 PM

Good questions! We've had the same problem with charging for
immuno-EM whe projects are unsuccessful. Our policy now
is that we will charge for unsuccessful immuno-EM attempts
when the lack of success is not the fault of the lab, but due to
the type of sample, antigen and antibody provided by the user.
As long as you warn the user that he/she will get charged for
the work regardless of the results of the labeling, you should be
fine. After all, an absence of specific labeling with an antibody
is a result in itself!

As for the charges here at Yale, also unsubsidized:
- Immuno-labeling : $120 per run (up to 10 different antibody
dilutions/conditions)
- Double-labeling: $220 per run
- Scope time: $40/hour unassisted; $80/hour assisted
- Complete immuno-EM service (includes sample prep, cryo-sectioning,
immuno-labeling, EM and up to 10 representative pictures): $300 per
sample (surcharge of $100 in case of double-labeling).
All these charges to go up 3.5% this month.

Hope this helps!

Marc

On Tuesday, July 6, 2004, at 09:46 PM, by way of MicroscopyListserver
wrote:

}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
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} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (camiller-at-anatomy.iupui.edu) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Tuesday, July 6, 2004 at 12:35:23
} -----------------------------------------------------------------------
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}
} Email: camiller-at-anatomy.iupui.edu
} Name: Caroline Miller
}
} Organization: Indiana University
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: I run a core service facility with a fee schedule. How much
} do other facilities charge for immuno staining and how are charges
} handled for attempts that are unsuccessfull? How much do facilities
} charge for scope time, independent vs. full service? This facility is
} not subsidized by the unversity.
}
} -----------------------------------------------------------------------
} ----
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 02:34:04 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Ian,

If any is still left in Scotland try one made out of wood. They used
to make chairs from this material last century. If you look around in
some specialty antique stores you may still find one. They were once
frequently broken over patrons' heads during saloon bar fights in
John Wayne westerns, and no doubt they must have also been available
for a similar purpose in Glasgow's pubs. Some may have survived up to
the present day.

As an added bonus, degaussing chairs made from this material is a no-brainer.

Ours is made from oak. It has a beautifully embroidered cotton seat
with non-ferromagnetic padding. Amazing what they used to make even
before EELS was invented.

BTW the legs on ours have become a bit wobbly of late because it has
been so popular in the lab. Does anyone out there know where one can
get a glue suitable for microscopy?

Cheers! :-)

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 04:25:38 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Ian

carbon fibre chair?

http://www.jeccomposites.com/news/news_fiche.asp?id=578&

Chris

} } Dear all,
} } You may be aware that operating an EELS spectrometer is affected by the
} } proximity of a chair containing parts made out of ferromagnetic steel,
} } as in most office swivel chairs. We are interested in getting hold of a
} } non-magnetic chair to minimise this interaction. I have seen that one
} } IKEA chair, "Procent", appears not to contain steel apart from a small
} } amount in the castors (at least according to the IKEA website). Does
} } anyone have any experience with this chair?
} }
} } Does anyone have an alternative suggestion for a non-magnetic chair
} } suitable for microscopy? It would be preferable if this chair was
} } available in the UK.
} }
} } Best wishes
} }
} } --
} } Ian MacLaren
} } Department of Physics and Astronomy
} } University of Glasgow
} } Glasgow G12 8QQ
} } Scotland
} } http://www.physics.gla.ac.uk/~maclariz/
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 07:44:48 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello,

could someone help me with or does someone have the alignment procedures
for a ISI-DS-130 SEM.
I have big trouble using it abov 2000x (!) and I have no idea how to
align that SEM.

I'd also like to know if there are others involved who still using a
ISI-DS 130?
I need also parts for the ISI-DS 130, maybe someone know where a not
used ISI-DS 130 or parts of it are waiting for me?

Thanl you very much for your help.
Timo Junker

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 09:18:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all!

To solve the charging phenomenon problem of HR FESEM observations, in my
application (polished cross-sections of Silicium dies samples, coated in
epoxy resin, i'm trying to chargea very little quantity of resin with a
very little quantity of metal powder (copper, silver graphite), in
order to keep the resin transparent, just enough to evacuate charges.

Is there a way to measure the very high resistivity of this charged
resin?

My goal is to obtain resistivities { 10e12 ohm*cm...

thanx in advance

Sylvain MAURY

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 12:22:35 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I typed "non magnetic chair" into Google and got 213,000 hits. Here is
one:
http://www.magmedix.com/products/accessories/non_magnetic_chair.html

John Mardinly
Intel

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Friday, July 09, 2004 2:24 AM
To: microscopy-at-msa.microscopy.com

Dear Ian

carbon fibre chair?

http://www.jeccomposites.com/news/news_fiche.asp?id=578&

Chris

} } Dear all,
} } You may be aware that operating an EELS spectrometer is affected by
the
} } proximity of a chair containing parts made out of ferromagnetic
steel,
} } as in most office swivel chairs. We are interested in getting hold
of a
} } non-magnetic chair to minimise this interaction. I have seen that
one
} } IKEA chair, "Procent", appears not to contain steel apart from a
small
} } amount in the castors (at least according to the IKEA website). Does
} } anyone have any experience with this chair?
} }
} } Does anyone have an alternative suggestion for a non-magnetic chair
} } suitable for microscopy? It would be preferable if this chair was
} } available in the UK.
} }
} } Best wishes
} }
} } --
} } Ian MacLaren
} } Department of Physics and Astronomy
} } University of Glasgow
} } Glasgow G12 8QQ
} } Scotland
} } http://www.physics.gla.ac.uk/~maclariz/
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 14:28:44 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

John;

This may not be such a high tech solution but do they still make chairs
of wood? Why get fancy?

Peter Tomic
Agere Systems

-----Original Message-----
} From: Mardinly, John [mailto:john.mardinly-at-intel.com]
Sent: Friday, July 09, 2004 1:21 PM
To: Chris Jeffree; microscopy-at-msa.microscopy.com

I typed "non magnetic chair" into Google and got 213,000 hits. Here is
one:
http://www.magmedix.com/products/accessories/non_magnetic_chair.html

John Mardinly
Intel

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Friday, July 09, 2004 2:24 AM
To: microscopy-at-msa.microscopy.com

Dear Ian

carbon fibre chair?

http://www.jeccomposites.com/news/news_fiche.asp?id=578&

Chris

} } Dear all,
} } You may be aware that operating an EELS spectrometer is affected by
the
} } proximity of a chair containing parts made out of ferromagnetic
steel,
} } as in most office swivel chairs. We are interested in getting hold
of a
} } non-magnetic chair to minimise this interaction. I have seen that
one
} } IKEA chair, "Procent", appears not to contain steel apart from a
small
} } amount in the castors (at least according to the IKEA website). Does

} } anyone have any experience with this chair?
} }
} } Does anyone have an alternative suggestion for a non-magnetic chair
} } suitable for microscopy? It would be preferable if this chair was
} } available in the UK.
} }
} } Best wishes
} }
} } --
} } Ian MacLaren
} } Department of Physics and Astronomy
} } University of Glasgow
} } Glasgow G12 8QQ
} } Scotland
} } http://www.physics.gla.ac.uk/~maclariz/
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 9 14:53:11 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Peter;
I have heard high praise for Shaker furniture, hand made in
Pennsylvania, which of course reminds me of the famous Shaker folk tune
used by Aaron Copeland in 'Appalachian Spring', which starts: 'The GIF
to be simple, the GIF to be free, the GIF to come down right where you
want to be'..........

John Mardinly
Intel

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Sent: Friday, July 09, 2004 12:26 PM
To: Mardinly, John; Chris Jeffree; microscopy-at-msa.microscopy.com

I typed "non magnetic chair" into Google and got 213,000 hits. Here is
one:
http://www.magmedix.com/products/accessories/non_magnetic_chair.html

John Mardinly
Intel

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Friday, July 09, 2004 2:24 AM
To: microscopy-at-msa.microscopy.com

Dear Ian

carbon fibre chair?

http://www.jeccomposites.com/news/news_fiche.asp?id=578&

Chris

} } Dear all,
} } You may be aware that operating an EELS spectrometer is affected by
the
} } proximity of a chair containing parts made out of ferromagnetic
steel,
} } as in most office swivel chairs. We are interested in getting hold
of a
} } non-magnetic chair to minimise this interaction. I have seen that
one
} } IKEA chair, "Procent", appears not to contain steel apart from a
small
} } amount in the castors (at least according to the IKEA website). Does

} } anyone have any experience with this chair?
} }
} } Does anyone have an alternative suggestion for a non-magnetic chair
} } suitable for microscopy? It would be preferable if this chair was
} } available in the UK.
} }
} } Best wishes
} }
} } --
} } Ian MacLaren
} } Department of Physics and Astronomy
} } University of Glasgow
} } Glasgow G12 8QQ
} } Scotland
} } http://www.physics.gla.ac.uk/~maclariz/
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 10 04:35:26 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

At most universities there are old maple chairs stored some where
that are almost indestructible. Find some of those and go over them
wiht a metal detector and remove any metal by cutting it out with a
drill that takes out a core and fill the hole with a hard wood dowel
and epoxy and make ultra high density polyethylene glides instead of
casters and you will have a very sturdy non magnetic chair.

As a last resort having one built should not be to outrageous
compared to scientific specialty equipment.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

: } } Dear all,
: } } You may be aware that operating an EELS spectrometer is
affected by
: the
: } } proximity of a chair containing parts made out of ferromagnetic
: steel,
: } } as in most office swivel chairs. We are interested in getting
hold
: of a
: } } non-magnetic chair to minimise this interaction. I have seen
that
: one
: } } IKEA chair, "Procent", appears not to contain steel apart from
a
: small
: } } amount in the castors (at least according to the IKEA website).
Does
: } } anyone have any experience with this chair?
: } }
: } } Does anyone have an alternative suggestion for a non-magnetic
chair
: } } suitable for microscopy? It would be preferable if this chair
was
: } } available in the UK.
: } }
: } } Best wishes
: } }
: } } --
: } } Ian MacLaren
: } } Department of Physics and Astronomy
: } } University of Glasgow
: } } Glasgow G12 8QQ
: } } Scotland
: } } http://www.physics.gla.ac.uk/~maclariz/
: }
: }
: }
:
:
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 12 14:03:48 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello,
Last week we had a power problem (a short) in the power supply to the
computer controlling a XL30 ESEM. Earlier (3 months) older system, had a
similar power failure on a power strip inside an electroscan ESEM
installed on the same power outlet. I'm thinking that there is a problem
in the 208 voltage line that causes spikes or something to blow out the
power supplies. Anyone have any ideas on ways the voltage can be
regulated/filtered to reduce the likelihood of this happening again?

For computers, I use UPS which filters out most of the voltage spikes. I
don't know what would be possible with a big scanning electron microscope
using 208/230 Volts and probably a huge amount of amps.
Any advice appreciated.
Thanks

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 12 15:28:32 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Gordon;

Check with the SEM manufacturer and see what they recommend. The fact
that it runs on 208 volts should not be an issue and all you may need is
something like a surge suppressor or line regulator.

One thing I would check immediately is how well your microscope is
grounded and by that I mean the earth ground. You can have voltage
offsets on the neutral leg of the power line if the instrument grounding
is poor which may lead to some of your issues. I'm sure Berkeley has an
electrician or two that can help.

Regards,

Peter Tomic
Agere Systems

-----Original Message-----
} From: Gordon Vrololjak [mailto:gvrdolja-at-nature.Berkeley.EDU]
Sent: Monday, July 12, 2004 3:07 PM
To: microscopy-at-msa.microscopy.com

Hello,
Last week we had a power problem (a short) in the power supply to the
computer controlling a XL30 ESEM. Earlier (3 months) older system, had
a similar power failure on a power strip inside an electroscan ESEM
installed on the same power outlet. I'm thinking that there is a
problem in the 208 voltage line that causes spikes or something to blow
out the power supplies. Anyone have any ideas on ways the voltage can
be regulated/filtered to reduce the likelihood of this happening again?

For computers, I use UPS which filters out most of the voltage spikes.
I don't know what would be possible with a big scanning electron
microscope using 208/230 Volts and probably a huge amount of amps. Any
advice appreciated. Thanks

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/
\/\/\
Gordon Ante Vrdoljak Electron
Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA
94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 02:26:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

You should first check with the plant facilities people. There are a
variety of issues here and in a facility like yours they probably start
with its age. As a facility, and the area around it, grows over the years,
they often strain the local power distribution system. Also, building
wiring and connections age causing increased resistance to the electrical
power. The power grid both sources and sinks current. In other words, you
can take power out and put it in - case in point, you've probably heard of
people using wind or solar energy for power and selling excess back to the
grid.

This ability of the grid to sink current can often mask very normal
problems. Inductive loads, such as motors used for HVAC and pumps, can
produce high voltage spikes that are normally absorbed by the grid. But,
when the resistance to the grid gets high enough in building wires and
power distribution wiring, those spikes can have a greater local effect
since they are absorbed less by the grid.

Peter's comments are a little off - no offense intended, they are common
misconceptions. The neutral and hot wires come directly from the power
grid. Along the way, there will be boost and step-down transformers that
adjust the voltage. At each of these, the output will have the neutral
side connected to a ground. On long stretches of wires the neutral will
also be occasionally connected to ground. The idea is that the neutral
will be close to the local ground potential, but not necessarily the same,
at any location nearby. This actually creates a problem that many people
have experienced - lightning strike damage. As crazy as it sounds, most
electrical failures from lightning strikes are actually caused by the
strike raising the potential of the local ground, rather than a direct hit
on a power line. While the potential to the ground can vary, the potential
between the hot and neutral lines is set by the power company and the
various transformers along the way.

The concept here is that the hot line brings power to the building and the
neutral carries it back. These connections from the grid are almost always
very reliable and consistent. The ground connection is a locally grounded
connection, usually an intimate ground connection made near where the hot
and neutral lines enter a building. The neutral may or may not be
connected to that local ground.

The ground connection is normally a human safety consideration. In both
consumer and industrial products you have two types of protection for
electrical shock - grounded frame and double insulated. SEMs are generally
of the grounded frame type where the outside of the machine is a metal case
that is connected to the local ground. Should you contact the frame and a
locally grounded object, such as a water drain, you hopefully won't
experience the discomfort of a current passing through your body since they
are at similar potentials. Double insulated machines generally have a p
lastic exterior that provides insulation from any electrical currents
contained within, once again preventing you, as the operator, from
experiencing any discomfort by making an electrical connection with
internal currents.

Now, in an instrument like an SEM, both the power and neutral will be well
isolated from the ground. They generally are wired to the primaries of
transformers whose outputs lead to power supplies. The outputs of those
supplies generally have a connection to the instrument ground which is
connected to the local ground, but there is at least a 1500V isolation
between that instrument ground and the hot or neutral lines. Grounding of
the instrument frame, or chassis ground as it is known to EEs, has no real
normal connection to the power grid neutral. Instead, it is used as a
human protective means to avoid exposure to voltages that could cause
adverse currents should a locally grounded conductor be contacted at the
same time.

Having said all of that, the extremely sensitive instruments we work with
have a special problem with local grounds. Since any electrical current
generates a magnetic field and magnetic fields affect the path of moving
charges, we can have a problem with 'ground loops'. These affect the
imaging capabilities of SEMs by inducing noise and are the result of
differences in the ground potential on various portions of the instrument.
Basically, all chassis grounds of the various frame components of an SEM
should have a singular source - a connection at one point that is truly
representative of a local ground.

On to practical solutions to the original problem. Once again, start with
your institution's facilities people. It may be a challenge to them, but
let it be. Any problems you are experiencing are probably a problem of
local building wiring or local power grid utilization. If it can't be
solved there, you have alternatives in power conditioning solutions. The
fact that you are running at 208 volts actually make this easier and
cheaper as the current requirements of your instrument are nearly half what
they would be if it were running at 120 volts. However, 208 volt systems
are fairly unusual. Check with the manufacturer or service organization to
see if your instrument can be easily changed to 240 volts. Conditioning
systems, including full uninteruptable power systems are available, though
expensive at these currents, for more standard 120 or 240 volt systems.

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174

phone (630) 513-7093 fax (630) 513-7092 http://www.sem.com

On Monday, July 12, 2004 3:31 PM, Tomic, Peter (Peter)
[SMTP:ptomic-at-agere.com] wrote:
}
}
}
------------------------------------------------------------------------
------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
-------
}
} Gordon;
}
} Check with the SEM manufacturer and see what they recommend. The fact
} that it runs on 208 volts should not be an issue and all you may need is
} something like a surge suppressor or line regulator.
}
} One thing I would check immediately is how well your microscope is
} grounded and by that I mean the earth ground. You can have voltage
} offsets on the neutral leg of the power line if the instrument grounding
} is poor which may lead to some of your issues. I'm sure Berkeley has an
} electrician or two that can help.
}
} Regards,
}
} Peter Tomic
} Agere Systems
}
} -----Original Message-----
} } From: Gordon Vrololjak [mailto:gvrdolja-at-nature.Berkeley.EDU]
} Sent: Monday, July 12, 2004 3:07 PM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy] voltage problems
}
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ------------------------------------------------------------------------
} -------
}
} Hello,
} Last week we had a power problem (a short) in the power supply to the
} computer controlling a XL30 ESEM. Earlier (3 months) older system, had
} a similar power failure on a power strip inside an electroscan ESEM
} installed on the same power outlet. I'm thinking that there is a
} problem in the 208 voltage line that causes spikes or something to blow
} out the power supplies. Anyone have any ideas on ways the voltage can
} be regulated/filtered to reduce the likelihood of this happening again?
}
} For computers, I use UPS which filters out most of the voltage spikes.
} I don't know what would be possible with a big scanning electron
} microscope using 208/230 Volts and probably a huge amount of amps. Any
} advice appreciated. Thanks
}
} \/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/
} \/\/\
} Gordon Ante Vrdoljak Electron
} Microscope Lab
} ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
} gvrdolja-at-nature.berkeley.edu UC Berkeley
} phone (510) 642-2085 Berkeley CA
} 94720-3330
} fax (510) 643-6207 cell (510) 290-6793
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 13:11:11 2004

Contents Retrieved from Microscopy Listserver Archives
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I have UPS from Toshiba (1400XL Plus Series) installed for
XL30 ESEM. Works fine (I had a lot of short power outages
during building renovation).

Regards,

Vladimir

} Hello,
} Last week we had a power problem (a short) in the power
} supply to the computer controlling a XL30 ESEM. Earlier (3
} months) older system, had a similar power failure on a power
} strip inside an electroscan ESEM installed on the same power
} outlet. I'm thinking that there is a problem in the 208
} voltage line that causes spikes or something to blow out the
} power supplies. Anyone have any ideas on ways the voltage
} can be regulated/filtered to reduce the likelihood of this
} happening again?
}
} For computers, I use UPS which filters out most of the
} voltage spikes. I don't know what would be possible with a
} big scanning electron microscope using 208/230 Volts and
} probably a huge amount of amps. Any advice appreciated. Thanks
}
} \/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/
} \/\/\/\/\/\/\/\
} Gordon Ante Vrdoljak
} Electron Microscope Lab
} ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
} gvrdolja-at-nature.berkeley.edu UC Berkeley
} phone (510) 642-2085
} Berkeley CA 94720-3330
} fax (510) 643-6207 cell (510) 290-6793
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 14:34:43 2004

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Hello Timo,

Below is a condensed alignment procedure for the
bottom stage. To align the upper stage select the
Stage 1 functions and follow the same procedure. You
should achive magnifications over 100,000X easily with
a LaB6 at ~15kV in the bottom stage and
200,000-300,000X in the upper stage. For the sake of
brevity I left out a lot of information. Let me know
if this suffices.

ISI DS 130C Dual Stage Scanning Electron Microscope
Alignment Procedures

Description of Console:

Upper Left:
Gamma correction for CRT A (left) and B (right)

Upper Left Center:
Scan Modes: Spot: For EDS/WDS
Line: Wave Form only works with slow scan speed
PIC: Normal Imaging
LP: Line Profile
EXT: External Port (e.g. Backscatter Detector if
attached)

Upper Center:
Selected Area: SA: controlled by Position-xy and
Width-xy knobs.
Signal Processing: Off for normal SEI imaging
Derivative: For positive and negative mixing (Set to
Normal)
Y-modulation: Changes normal Z-modulated image to
modulation of the Y-axis (bright areas are vertical).

Upper Right:
Alignment 1: Shift xy and tilt xy: For Upper Stage 1
Gun Alignment
Alignment 2: For Lower Stage 2 Gun Alignment
Focal Depth: For Upper Stage 1: 1 = High Resolution
(HR) 2 = Normal

Lower Left:
Brightness Contrast controls for illumination of CRT
monitors A and B.
Scan Rotation and Tilt Correction for image
orientation
Image Shift xy for fine movement
Scan Speeds: Rapid R1 and R2 and Slow Scan S1 and S2

Lower Center:
Magnification knob with digital readout
Dual Mag with Split Screen S with X1 to X10 for
magnification of split image
Select Dual D X1 mode for normal operation.
Monitor selection A left and B right as active CRT
EXT mode for selection of External detector (e.g. BEI
detector)
STM = STEM mode
XRY = Diffraction mode
Detector HT: Depress for normal viewing
Stage selection: 1st (upper) or 2nd (lower)
Focus Fine and Course
Stigmator xy for astigmatism; Neutral=5

Function: Probe Current Selection:
HR = High Resolution
STD = Standard Probe Current
LM = Low Magnification in 1st Stage
LCT = Large Current
ECP = Electron Channeling Pattern
FR = Free Function (Full Clockwise = Maximum Current)
Spot Size LS = Large and Small (Fine adjustment of
probe current)

Lower Right:
FIL: Filament; Depress for normal operation
Filament image: Off for normal operation; Depress for
checking saturation during alignment
Filament knob for controlling saturation

Normal Alignment for 2nd Stage with LaB6 Filament

Preliminary Settings:
Stage = 2nd
Function = STD
Dual D X1
Stigmators X and Y = 5
Mode = PIC
Monitors A & B = SEI
Detector HT Depressed
FIL Depressed
Center alignment knobs (Gun shift/tilt and Alignment 1
& 2 shift/tilt): To do this rotate knob completely
clockwise. Determine the number of counterclockwise
rotations until stopped. Rotate clockwise half the
number of counted rotations.
Start at 10-15mm working distance.

Alignment:
Depress HT on LaB6 box if applicable
Depress FIL image.
Function = LM
Coarse Saturation:
§ Increase current slowly with Filament Knob (with
LaB6 the current is increased a notch ~every 2-3
minutes) until spot appears. Saturate spot to the
sharpest/brightest point. Center spot with Gun
alignment tilt xy.
Fine Saturation:
§ Scan mode = Line
§ Waveform monitor = A
§ Scan Speed = S2
§ Memorize this: Line/A/S2 because you repeat do this
step constantly during imaging as the DS-130 is not a
stable instrument.
§ Center waveform on the CRT with the
brightness/contrast knobs
§ Bring filament to saturation with Filament Knob.
This is a peak maxim. There is no plateau as in other
SEMs
§ Maximize peaks with Gun Alignment Tilt xy. Use Tilt
only Do not use Gun Shift.
Repeat fine saturation procedure until optimized.

Focus:
Achieve best focus with focus knob.
Turn focus knob counter clockwise slightly.
Notice direction of image shift (e.g. up and right)
Turn focus back to best focus.
Shift the image in the same direction (e.g. up and
right) using Alignment 2 tilt x & y knobs at upper
right console
Repeat focus steps at increasing magnifications until
shift is negligible
Stigmate with stigmate x & y knobs until image is
crisp.

You must repeat the fine saturation and focus
procedures each time you change the probe current or
kV and whenever the current becomes unstable (which is
often).

Patricia J. Nelson
Characterization & Analytical Services
Strategic Technologies
Engelhard Corporation
Iselin, NJ 08830-0770
(732) 205-5217

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 16:12:54 2004

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Hi folks,

Just setting up a computerized image capture system for an ISI SX-30e and
was wondering if anyone knew a good place to grab the SE and/or video
signal?

Thanks,

Sandeep

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 16:14:18 2004

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This manufacturer is worth a look. They have apparently supplied to Gatan's demo
lab, among others.

No financial interest.

Chris

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 16:16:04 2004

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This manufacturer is worth a look. They have apparently supplied to Gatan's demo
lab, among others.

www.magnotix.com

No financial interest.

Chris

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 17:18:42 2004

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While you might be able to clean up your power source, I suggest you also
consider the possibility that the power supply within the XL30 ESEM simply
was not properly designed to work with 208/230 Volts. I once worked for a
company where we shipped product with a power supply that meets this
unfortunate description. Details follow.

I suggest that you contact the OEM. You might ask if the product was
tested to operate at 208/230 under simulated brown out conditions. There
are modifications to switching power supplys that may be made to accommodate
your voltage requirement and allow more reliable operation.

Anything plugged directly into the local power grid is subject to "brown
outs", which can stress a power supply. Brown outs result from current
being delivered through a power company's transformer. When current load
increases, transformers switch from a certain number of windings to a
different number to accommodate the voltage drop over the power transmission
line. This is specified to happen within a certain time, i.e. less than one
cycle, i.e. less than 1/60 seconds. Switching power supplies that power
your equipment must accommodate this brown out. Moreover, the stress
imposed upon components of the switching power supply is different depending
on the operating voltage.

One product that I was shipping to customers years ago incorporated a 3rd
party designed switching power supply which gave intermittent failures when
operating in the United Kingdom. No problem operating at other line
voltages in other countries. Although the power supply was designed to
operate over a wide range of voltages, it was not tested under common
condition of "brown out" at the United Kingdom operating voltage. Continued
shipments to that country required several conversations and a bit of action
by the manufacturer of the switching power supply.

Good luck,
John Moore

----- Original Message -----
} From: "Dusevich, Vladimir" {DusevichV-at-umkc.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Tuesday, July 13, 2004 2:14 PM

I have UPS from Toshiba (1400XL Plus Series) installed for
XL30 ESEM. Works fine (I had a lot of short power outages
during building renovation).

Regards,

Vladimir

} Hello,
} Last week we had a power problem (a short) in the power
} supply to the computer controlling a XL30 ESEM. Earlier (3
} months) older system, had a similar power failure on a power
} strip inside an electroscan ESEM installed on the same power
} outlet. I'm thinking that there is a problem in the 208
} voltage line that causes spikes or something to blow out the
} power supplies. Anyone have any ideas on ways the voltage
} can be regulated/filtered to reduce the likelihood of this
} happening again?
}
} For computers, I use UPS which filters out most of the
} voltage spikes. I don't know what would be possible with a
} big scanning electron microscope using 208/230 Volts and
} probably a huge amount of amps. Any advice appreciated. Thanks
}
} \/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/
} \/\/\/\/\/\/\/\
} Gordon Ante Vrdoljak
} Electron Microscope Lab
} ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
} gvrdolja-at-nature.berkeley.edu UC Berkeley
} phone (510) 642-2085
} Berkeley CA 94720-3330
} fax (510) 643-6207 cell (510) 290-6793
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 13 19:11:00 2004

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Isn't the 208 simply the voltage, in the US, between any two phases of a three-phase
mains supply?

Here, in NZ, where the domestic single phase voltage (ie between any phase and
neutral) is 230, the voltage between two phases is 400, so I guess that the US, with its
phase-to-neutral voltage of 115, the voltage between two phases would be about 200,
or maybe 208.

Most major manufacturers have links and jumpers in the primaries of their power
transformers to cope with the wide variety of supply voltages which occur
internationally.

I don't see that there is anything 'unfortunate' about that description, but one always has
to check that the gear is, in fact, correctly set up for the local conditions.

You will probably get brownout problems if the links are set for 230/240 and the
instrument is hooked up between the phases of a US supply. Better to set it for 110 and
rune it between the phase and neutral.

What country are you in, John?

cheers

rtch

} From: "John" {jmontara-at-earthlink.net}
To: {microscopy-at-msa.microscopy.com}

Hi, All-

Long story, but someone in a tech company here just discovered they have
an Amray 1820 sitting in a crate on Kauai. I'm not familiar enough with
Amray models to know if this is an instrument that is worth setting up or
not. We're fishing for opinions, contacts, etc.

Mahalo!
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 08:05:23 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (muchphoto-at-Earthlink.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Wednesday, July 14, 2004 at 07:35:29
---------------------------------------------------------------------------

Email: muchphoto-at-Earthlink.net
Name: Michael Reese Much

Education: Undergraduate College

Location: Bethlehem, PA, USA

Question: I have some Canada Balsam which seems very thick. Any recommendations on lower its viscosity. Mike

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From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 08:06:18 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (stephanie.l.mccracken-at-medtronic.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 13, 2004 at 10:52:18
---------------------------------------------------------------------------

Email: stephanie.l.mccracken-at-medtronic.com
Name: Stephanie

Title-Subject: [Microscopy] [Filtered] MListserver:titanium oxide etch?

Question: Does anyone know of a good titanium oxide etch? I am trying to sort out areas of titanium oxide from clean titanium. Chemical or plasma options are available to me. Any ideas?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 08:07:20 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sam.lawrence-at-aetostech.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, July 12, 2004 at 18:36:16
---------------------------------------------------------------------------

Email: sam.lawrence-at-aetostech.com
Name: Sam Lawrence

Organization: Aetos Technologies, Inc.

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Aetos Technologies, Inc. is seeking a highly motivated individual capable of providing advanced technical applications and technical sales support for our High Resolution Optical Microscope product line. The successful applicant will have extensive practical experience using research-level microscopes in a variety of biological research applications (3-5 years full time). Strong people and presentation skills, both verbal and written, are essential. A bachelor's or graduate degree in the biological or optical sciences is required. Business experience is a plus.

Travel up to 30% may be required. Starting date is late summer 2004. Company is located in a Southeastern U.S. university town with an excellent quality of life. Relocation is required. Compensation will be commensurate with training and experience.

Interested individuals should send resume, short sample of writing/training materials and references (up to 3) to {mailto:sam.lawrence-at-aetostech.com} sam.lawrence-at-aetostech.com. We are an equal opportunity employer.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 12:25:52 2004

Contents Retrieved from Microscopy Listserver Archives
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Listers,

Hitachi EMs with LaB6 emitters use a special (" ") ammeter for
checking current to the emitter, degassing a new crystal, and so
forth. Inside that big box is a regular Yokogawa 0 to 3 Amp analog
ammeter, model number 2011.
Ours got fried by a power spike, so I'm trying to find a replacement,
preferably a good, used one. Does anyone have an orphan ammeter, in
the Hitachi box or out, perhaps from a LaB6 instrument that has been
decommissioned?
Thanks.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 12:27:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,

I was wondering if anyone can recommend a good course/seminar on failure analysis techniques, mostly as they pertain to materials science/metallurgy and microscopy?

Thanks,

Jane LaGoy
R&D Engineer
Bodycote HIP, Inc.
155 River St.
Andover, MA 01810
jlagoy-at-bodycote-imt.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 13:50:07 2004

Contents Retrieved from Microscopy Listserver Archives
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Have you tried plasma treatment with CF4 only? Normally, it is recommended to use CF4 with about 10% O2, but since you don't want to oxidize the Ti metal, try just the CF4. Or you might want to try CF4+O2 and then switch to CF4 only to finish.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: stephanie.l.mccracken-at-medtronic.com
[mailto:stephanie.l.mccracken-at-medtronic.com]
Sent: Wednesday, July 14, 2004 9:10 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (stephanie.l.mccracken-at-medtronic.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 13, 2004 at 10:52:18
---------------------------------------------------------------------------

Email: stephanie.l.mccracken-at-medtronic.com
Name: Stephanie

Title-Subject: [Microscopy] [Filtered] MListserver:titanium oxide etch?

Question: Does anyone know of a good titanium oxide etch? I am trying to sort out areas of titanium oxide from clean titanium. Chemical or plasma options are available to me. Any ideas?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 14:30:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Check with the Buehler, Ltd. people (http://www.buehler.com), Allied
High Tech (www.alliedhightech.com) or ASM International
(http://www.asminternational.org). ASM is a society heavily weighted
with metallurgists and they offer some good course.

tantalum73-at-juno.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 15:29:51 2004

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ASM offers an excellent course called "Principles of
Failure Analysis". I took one 20 years ago and credit
this course for helping to launch my career in
metallurgical failure analysis. Though microscopy is
only part of this course, it thoroughly covers the
microscopy techniques needed for failure analysis.

http://www.asminternational.org/

http://www.asminternational.org/Template.cfm?Section=CourseCalendar&Template=/Calendar/CalendarEventList.cfm&list=false&training=1

Stu Smalinskas, P.E.
Metallurgist
SKF USA
Plymouth, Michigan
(734) 414-6862

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Jane wrote:

Hello,

I was wondering if anyone can recommend a good
course/seminar on failure analysis techniques, mostly
as they pertain to materials science/metallurgy and
microscopy?

Thanks,

Jane LaGoy
R&D Engineer
Bodycote HIP, Inc.
155 River St.
Andover, MA 01810
jlagoy-at-bodycote-imt.com

__________________________________
Do you Yahoo!?
Yahoo! Mail - Helps protect you from nasty viruses.
http://promotions.yahoo.com/new_mail

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 15:48:58 2004

Contents Retrieved from Microscopy Listserver Archives
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The best short courses for failure analysis and other materials
science/metallurgy related areas are provided by ASM International. They
have a variety of courses at different levels relating to failure
analysis. None specifically emphasize microscopy, but some include
microscopy topics with lab experiences with LM and SEM on fractures and
microstructures. Courses are offered mostly in Ohio plus less frequently
at a few other locations. Some are available as home study.

The ASM fall meeting - this year in Columbus, OH has three days of
technical programming on failure analysis, but not necessarily
microscopy oriented. The ASM/IMS conference, early August in Savannah,
also has some FA programming with a strong microscopy emphasis.

Info on all of this is at the ASM web site -
http://www.asminternational.org\

--
Larry D. Hanke, P.E.
Materials Evaluation and Engineering, Inc.
Practical Solutions Through Technology and Innovation
http://www.mee-inc.com (763) 449-8870

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 14 17:02:14 2004

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Becky,

Check out the following courses offered by ASM International. I found
them by performing a keyword search at
http://www.asminternational.org/Template.cfm?Section=BrowsebyTopic&Template=
ConferenceTopiclist.cfm using the keyword failure.

Applied Techniques for Failure Analysis
Failure Analysis of Tools and Dies
Failure Evaluation, Life Assessment & Life Extension of Equipment
How to Organize and Run a Failure Investigation
How to Organize and Run a Failure Investigation
Key Concepts in Reviewing and Doing Failure Analysis Work
Principles of Failure Analysis
Principles of Failure Analysis Online
The Role of the Atomic Force Microscope in Failure and Yield Analysis

Jeff Stewart
Metallographic Laboratory Manager
Stern-Leach Company
49 Pearl Street
Attleboro, MA 02703
Voice: 508-222-7400 x1329
Fax: 508-699-4030
email: jeff-at-metallography.com
Founder/Webmaster
www.metallography.com

----- Original Message -----
} From: "Becky Holdford" {r-holdford-at-ti.com}
To: {tantalum73-at-juno.com}
Cc: {Microscopy-at-MSA.Microscopy.com}
Sent: Wednesday, July 14, 2004 3:33 PM

--------------------------------------------------------------
MMMS - Midwest Microscopy and Microanalysis Society
Affiliate of the Microscopy Society of America and the Microbeam
Society of America
--------------------------------------------------------------

Presents

Investigations in Microscopy

Friday, July 23, 2004

Free to MMMS members: Regular Membership $10, Student Membership $5
(Membership applications will be accepted at the meeting)

USG Research and Technology Center
700 N. Highway 45
Libertyville, IL 60048

RSVP by Wednesday, July 16, 2004
Arvid Casler
MMMS Program Coordinator
847-566-7716 Voice Mail and Fax
arvid_casler-at-fmo.com

--------------------------------------------------------------
Seminar Schedule
--------------------------------------------------------------

1:00 PM - 1:30 PM Setup and Registration

1:30 PM - 1:40 PM Dr. Brett Link
Associate Lab Director of the Formulated Products Laboratory
USG Research Technology Ctr.
Welcome

1:40 PM - 2:40PM Wayne Niemeyer
McCrone Associates, Inc.
Analytical Microscopy - The Identification of "Invisible
Clues from a Microscopic World"

2:45 PM - 3:00 PM Robb Mierzwa
MMMS President
Microscopy and Microanalysis 2006 at Chicago's Navy Pier

3:00 PM Art Struss
USG Research Technology Ctr.
Microscopy of Building Materials at USG

Reception to Follow

Robert Mierzwa
Midwest Regional Sales Manager
JEOL USA, Inc.
3906 Lisa Ave.
Sheboygan WI 53083
TEL (920) 803-8945
FAX (920) 803-8946
Email: mierzwa-at-jeol.com {mailto:mierzwa-at-jeol.com}

JEOL Products: http://www.jeol.com/eo.html

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 15 11:42:46 2004

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Dear Listers
I have a grad student in anthology who wishes to examine cross sections of
Peruvian mummy hair to answer some questions about trace element nutrition.
SEM-EDX has been unsatisfactory (issue of elemental resolution) so our
Surface Science Group here at UWO has suggested the use of TOF-SIMS.
There are a few constraints/requirements on the sample preparation -
1) sample must not be rehydrated to prevent dis/re-location of trace
elements
2) Cross sections are required
3) for best TOF-SIMS results surface of sections needs to be as smooth as
possible
4) embedded using typical wax or plastic methods to be avoided (see 1)above)
5) sections could be as thick as 50-100 micrometers
Any suggestions would be welcomed.
Thanks in advance...
Rick
Richard Harris
Laboratory Supervisor
Department of Biology
University of Western Ontario
London Ontario CANADA
Ph. 519-661-2111 ext. 86780
Fax 519-661-3935

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 15 19:17:21 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (purplechalkdust-at-sbcglobal.net) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, July 15, 2004 at 11:17:51
---------------------------------------------------------------------------

Email: purplechalkdust-at-sbcglobal.net
Name: Sonjia Primous

Organization: teacher

Title-Subject: [Microscopy] [Filtered] microscopy-based lessons and activities

Question: Hello
I am looking for lessons and activities that I can implement in my fifth grade classroom. I was just given a class set on microscopes and would like to center my science curriculum around them for the upcoming school year. I am part of a teacher intern program through Argonne National Laboratory in Illinois, and I am looking for assistance in the area of microscopy.

Thank you for your time, and I hope to hear a reply soon,
Sonjia Primous

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From MicroscopyL-request-at-ns.microscopy.com Thu Jul 15 19:26:07 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (elosalga2002-at-yahoo.com) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Thursday, July 15, 2004 at 14:10:43
---------------------------------------------------------------------------

Email: elosalga2002-at-yahoo.com
Name: Salgado , Eloisa

Education: Undergraduate College

Location: Tegucigalpa, Honduras

Question:
I do not have much experience in fluorescence microscopes. I do like to know more about this

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From MicroscopyL-request-at-ns.microscopy.com Thu Jul 15 20:40:22 2004

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Hi All,

I have a couple of questions from a researcher in Australia,
hopefully someone out there may be able to help.

She has developed a technique for staining cultured cells for Al
which is present in parts per billion concentrations. The technique
appears to be able to show where the Al is in the samples. However
she needs to independently confirm these results with another
technique.

Ideally the Al, and other elements, would be mapped with micron
spatial resolution.

LAMMA (laser assisted micro mass analysis) has been suggested as a
possible technique. Is LAMMA available in Australia and who should
we talk with? If not, who else in the world should we contact?

Are there other techniques (preferably available in Australia) which
may be suitable? Nanosims may be a possibility.

Any feedback would be appreciated. Cheers,

Mark Blackford

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 15 22:40:20 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (frah0010-at-tc.umn.edu) from http://microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Thursday, July 15, 2004 at 22:28:03
---------------------------------------------------------------------------

Email: frah0010-at-tc.umn.edu
Name: Ellery Frahm

Organization: University of Minnesota, Electron Microprobe Lab

Education: Graduate College

Location: Minneapolis, Minnesota

Question: Hello all,

I teach a course called "Electron Microprobe Theory and Practice" here at the University of Minnesota, and I've decided to shake up the reading packet for the course a bit -- I and my students can tire of the textbook chapters rather quickly in the semester. I'd like to add some papers or articles that would be interesting to students new to the electron microprobe -- I'd like papers that involve history and development, others that involve debates, others that are just considered "core" to the field. I have a few papers in mind, but I thought I'd tap the expertise of this listserve for suggestions. Any ideas and suggestions are welcome.

Thanks in advance,

Ellery

--------------------
Ellery E. Frahm
Research Scientist/Manager
Electron Microprobe Laboratory
University of Minnesota - Twin Cities
Department of Geology & Geophysics
Lab Website: htt://probelab.geo.umn.edu

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From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 07:03:29 2004

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Dear Eloisa,

Please try these web sites for introduction. Then, it will be
time to ask us some more about microscopy.

Nikon Microscopy U
http://www.microscopyu.com/

Optical Microscopy Primer
http://micro.magnet.fsu.edu/primer/

WWW Virtual Library:Microscopy
http://www.ou.edu/research/electron/www-vl/

Cheers and good luck,

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SSS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:elosalga2002-at-yahoo.com]
Sent: Thursday, July 15, 2004 8:29 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (elosalga2002-at-yahoo.com) from
http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on
Thursday, July 15, 2004 at 14:10:43
------------------------------------------------------------------------
---

Email: elosalga2002-at-yahoo.com
Name: Salgado , Eloisa

Education: Undergraduate College

Location: Tegucigalpa, Honduras

Question:
I do not have much experience in fluorescence microscopes. I do like to
know more about this

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 07:35:53 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Morning Ms. Primous,

You can start by getting your introduction from the excellent
sites listed below.

Nikon Microscopy U
http://www.microscopyu.com/

Optical Microscopy Primer
http://micro.magnet.fsu.edu/primer/

WWW Virtual Library:Microscopy
http://www.ou.edu/research/electron/www-vl/

Here's LessonPlanet.COM:
http://www.lessonplanet.com/search/Science/Biology/Microscopes

Digital microscopy for $45, if you can find one anymore
http://www.teacherlink.org/content/science/microscope/frlp.htm

Hope this helps,

Fred Monson

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SSS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: by way of MicroscopyListserver
[mailto:purplechalkdust-at-sbcglobal.net]
Sent: Thursday, July 15, 2004 8:20 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (purplechalkdust-at-sbcglobal.net) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, July 15, 2004 at 11:17:51
------------------------------------------------------------------------
---

Email: purplechalkdust-at-sbcglobal.net
Name: Sonjia Primous

Organization: teacher

Title-Subject: [Microscopy] [Filtered] microscopy-based lessons and
activities

Question: Hello
I am looking for lessons and activities that I can implement in my
fifth grade classroom. I was just given a class set on microscopes and
would like to center my science curriculum around them for the upcoming
school year. I am part of a teacher intern program through Argonne
National Laboratory in Illinois, and I am looking for assistance in the
area of microscopy.

Thank you for your time, and I hope to hear a reply soon, Sonjia Primous

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 07:42:18 2004

Contents Retrieved from Microscopy Listserver Archives
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Bonjour Dear Listers,

I will like to localize quantitatively by cytochemistry ( if possible)
phenolic compounds in bacteria for studies with light and or electron
microscopy. These specific phenolic compounds are presents in bacteria
only in particular conditions. Do you have some methods or reference for
me. It is possible also for me to use fluorescence (epi and confocal) for
this study .

Thanks and have a good day and a nice week-end.

Gilles Grondin

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 07:45:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kryan-at-xsil.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, July 16, 2004 at 05:52:00
---------------------------------------------------------------------------

Email: kryan-at-xsil.com
Name: Kieran Ryan

Organization: DCU

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi All,
I 'm having an imaging problem with a device I designed for my masters project hopefully someone out there may be able to help.

The device is for analysing optical fibres of about 120um diameter so achromatic microscope objectives. On high magnification images the image produced is fine, however on lower magnification images vignetting of the image occurs. What causes this vignetting seems to be linked to the illumination used. The system employs a coaxial illumination system to illuminate the optical fibre surface. The problem appears to be the spot sized formed by the illumination system isn't large enough to cover the entire FOV. My illumination system consists of an LED Condenser lens and fixed aperture. Is anybody familiar with this problem and can they help me solve it??
Thanks
Kieran Ryan

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From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 07:46:24 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rdiez-at-jhmi.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, July 16, 2004 at 07:33:55
---------------------------------------------------------------------------

Email: rdiez-at-jhmi.edu
Name: Roberto Diez

Organization: Johns Hopkins University

Title-Subject: [Microscopy] [Filtered] Custom antibodies wanted

Question: Hi all,
I need reliable antibodies for my protein of interest (uncharacterised). Has anyone had success ordering a customized antibody. I would be very greatful if some of you out there can share with me your experiences. What do I need to do first? How long did it take to produce the antibody? How good was the specificity and sensitivity. Were the antibodies good for Western blot, ELISA, microscopy, FACS,...? And last, but not least, what was the price tag?
Our laboratory does downstream work to large proteomics initiatives, and so we are often confronted to quest for antibodies against uncharacterized proteins. I'm sure many other labs are having this challenge. I'd like to hear from them as well.
Thanks in advance.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 10:34:13 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

RE: Custom antibodies

I understand your concerns; we were in the same situation a year ago. We now mostly work with one company that we find quite trustworthy and reliable called HyperOmics Farma (www.hyperomics.com).

Custom antibody services are quite varied in terms of the rapidity in production, quality of the antibodies produced, the hosts, the technical help (in preparing the antigens, etc...), and especially follow up services offered by these antibody providers. So you really want to be careful which you decide upon, especially as the custom antibodies are costly anywhere you go (usually starting at about $1000/AB).

We've tried quite a few places to raise antibodies to human plasma and intracellular protein antigens and actually we have had the most success interacting with HyperOmics Farma. They are a chicken-antibody company here in Canada. I had no idea antibodies were being made in chickens....actually the antibodies are purified from the eggs. The antibodies we received were of high affinity, highly specific and of high titer all of which was great for us and easy to work with. AND, the very best aspect was that the antibodies were made really fast....we received fully useable purified antibodies within 2 months (which is significantly less than 4-6 months in mammalian hosts) and for us time is really critical. We used them with great success for Western Blots, ELISAs, and immunofluorescence microscopy. Actually we obtained better results with the chicken antibodies than with rabbit or mouse antibodies we had made; the greater phylogenetic distance between chickens & mammals has a lot to do with that, i.e, mammalian antigens are much more antigenic when injected in chicken hosts than when injected in mammalian hosts. We'd also considered phage display antibodies at one point but gave up on that idea based on the monovalent nature and consequent low affinity issues (and actually they were alot more expensive than regular antibodies made in animals).

The technical specialists were extremely helpful for us and that's really important actually when you offer 'custom' services. The prices were quite reasonable, starting at $650/Ab for small quantities. If you're interested, I think they offer the possibility of banking your antibodies for future commercialization (with royalties to the original investigators - this might be interesting for your customers at Johns Hopkins).

Good Luck!!

Sophie Dahan, Ph.D.
Program Leader & Senior Scientist,
Caprion Phamaceuticals,
Montreal, Quebec,

Tel: 514-940-3600 X3736
Fax: 514-940-3620

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 11:05:23 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

RE: Custom antibodies

I understand your concerns; we were in the same situation a year ago. We now mostly work with one company that we find quite trustworthy and reliable called HyperOmics Farma (www.hyperomics.com).

Custom antibody services are quite varied in terms of the rapidity in production, quality of the antibodies produced, the hosts, the technical help (in preparing the antigens, etc...), and especially follow up services offered by these antibody providers. So you really want to be careful which you decide upon, especially as the custom antibodies are costly anywhere you go (usually starting at about $1000/AB).

We've tried quite a few places to raise antibodies to human plasma and intracellular protein antigens and actually we have had the most success interacting with HyperOmics Farma. They are a chicken-antibody company here in Canada. I had no idea antibodies were being made in chickens....actually the antibodies are purified from the eggs. The antibodies we received were of high affinity, highly specific and of high titer all of which was great for us and easy to work with. AND, the very best aspect was that the antibodies were made really fast....we received fully useable purified antibodies within 2 months (which is significantly less than 4-6 months in mammalian hosts) and for us time is really critical. We used them with great success for Western Blots, ELISAs, and immunofluorescence microscopy. Actually we obtained better results with the chicken antibodies than with rabbit or mouse antibodies we had made; the greater phylogenetic distance between chickens & mammals has a lot to do with that, i.e, mammalian antigens are much more antigenic when injected in chicken hosts than when injected in mammalian hosts. We'd also considered phage display antibodies at one point but gave up on that idea based on the monovalent nature and consequent low affinity issues (and actually they were alot more expensive than regular antibodies made in animals).

The technical specialists were extremely helpful for us and that's really important actually when you offer 'custom' services. The prices were quite reasonable, starting at $650/Ab for small quantities. If you're interested, I think they offer the possibility of banking your antibodies for future commercialization (with royalties to the original investigators - this might be interesting for your customers at Johns Hopkins).

Good Luck!!

Sophie Dahan, Ph.D.
Program Leader & Senior Scientist,
Caprion Phamaceuticals,
Montreal, Quebec,

Tel: 514-940-3600 X3736
Fax: 514-940-3620

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 11:10:17 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Thank you so much Sophie.
I will definitely give this company a call. The website link was also
helpful. Thanks again.
Roberto

-----Original Message-----
} From: Sophie Dahan [mailto:sdahan-at-caprion.com]
Sent: Friday, July 16, 2004 11:14 AM
To: by way of MicroscopyListserver

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rdiez-at-jhmi.edu) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, July
16, 2004 at 07:33:55
---------------------------------------------------------------------------

Email: rdiez-at-jhmi.edu
Name: Roberto Diez

Organization: Johns Hopkins University

Title-Subject: [Microscopy] [Filtered] Custom antibodies wanted

Question: Hi all,
I need reliable antibodies for my protein of interest (uncharacterised).
Has anyone had success ordering a customized antibody. I would be very
greatful if some of you out there can share with me your experiences. What
do I need to do first? How long did it take to produce the antibody? How
good was the specificity and sensitivity. Were the antibodies good for
Western blot, ELISA, microscopy, FACS,...? And last, but not least, what
was the price tag?
Our laboratory does downstream work to large proteomics initiatives, and so
we are often confronted to quest for antibodies against uncharacterized
proteins. I'm sure many other labs are having this challenge. I'd like to
hear from them as well.
Thanks in advance.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 11:29:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

} Email: purplechalkdust-at-sbcglobal.net
} Name: Sonjia Primous
}
} Organization: teacher
}
} Title-Subject: [Microscopy] [Filtered] microscopy-based lessons and activities
}
} Question: Hello
} I am looking for lessons and activities that I can implement in
} my fifth grade classroom. I was just given a class set on
} microscopes and would like to center my science curriculum around
} them for the upcoming school year. I am part of a teacher intern
} program through Argonne National Laboratory in Illinois, and I am
} looking for assistance in the area of microscopy.
}
} Thank you for your time, and I hope to hear a reply soon,
} Sonjia Primous
}
} ---------------------------------------------------------------------------
Sonjia -

Since you've found "Ask-a-microscopist", you've been quite close to
the answer to your question; visit "Project MICRO" (URL below) and
look at the description of MSA's manual, "Microscopic Explorations";
it's for grades 5-8. It was written at the Lawrence Hall of Science
for their Great Explorations in Math and Science (GEMS) series, and
you'll find a helpful GEMS "Site" near you, in Greyslake (sp.?); see
MICRO for a link to a list of all of the GEMS Sites. You'll also
find a list of local MICRO programs there, and your local (Chicago)
coordinator, Joe Nielly of Abbott Labs, can find you a microscopist
to help during the school year.

If you have further questions, please contact me directly; I promise
detailed answers. I hope that you'll share your experiences with
your curriculum with MICRO!

Caroline

--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 12:27:35 2004

Contents Retrieved from Microscopy Listserver Archives
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I am soliciting possible platform presentations for inclusion into a
session on microscopy outreach and training for the 2005 meeting in
HAWAII. People planning to attend this meeting in between hitting
the beaches should consider participating in this session dedicated
to advancing the inclusion of microscopy and imaging in classrooms,
in the research lab, and among the lay public.

TEACHING MICROSCOPY AND IMAGING IN THE DIGITAL AGE

Computer technology is changing the ways we access equipment, view
samples, record, manage, and disseminate images. Inside the
laboratory, digital imaging has created the need for archiving
systems, for managing and manipulating images, and for creating new
digital tools to assist new users. Outside the lab, computer
controlled instruments and digital imaging make it possible for
classroom students to view and analyze microscopy data and images
without requiring physical access to distant microscopes. In
addition, digital imaging has greatly increased the possibilities for
the public at large to see microscopic images in print media and
museum exhibitions. This session will look at digital training
approaches (e.g., virtual microscopes and telemicroscopy) , new
teaching tools (digital training sessions), and outreach programs in
classrooms and other public venues.

--
Dr. Steven Barlow
EM Facility/Biology Dept.
San Diego State University
5500 Campanile Drive
San Diego CA 92182-4614
phone: (619) 594-4523
fax: (619) 594-5676
email: sbarlow-at-sunstroke.sdsu.edu
http://www.sci.sdsu.edu/emfacility

Chairman, Educational Outreach subcommittee
promoting microscopy instruction and increased access to microscopes
Microscopy Society of America
http://www.msa.microscopy.com/

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 16 13:26:24 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear researcher:

Can anyone lead me to a book or a site that shows TEM images of the
following cell types. If you have a "personal" collection of this type
of images, and do not mind to share with us, would you email them to me
off-line. One user of our facility is trying to identify cells in her
sample. Thank you in advance for your generous help.

1. Freshly isolated human blood basophils (not cultured)
2. Human plasmacytoid dendritic cells
3. Human myeloid dendritic cells
4. Human blood natural killer (NK) cells

Hong
Emory EM

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 18 12:12:53 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jcormier-at-mailcan.com) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Saturday, July 17, 2004 at 09:56:54
---------------------------------------------------------------------------

Email: jcormier-at-mailcan.com
Name: Justin Cormier

Organization: none

Education: Undergraduate College

Location: miami, FL USA

Question: I am curious about how one becomes a microscopist? How much school is needed? Is it very hard to find positions in microscopy? Do you like your job?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 18 14:53:12 2004

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} From: "Jim Wittig" {j.wittig-at-vanderbilt.edu}

--------------------------------
MSA Education Committee Announcement
M&M2004 Exhibitor Tutorials and Demos
August 3, 2004
Savannah, Ga.
http://mm2004.microscopy.org
--------------------------------

Once again the MSA Education Committee is organizing Exhibitor
Demonstrations and Tutorials at the MM2006 Meeting in Savannah (
http://mm2004.microscopy.org ) . This event will be held on Tuesday,
August 3 from 6:00 to 8:00 pm in the Exhibit Hall. These
mini-seminars or tutorial demonstrations are held in the booths of
the participating companies after the Hall is closed to
non-participants at ~ 5:00 pm.

Signup sheets with titles and descriptions are at the MSA Education
table in the MSA Mega Booth. When you sign up you will be issued a
ticket, which you will need to renter the Hall after it is closed.
You need to sign up no later than noon on Tuesday. The number of
attendees is limited, so visit the MSA Education table soon, since
the demonstrations get filled up quickly!

Here's the current list of participating Exhibitors and titles:

Bal-Tec AG
SEM Controlled Broad Ion Beam Sample Preparation

Chroma Technology Corp
Filter Design for Fluorescence Microscopy

Diatome U.S./Leica Microsystems
New Era in Ultramicrotomy: The Oscillating Diamond Knife and the
most advanced Ultramicrotome technology

EDAX/TSL
Simultaneous EBSD and EDS: See what you can do with a Chl-Scan System

HKL Technology
TBA

Imago Scientific Instruments Corporation
TBA

QuantomiX, Inc.
Electron Microscopy (SEM) of Fully Hydrated Samples - from Cell
Biology to Materials

Soft Imaging System
Automatic Strain Analysis of TEM/CBED Images

SPI Supplies
Osmium Plasma Coating for High Resolution FESEM Applications

Thermo Electron Corporation
1) Introduction to modern Raman microscopy as a routine analysis
tool for molecular characterization of materials
2)Better, Faster, Easier ways to acquire, process and present
compositional data

------------------------------
Stop by the MSA Megbooth for more details.
-------------------------------
"Jim Wittig" {j.wittig-at-vanderbilt.edu}

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 18 17:19:10 2004

Contents Retrieved from Microscopy Listserver Archives
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I do not know which kind of microscopist you want to be. If
you want to be an electron microscopsit, it will take a little
time to master the techniques. You could be a microscopsit
sooner or later after some practice.

It is hard to predict the future for the electron
microscopist, in particular for those with Ph.D degrees. It
seems to me that we need more and more microscopists. But many
companies or schools do not need electron microscopists with
very long professional experiences. I have more than 10 years'
experiences in TEM, but I still dare to say that I can find a
suitable job easily.

Changhui

---- Original message ----
} Date: Sun, 18 Jul 2004 12:19:58 -0500
} From: jcormier-at-mailcan.com (by way of Ask-A-Microscopist)
} Subject: [Microscopy] AskAMicroscopist: how one becomes a
microscopist
} To: microscopy-at-microscopy.com
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society
of America

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 18 23:20:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Justin

I love my job, it is want I wanted to do since I was a child trying to
observe snow by a toy-microscope spending time in the garden or using
home frige for preserving snow (unsucessfully), I lived in Verona that
period...

Basic studies always help including some optics then you can specialize
for a specific kind of microscope. A part from technical aspects and
theory of image formation, please do not forget an important chapter
that is SAMPLE preparation. This means you should also know about the
sample, investigating probe and sample interactions etc...

I was so lucky to have the opportunity to play and work with AFM, STM,
SNOM, SEM, acoustic, optical...optical and AFM are my favourite.

I think that in this period there is a good demand for
microscopists... probably in the future it will increase demand for
nanoscopits...
All my best
ALby
On 19 lug 2004, at 00:22, Changhui LEI wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} I do not know which kind of microscopist you want to be. If
} you want to be an electron microscopsit, it will take a little
} time to master the techniques. You could be a microscopsit
} sooner or later after some practice.
}
} It is hard to predict the future for the electron
} microscopist, in particular for those with Ph.D degrees. It
} seems to me that we need more and more microscopists. But many
} companies or schools do not need electron microscopists with
} very long professional experiences. I have more than 10 years'
} experiences in TEM, but I still dare to say that I can find a
} suitable job easily.
}
} Changhui
}
} ---- Original message ----
} } Date: Sun, 18 Jul 2004 12:19:58 -0500
} } From: jcormier-at-mailcan.com (by way of Ask-A-Microscopist)
} } Subject: [Microscopy] AskAMicroscopist: how one becomes a
} microscopist
} } To: microscopy-at-microscopy.com
} }
} }
} }
} } ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------
} } ---------
} }
} } Below is the result of your feedback form (NJZFM-ultra-55).
} It was submitted by (jcormier-at-mailcan.com) from
} http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
} on Saturday, July 17, 2004 at 09:56:54
} } ----------------------------------------------------------------------
} } -----
} }
} } Email: jcormier-at-mailcan.com
} } Name: Justin Cormier
} }
} } Organization: none
} }
} } Education: Undergraduate College
} }
} } Location: miami, FL USA
} }
} } Question: I am curious about how one becomes a microscopist?
} How much school is needed? Is it very hard to find positions
} in microscopy? Do you like your job?
} }
} } ----------------------------------------------------------------------
} } -----
} }
}
}
------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 05:41:45 2004

Contents Retrieved from Microscopy Listserver Archives
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In the UK you would be best to take a science degree and
then look for a vacancy. I actually did a PhD first. I now
run an electron microscope lab in a university. At the
time, 1989, there were no other applicants who attended the
interview - so one can get lucky! I love the job although
last night my wife encouraged me to look for one that pays
better!

Dave

On Sun, 18 Jul 2004 12:19:58 -0500 by way of
Ask-A-Microscopist {jcormier-at-mailcan.com} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jcormier-at-mailcan.com) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Saturday, July 17, 2004 at 09:56:54
} ---------------------------------------------------------------------------
}
} Email: jcormier-at-mailcan.com
} Name: Justin Cormier
}
} Organization: none
}
} Education: Undergraduate College
}
} Location: miami, FL USA
}
} Question: I am curious about how one becomes a microscopist? How much school is needed? Is it very hard to find positions in microscopy? Do you like your job?
}
} ---------------------------------------------------------------------------
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 07:35:26 2004

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We have 2 EM systems that are available for free. They were both under
service contract until a few years ago.

Philips TEM Model 300
Philips SEM Model 501

Please contact me directly for more details.

Thanks,

Steve Widing
Technical Coordinator
Biology Department
Temple University
Philadelphia, PA
email swiding-at-temple.edu
office 215-204-8840

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 08:58:03 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (g0305901-at-nus.edu.sg) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, July 19, 2004 at 08:54:44
---------------------------------------------------------------------------

Email: g0305901-at-nus.edu.sg
Name: chen jie

Organization: national university of singapore

Title-Subject: [Microscopy] [Filtered] a question about Transmission Electronic Microscope.

Question: Dear sir or Madam,

Now, I am doing some experiment through Transmission Electronic Microscope.
Could you tell me If the sample is dangerous after the samples are treated by

Osmium Tetroxide and then are embedded by Resin for 24 hours in 60 degree in oven ?If it is still harmful,how

to protect when the samples are trimed and sectioned for TEM?

thank you for your help!

chenjie

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 10:24:32 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello Listers:

Does anyone out there have the pads that sit under the older LKB type
ultramicrotomes? I remember they were covered in white plastic and there
were two per microtome.

Thanks

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 10:36:47 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello Listers:

Does anyone out there have the pads that sit under the older LKB type
ultramicrotomes? I remember they were covered in white plastic and there
were two per microtome.

Thanks

Karen

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 12:08:56 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear List,
I find myself with a reservation for a room at MSA that was obtained
as a double occupancy, and the other occupant has made other plans. If
anyone wants to share a room from 31 July through 4 August, please let
me know off list.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 17:26:12 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Jul 19, 2004, at 7:05 AM, by way of MicroscopyListserver wrote:

} Now, I am doing some experiment through Transmission Electronic
} Microscope.
} Could you tell me If the sample is dangerous after the samples are
} treated by
}
} Osmium Tetroxide and then are embedded by Resin for 24 hours in 60
} degree in oven ?If it is still harmful,how
}
} to protect when the samples are trimed and sectioned for TEM?
}
Dear Chen Jie,
It all depends on what the sample is. Most viruses and, I think, all
bacteria are killed by the fixation and embedding procedures and are no
longer dangerous; however, prions--e.g., the organism causing mad cow
disease--are not necessarily killed by the procedures. The real
experts in the field can tell you what precautions are necessary or
advisable when sectioning blocks containing pathologenic organisms (and
where I may have erred in my assessment).
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 23:10:14 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

} Date: Mon, 19 Jul 2004 18:27:24 -0700
} To: Microscopy ListServer
} From: Sergey Ryazantsev {sryazant-at-ucla.edu}
} Subject: [Microscopy] Re: LKB anti vibration pads
}
} Hello Karen
} I don't think those old pads would work: rubber tends deteriorate with
} age. You could made very effective anti-vibration pad by yourself. It's
} easy: find in some story (like OSH or Home Depot in USA) the sheet of
} rubber approximately 1-1.5 cm thick. It should be solid relatively hard
} rubber, not porous one. Cut the sheet on pieces of the size you need and
} stack them to create necessary height. If you will put a thin aluminum
} sheet (1 mm) between each rubber layer (same size as rubber), you'll
} create superior anti-vibrating pad! Good luck, Sergey.
}
} At 08:43 AM 7/19/2004, you wrote:
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 19 23:10:27 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

} Date: Mon, 19 Jul 2004 16:33:09 -0700
} To: Microscopy ListServer
} From: Sergey Ryazantsev {sryazant-at-ucla.edu}
} Subject: [Microscopy] Re: Re: Re: AskAMicroscopist: how one becomes a
} microscopist
}
} I really love my job. I think, EM (not necessary only EM) is good for
} people with natural curiosity: to see things smaller, smaller and
} smaller... sharper, sharper and sharper.... Curiosity, perhaps, is the
} reason to me to stay with EM for so long. Another thing about EM (perhaps
} more EM than other microscopy): there is some technical aspect here. You
} have to have deal with sophisticated equipment; sometime repair it,
} sometime hate it... and be in love with it... It's great challenge to
} have deal with all those beautiful/ugly machines. If you don't like to
} have deal with "iron", you'll probably get annoyed quite soon. To me, EM
} is a method to answer my scientific questions. I used to use other
} methods if I need it: HPLC, gel-electrophoresis, protein purification
} (good sample is most important thing in EM!) etc. Another aspect of
} modern EM: you have to be smart with computers (3D reconstruction software
} etc). People comes in EM from different backgrounds. Being a student I
} used EM in my histology project (stem cells actually, 25 years ago in
} Russia). I used EM to see the structure of the IgGs later. When I did
} IgG stuff, my mentor was a physics-guy, who come into molecular biology,
} so he (Victor Vasiliev) put a lot of emphasis on understanding how EM
} works, how image creates and how electrons interfere with your
} sample. For couple of years I got exclusive training in physics and
} mechanics. It was fun: in order to let me work in his Lab, Victor
} Vasiliev suggests I have to built freeze-drying apparatus by myself. I
} still don't know how, but I passed the test... Another my project was on
} ribosome's crystal structure, so I got a lot from crystallographers and
} CTF becomes very familiar to me... and sections were 10 nm thick. When
} you invest so much in something, it becomes the part of you. EM becomes
} part of me and there I am.
}
} From practical point of view, EM is not a best area for quick
} success. It takes time to get into it and results in most cases you must
} share with others (providing "images" for others). It's not so often
} happening that EMicroscopist is a first author (depends) or PI. So, from
} the "career" point of view, EM is not so promising (at least to
} me). Money - not good. BUT: great area to satisfy your curiosity and
} challenge him/herself with difficult samples, machines etc. Material
} science area with all that "nanothechnology" stuff is very promising and
} will grow fast in the near future (my personal prognosis). Sergey
}
} At 09:25 PM 7/18/2004, you wrote:
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 00:29:14 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

} Date: Mon, 19 Jul 2004 16:33:09 -0700
} To: Microscopy ListServer
} From: Sergey Ryazantsev {sryazant-at-ucla.edu}
} Subject: [Microscopy] Re: Re: Re: AskAMicroscopist: how one becomes a
} microscopist
}
} I really love my job. I think, EM (not necessary only EM) is good for
} people with natural curiosity: to see things smaller, smaller and
} smaller... sharper, sharper and sharper.... Curiosity, perhaps, is the
} reason to me to stay with EM for so long. Another thing about EM (perhaps
} more EM than other microscopy): there is some technical aspect here. You
} have to have deal with sophisticated equipment; sometime repair it,
} sometime hate it... and be in love with it... It's great challenge to
} have deal with all those beautiful/ugly machines. If you don't like to
} have deal with "iron", you'll probably get annoyed quite soon. To me, EM
} is a method to answer my scientific questions. I used to use other
} methods if I need it: HPLC, gel-electrophoresis, protein purification
} (good sample is most important thing in EM!) etc. Another aspect of
} modern EM: you have to be smart with computers (3D reconstruction software
} etc). People comes in EM from different backgrounds. Being a student I
} used EM in my histology project (stem cells actually, 25 years ago in
} Russia). I used EM to see the structure of the IgGs later. When I did
} IgG stuff, my mentor was a physics-guy, who come into molecular biology,
} so he (Victor Vasiliev) put a lot of emphasis on understanding how EM
} works, how image creates and how electrons interfere with your
} sample. For couple of years I got exclusive training in physics and
} mechanics. It was fun: in order to let me work in his Lab, Victor
} Vasiliev suggests I have to built freeze-drying apparatus by myself. I
} still don't know how, but I passed the test... Another my project was on
} ribosome's crystal structure, so I got a lot from crystallographers and
} CTF becomes very familiar to me... and sections were 10 nm thick. When
} you invest so much in something, it becomes the part of you. EM becomes
} part of me and there I am.
}
} From practical point of view, EM is not a best area for quick
} success. It takes time to get into it and results in most cases you must
} share with others (providing "images" for others). It's not so often
} happening that EMicroscopist is a first author (depends) or PI. So, from
} the "career" point of view, EM is not so promising (at least to
} me). Money - not good. BUT: great area to satisfy your curiosity and
} challenge him/herself with difficult samples, machines etc. Material
} science area with all that "nanothechnology" stuff is very promising and
} will grow fast in the near future (my personal prognosis). Sergey
}
} At 09:25 PM 7/18/2004, you wrote:
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 00:29:14 2004

Contents Retrieved from Microscopy Listserver Archives
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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

} Date: Mon, 19 Jul 2004 18:27:24 -0700
} To: Microscopy ListServer
} From: Sergey Ryazantsev {sryazant-at-ucla.edu}
} Subject: [Microscopy] Re: LKB anti vibration pads
}
} Hello Karen
} I don't think those old pads would work: rubber tends deteriorate with
} age. You could made very effective anti-vibration pad by yourself. It's
} easy: find in some story (like OSH or Home Depot in USA) the sheet of
} rubber approximately 1-1.5 cm thick. It should be solid relatively hard
} rubber, not porous one. Cut the sheet on pieces of the size you need and
} stack them to create necessary height. If you will put a thin aluminum
} sheet (1 mm) between each rubber layer (same size as rubber), you'll
} create superior anti-vibrating pad! Good luck, Sergey.
}
} At 08:43 AM 7/19/2004, you wrote:
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 09:11:26 2004

Contents Retrieved from Microscopy Listserver Archives
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chen jie

from the infectious disease side, bill tivol has really summed it up
fairly well. the treatments for 'fixing' tissue are quite good for
inactivating all known infectious agents - except for the prions. the
literature shows they require fairly harsh treatment. there are
recorded cases of the scrapie form of the prion protien maintaining its
catalytic capability even after treatment with formaldehyde and
alcohol. i have not seen any information regards the ability to survive
OsO4, however. the accepted treatment for the infectious prion forms is
10%NaOH.

as far as your original question, however, is OsO4 still dangerous after
all the treatments you have applied in washing, dehydrating and
embedding. i have seen no report of hazard after these steps. however,
you really have to contact your local Biological/Chemical Safety people
for disposal of the waste fix and washes. you really cannot dump them
down the drain. the Biological/Chemical Safety people will ensure that
proper disposal is done.

in short, unless you are working with prions, wear the right safety
clothing, follow the recipes, and dispose of wastes properly and you
will be subject to little risk.

caveat, nothing is totally risk free.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Work Phone: 204-789-3313
Pager: 204-931-954
Home Phone: 204-489-6924
Cell: 204-781-1502
Fax: 204-789-3926/204-489-6924

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 13:14:35 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi everyone,
I have a poor cooling water flow in my Philips TEM. I cleaned strainers,
filter lines, but alas, I still have poor flow.

On a previous position the TEM crew use to clean the pipes with some sort
of phosphoric acid cleaner. Any information would be welcome as well as
non-acid suggestions. I can use the scope until i get some flow through
it. It's a Phillip's 400 and its a bit sluggish right now.....

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 13:58:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Frank,
I am going through a semiannual-PM on my CM300 right now. My FEI service engineer has put about 0.5L of CLR (Calcium-Lime Remover - commercial product used in bathroom cleaning) into my Haskris chiller last night and replaced the water this morning. There was a lot of crud and algae that was flushed out of the scope (5 years in service, 1st procedure). He flushed the system with 25 gallons of tap water and restarted the instrument. The CM was operational through the night while the solution worked, however for water flushing we needed to put it in stand-by mode.

Please note, I observed the procedure and am shearing these observations. However, I do not take any responsibility for success of it on your microscope or its safety on the 400. It would be best if you contact FEI and get in touch with their service support. Even though you are not under service contract they tend to be very receptive to customers.

Jerzy
******************************************************
Jerzy Gazda, Ph.D. CeriumLaboratories L.L.C. - AMD Inc.
Supervising Engineer 5204 E. Ben White Blvd. - MS 512
Austin, TX 78741
TEL: 1-800-538-8450, Ext. 51453
jerzy.gazda-at-ceriumlabs.com
******************************************************

-----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
Sent: Tuesday, July 20, 2004 1:21 PM
To: microscopy-at-msa.microscopy.com

Hi everyone,
I have a poor cooling water flow in my Philips TEM. I cleaned strainers,
filter lines, but alas, I still have poor flow.

On a previous position the TEM crew use to clean the pipes with some sort
of phosphoric acid cleaner. Any information would be welcome as well as
non-acid suggestions. I can use the scope until i get some flow through
it. It's a Phillip's 400 and its a bit sluggish right now.....

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 14:07:08 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

When I was 9, Father, knowing my mind - to science was inclin-ed,
Brought home from a friend, a little scope that for me, was just
prim-ed.
It was really quite old, of dull, shiny brass with power way up at 3 X
2,
But I looked and viewed oft I could, not wishing to have else to do.

When off to college I was sent, to prep for higher things
The microscopes I went to find, and there I lost my wings.
For years I looked with no thought to relax at every wisp of glass
On which I observed, with naked eye, anything of color classed.

It was so easy long ago to become a microscopist's mate.
If you made the mistake of being awake when becoming a 'croscopist's
date.
Such interesting folk, these persons thus yoked, to tubes of concocted
close viewers,
By the eye and the brain, connected were they, so much so, they appeared
to be skewered.

You would think after years, like ten or at least twenty,
the eye would lose its perspective,
The glass would run out, color fade and dye out, and zeal turn
introspective.
But to be blessed with such easy and early respite, not for the
inveterate seer,
No rest is provided, with eye undivided. No, no ocular rest at all.

As the dog ever chases after the hare, and the fisherman goes after
Chinook,
Like fish in the lake chase after the bait, the microscopist just
squints - for a look.

And finally when done, after years of denyin',
There's no use anymore for the cryin'.
The person who looks, would merely be lyin'
If s/he tried to admit,
There's no slide in the kit,
Worth tryin' to view,
Before dyin'.

Fred Monson, '39 - no poet, and he know it!

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SSS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 14:57:25 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rebecca.burgin-at-onsemi.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 20, 2004 at 14:32:32
---------------------------------------------------------------------------

Email: rebecca.burgin-at-onsemi.com
Name: Rebecca Burgin

Organization: ON Semiconductor

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Colleagues,

I am looking for information on SEM magnification standards
that are available in the microscopy community. Your inputs
are greatly appreciated.

Rebecca

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 15:28:31 2004

Contents Retrieved from Microscopy Listserver Archives
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Frank,

We've experienced poor water flow due to a

Geoff Williams
Microscopy Facility Supervisor

Central Michigan University Biology Department Microscopy Facility
http://www.cst.cmich.edu/centers/microscopy/

} -----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
} Sent: Tuesday, July 20, 2004 2:21 PM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Advice needed
}
}
}
}
------------------------------------------------------------------------
--
} ----
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------
--
} -----
}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned
strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some
sort
} of phosphoric acid cleaner. Any information would be welcome as well
as
} non-acid suggestions. I can use the scope until i get some flow
through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 15:42:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Oops I Guess my email somehow got messed up. Forgive me...

Anyway, we've experienced restriction due to grenn copper (oxide) build
up in flow meters and some of the smaller diameter passages. I used a
dilute bit of nitric acid to clean it. But I was able to identify the
area of restriction. We use Distilled water in our chiller loop with
copper pipes. It may be worth a quick investigation if you can
determine (without too much of a mess) where the restriction is (ie in
the lenses, or the Diff pump cooling coils) and just acid clean the
trouble spot. I would caution against flushing nitric acid through the
whole system esp if there is any copper piping. I was able to isolate
the areas and determine that they were okay in nitric acid (or the acid
of choice).

Good luck

Geoff Williams
Microscopy Facility Supervisor

Central Michigan University Biology Department Microscopy Facility
http://www.cst.cmich.edu/centers/microscopy/

} -----Original Message-----
} From: Frank.Karl-at-degussa.com [mailto:Frank.Karl-at-degussa.com]
} Sent: Tuesday, July 20, 2004 2:21 PM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Advice needed
}
}
}
}
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America
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} On-Line Help
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} -----
}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned
strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some
sort
} of phosphoric acid cleaner. Any information would be welcome as well
as
} non-acid suggestions. I can use the scope until i get some flow
through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 16:46:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (amissaian-at-cheme.caltech.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 20, 2004 at 16:37:03
---------------------------------------------------------------------------

Email: amissaian-at-cheme.caltech.edu
Name: Ani

Organization: Caltech

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for a digital camara to place on a cryo-ultramicrotome, for instructional purpuses. Also, a good scanner for TEM negatives. Any suggestions?
Thanks,

Ani

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 18:17:50 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

As an extension of the request below, how are digital images being dealt
with as they relate to magnification?

In the days of film and paper enlargements, you could easily (more or
less) calculate the magnification ratio.

With digital images, this seems harder. I can measure the magnification
at the sensor, but this has no correlation to how the image will be
viewed. Ignoring any "zooming", the image will look very different in
terms of size on two different monitors, or even the same monitor at
different resolutions (assuming a pixel per pixel display).

Has any "standard" method been accepted for communicating the
magnification of a digital image? I'm thinking of something along the
lines of 1000X at 600 DPI (American printers) or 0.001mm per pixel.

John W. Raffensperger, Jr.

Email: rebecca.burgin-at-onsemi.com
Name: Rebecca Burgin

Organization: ON Semiconductor

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Colleagues,

I am looking for information on SEM magnification standards
that are available in the microscopy community. Your inputs
are greatly appreciated.

Rebecca

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 19:04:49 2004

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A simple procedure I've used for a long time - a small pump and a couple of
gallons of plain old household vinegar. The vinegar is a mild enough acid
that you really don't have to worry about it, yet strong enough to clear
things out quite well. A peristaltic pump is nice, but anything that can
push the vinegar through can work, even one of those small submersible
fountain pumps.

Haven't tried it myself, but if you have a chiller I can't see any reason
not to clean it all at once. Drain a couple of gallons out, top it off
with vinegar, and let it run for awhile.

Using undiluted vinegar on just the EM, I'll usually run a gallon through
the system for 20 minutes or until it gets pretty grundgy. Then switch to
a fresh gallon and let that run for maybe an hour. If you're using a
chiller, you'll want to run a couple of changes of fresh water through the
system to get rid of the vinegar.

This is a good preventative thing to do, if you can remember, every few
years. Quicker and easier if you catch it before it becomes a problem.

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174

phone (630) 513-7093 fax (630) 513-7092 http://www.sem.com

On Tuesday, July 20, 2004 1:21 PM, Frank.Karl-at-degussa.com
[SMTP:Frank.Karl-at-degussa.com] wrote:
}
}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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-------
}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some sort
} of phosphoric acid cleaner. Any information would be welcome as well as
} non-acid suggestions. I can use the scope until i get some flow through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 20:45:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Karl,
On my old EM 300 I found that disconnecting the water lines
and blowing them out with compressed air followed by a thorough
flushing with water into a bucket before reconnecting was the easiest
and most reliable way to restore the flow to normal. Good Luck.

On 20 Jul 2004 at 14:20, Frank.Karl-at-degussa.com wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some sort
} of phosphoric acid cleaner. Any information would be welcome as well as
} non-acid suggestions. I can use the scope until i get some flow through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}
}
}

All the best,

Andy Buechele, Washington, D.C., U.S.A.

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 20:47:55 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

I showed your local serviceman from Philips how to install a brass DP
shutoff valve from Nupro and how to make some end caps to quickly isolate
water blockages and check flow rates. Give a service call to FEI and ask
Ron or Russ to call you. They are both really nice people.

The isolation valve fix I used on my CM scope was put in as a service note
by Ron over ten years ago. It's real cheap to do. It was less than $10,
if you installed it yourself. Ask for the service note on this subject but
applied to a CM12 and authored by Ron. The parts needed were a brass Nupro
valve, two hose clamps, a piece of rubber 1/16 inch thick, a borrowed cork
borer, and four Swegelok end caps.

It's nice to see in other posts that the green copper carbonate message is
finally getting through and killing off all the algae myths.

Put a whole house water filter in the chiller inlet line to save on
plugging that hard to reach strainer. It's worth the cost and traps
floating / circulating copper carbonate precipitate, aka 'pseudo-algae'.

They probably used phosphoric acid to avoid pit corrosion by chloride ions
on the SS fittings on the scope when using HCl. You can test for residues
of ClŻ in water with silver nitrate. Calcium phosphates can have limited
solubility.
We used HCl and the dirty penny trick. We then flushed with a lot of water
to remove most chlorides. A final rinse with distilled water until
chloride free and the scope was then placed back on the chiller with
distilled water in it.

Install that DP valve.

Paul Beauregard
Senior Research Associate

}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some sort
} of phosphoric acid cleaner. Any information would be welcome as well as
} non-acid suggestions. I can use the scope until i get some flow through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 21:01:50 2004

Contents Retrieved from Microscopy Listserver Archives
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Rebecca -

VLSI Standards carries NIST Traceable Nanolattice Standards (certified to
100 nm pitch) which are ideal for semiconductor application SEM
magnification calibration and monitoring. In fact, I believe On Semi /
Motorola may own some of these standards. For more information on these or
to request a quote, please see:

http://www.vlsistandards.com/products/so_nanolattice.asp?cid=3&sid=78

Thanks!

Marc Helvey
VLSI Standards, Inc.
3087 North First Street
San Jose, CA 95134-2006
Phone: (408) 428-1800, ext. 108
FAX: (408) 428-9555
E-mail: marc.helvey-at-vlsistd.com
Internet: http://www.vlsistandards.com

-----Original Message-----
} From: rebecca.burgin-at-onsemi.com [mailto:rebecca.burgin-at-onsemi.com]
Sent: Tuesday, July 20, 2004 1:04 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rebecca.burgin-at-onsemi.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, July 20, 2004 at 14:32:32
---------------------------------------------------------------------------

Email: rebecca.burgin-at-onsemi.com
Name: Rebecca Burgin

Organization: ON Semiconductor

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Colleagues,

I am looking for information on SEM magnification standards
that are available in the microscopy community. Your inputs
are greatly appreciated.

Rebecca

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 20 23:03:25 2004

Contents Retrieved from Microscopy Listserver Archives
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In case there's something in here that might be applicable to other instruments
(thinking, selfishly, of JEOL 840), can you please briefly explain this mod and its
purpose?

thanks

rtch

Date sent: Tue, 20 Jul 2004 21:53:40 -0400
To: Frank.Karl-at-degussa.com, microscopy-at-msa.microscopy.com
} From: Beauregard {beaurega-at-westol.com}

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (juan-at-nanostellar.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, July 20, 2004 at 22:50:49
---------------------------------------------------------------------------

Email: juan-at-nanostellar.com
Name: Juan

Title-Subject: [Microscopy] [Filtered] How to know the 3D shape of nano-particles?

Question: Is there a normal procedure/software that is able to get 3D shapes of nano-particles based on one 2D TEM image?

Or we have to take several TEM images at different tilt conditions, then make the judgement of 3D shapes based on all the 2D images.

Any suggestion or idea will be highly appreciated.

Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 04:13:32 2004

Contents Retrieved from Microscopy Listserver Archives
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John,
it has always been impossible to know the size of an image in an
article when you submit a picture for publication, which is essentially the
same problem as you describe. That is why all micrographs should have a
fiducial (micron) marker - but the scale you want should be in microns (or
nm, or whatever) per pixel. It is a simple matter to set up a library of
micron markers which you can cut and paste onto an image - so much easier
than cutting letraset lines to length with a scalpel..

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

-----Original Message-----
} From: Chiphead [mailto:chiphead-at-sbcglobal.net]
Sent: 21 July 2004 00:24
To: microscopy-at-microscopy.com

As an extension of the request below, how are digital images being dealt
with as they relate to magnification?

In the days of film and paper enlargements, you could easily (more or
less) calculate the magnification ratio.

With digital images, this seems harder. I can measure the magnification
at the sensor, but this has no correlation to how the image will be
viewed. Ignoring any "zooming", the image will look very different in
terms of size on two different monitors, or even the same monitor at
different resolutions (assuming a pixel per pixel display).

Has any "standard" method been accepted for communicating the
magnification of a digital image? I'm thinking of something along the
lines of 1000X at 600 DPI (American printers) or 0.001mm per pixel.

John W. Raffensperger, Jr.

Email: rebecca.burgin-at-onsemi.com
Name: Rebecca Burgin

Organization: ON Semiconductor

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Colleagues,

I am looking for information on SEM magnification standards
that are available in the microscopy community. Your inputs
are greatly appreciated.

Rebecca

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From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 07:20:52 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (yksze1970-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, July 21, 2004 at 04:13:54
---------------------------------------------------------------------------

Email: yksze1970-at-yahoo.com
Name: Yuk

Title-Subject: [Microscopy] [Filtered] MListserver: Advice on water cooling

Question: Dear Colleagues,

I found some SEM systems require cooling water to cool pump system, electron-optical lenes and electronic circuit boards in parallel branches mode or in series mode. I understand that there are advantages of using water cooling for the electronic boards : temperature stable and free from fan vibration.

Is water cooling system in parallel branches mode better than in series mode?

My laboratory is located at sub-tropical region (hot and high humidity) and laboratory temperature is maintained by air-conditioner. I would appreciate hearing from anyone who has used SEM with water-cooled electronic circuit boards particularly on the precaution of water condensation on circuit boards.

Please contact me directly at: yksze1970-at-yahoo.com

Thanks

Yuk

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 07:33:22 2004

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Frank,

The 400 vintage EMs used a peculiar device to regulate the water flow
through the
lenses, power supplies, and vacuum system. It was a small rubber
"button-like"
device (inside something that looks like a coupling or small filter
housing),
that limited the direction and quantity of flow to one liter per minute.
These things
were the source of several problems I've encountered over the years. They
tend to
harden and/or swell and should probably be checked, replaced, or even
removed
before resorting to any further acid treatment, back-flushing, or blow-thru
attempts. Your
particular instrument may still have these, or they may have been removed,
or replaced
with some alternative means of flow regulation.

I'd like to echo and emphasize the previous remarks regarding contacting
FEI's service reps,
they may end up saving you lots of time and money by bringing their wealth
of talent and
years of experience.

Enjoy !

Lee Hanna
Dupont Company
Wilmington, De

302-695-4887

This communication is for use by the intended recipient and contains
information that may be privileged, confidential or copyrighted under
applicable law. If you are not the intended recipient, you are hereby
formally notified that any use, copying or distribution of this e-mail,
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by return e-mail and delete this e-mail from your system. Unless
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this e-mail does not constitute a contract offer, a contract amendment,
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Francais Deutsch Italiano Espanol Portugues Japanese Chinese Korean

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From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 08:11:37 2004

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Listers,

There is a late addition to the M&M 2004 sessions that will not be
listed in your program. Please add this to your program information.
Information is as follows:

Core Facility Management Session

Wednesday, Aug. 4
8:30am to Noon
Room 104

Funding Opportunities for Acquiring Major Instrumentation

The first portion of the session will be devoted to brief presentations
followed by an extensive question and answer period.

Speakers will include:
Marjorie Tingle: Director, NIH Shared Instrumentation Grant Program

Angela Klaus: NSF Program Director, Division of Biological Infrastructure

Charles Bouldin: NSF Program Director, Division of Materials Research

Remainder of the session will consist of a meeting of Facility Managers to
discuss:
1. Topics of interest for future sessions
2. Request for the formation of a Focused Interest Group on Facility
Operations by the MSA Council.

Hope to see you all there,

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 11:32:05 2004

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Frank,

I think that phosphoric acid may not be as effective on a lime deposit as one would
wish, although it is probably less likely to cause corrosion than some other
acids. Calcium phosphate is low in solubility and the initial amount formed on a
heavy lime buildup may serve to inhibit attack on the material underneath.

Another alternative that is effective on lime and relatively benign toward metals
is sulfamic acid. This material is sold in hardware stores for uses such as
cleaning lime scale from food service items like coffee makers and for removing
lime scale in water wells. It is a granular solid (therefore no fumes), soluble in
water up about 10%. I have no experience with using this in chiller lines but it
has worked in a very controlled way in other cleaning roles and and has a lot of
advantages over liquid or volatile alternatives.

John Twilley

Frank.Karl-at-degussa.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some sort
} of phosphoric acid cleaner. Any information would be welcome as well as
} non-acid suggestions. I can use the scope until i get some flow through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 12:36:23 2004

Contents Retrieved from Microscopy Listserver Archives
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I need to embed cells plated on Thermanox coverslips (purchased from EM
Sciences) for TEM. Any advice on the best embedding medium to use will be
greatly appreciated.

Thanks,

Cora Bucana

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 14:54:47 2004

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______________________________________________________________________
This email has been scanned by the MessageLabs Email Security System.
For more information please visit http://www.messagelabs.com/email
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From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 15:08:14 2004

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}
} I found some SEM systems require cooling water to cool pump system,
} electron-optical lenes and electronic circuit boards in parallel
} branches mode or in series mode. I understand that there are
} advantages of using water cooling for the electronic boards :
} temperature stable and free from fan vibration.
}
} Is water cooling system in parallel branches mode better than in
} series mode?

The advantage of parallel connection is that, just as in electrical circuits, different water
flows can be arranged for different components.
In my JEOL JXA-840, for example, the diffusion pumps are supposed to have 3 l/m (it
has two DPs, and they are connected in series), the electronics boards 1.5 l/m, but the
objective lens only 0.5 l/m.

A disadvantage with parallel connection is that, unless you have a flow meter or sensor
in each of the branches, a blockage in one branch may not be noticed until it is too late
to prevent damage from overheating.

}
} My laboratory is located at sub-tropical region (hot and high
} humidity) and laboratory temperature is maintained by air-conditioner.
} I would appreciate hearing from anyone who has used SEM with
} water-cooled electronic circuit boards particularly on the precaution
} of water condensation on circuit boards.
}

As far as working in a high humidity goes, it is very important to ensure that your cooling
water is not too cold, to avoid water condensation, which can be very damaging. Its
temperature must be above the dewpoint. The cooling water does not need to be colder
than the temperature of the laboratory air.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 16:58:21 2004

Contents Retrieved from Microscopy Listserver Archives
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I am looking for comment on overall functionallity of the Microtek
ArtixScan 1800f scanner. Reliability, resoultion, speed. Will use this
to scan EM neg. etc.

Thanks

Robert J. Kayton, Ph.D.
C.R.O.E.T. L606
Oregon Health & Science Univ.
kayton-at-ohsu.edu
503-494-2504-Lab
503-703-3938-Cell
www.ohsu.edu/croet/facilities/emicroscopy

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 16:59:41 2004

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http://www-hrem.msm.cam.ac.uk/~mw259/Work/Tomo.html

A search of Google with the string: "3d tem tomography nanostructure"
yielded the above link which is certainly relevant to your question.

The brief answer is that under the best conditions a 2D image can
divulge 3D structure IF the section(?) includes/projects all perspective
views of the object WHEN you know that all objects in the specimen HAVE
the same shape.

Hope this helps,

Fred Monson

Frederick C. Monson, PhD
Center for Advanced Scientific Imaging
Mail to Geology
West Chester University of Pennsylvania
Schmucker II Science Center, Room SSS024
South Church Street and Rosedale Avenue
West Chester, PA, 19383
Phone/FAX: 610-738-0437
eMail: fmonson-at-wcupa.edu
CASI Page and Scheduling
http://darwin.wcupa.edu/CASI/

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:juan-at-nanostellar.com]
Sent: Wednesday, July 21, 2004 12:55 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (juan-at-nanostellar.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
July 20, 2004 at 22:50:49
------------------------------------------------------------------------
---

Email: juan-at-nanostellar.com
Name: Juan

Title-Subject: [Microscopy] [Filtered] How to know the 3D shape of
nano-particles?

Question: Is there a normal procedure/software that is able to get 3D
shapes of nano-particles based on one 2D TEM image?

Or we have to take several TEM images at different tilt conditions, then
make the judgement of 3D shapes based on all the 2D images.

Any suggestion or idea will be highly appreciated.

Thanks.

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 17:01:19 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi everyone,
I received a request from a the staff members of our department for a
water soluble mounting medium. He is working with algae and wants to
know if such a product exists. I am only familiar with Permount,
Harleco Synthetic Resin and Canada Balsam used with tissue that has
been processed and sectioned.
Does anyone have experience with such a product? Can you skip the
tissue dehydration process (just fix and cover slip)? What do your
slides look like? How stable is the product and how long does it last?
etc...
Once again I thank all the list supporters in advance for your
knowledgeable responses. If you wish, you may contact me directly at
dufresne-at-ms.umanitoba.ca. Merci.

André Dufresne

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 17:10:40 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi:

We are having a new TEM installed in our lab. The PI in charge wants to
thank the staff who have helped with the project by having a 'scope
warming' event and pass out some kind of microscope souvenir, like a
keychain, miniature microscope, or something equally cheap, but thoughtful.

Probably fewer than 10 would be needed, anybody have ideas and/or where
such things could be found?

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 18:43:14 2004

Contents Retrieved from Microscopy Listserver Archives
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Yuk,
I would suggest setting the plumbing up as the manufacturer designed it. As
Ritchie mentioned, the chief problem with parallel circuits is that they
often don't have separate flowmeters on each circuit, so you have no idea
what flow you're getting in each section, but you can add the fowmeters.
Series circuits must be plumbed correctly, that is the order of the cooled
components must be correct or you can have problems. For example, if the
diffusion pump is put first in line, everything else is going to be warm.
In general, any water cooled baffle in the vacuum system should probably be
first, to be coldest and it will add very little heat. Next might be
critical components like a lens control, then power supplies and finally the
DP. One advantage of a series setup is that the water gets warmer as it
proceeds through the system and you have fewer places that might get
condensation.

As to the condensation problem, the very first thing is to make sure that
your water supply is not too COLD. 70-72F (22-23C) is often a good
temperature to start with. Much colder than that and I'll bet on
condensation if the humidity gets out of control.

You mentioned that the space is air conditioned. Can you check the
humidity? If you can keep it down to 75%, you probably won't have much
trouble. One way to do that is to make sure that the air conditioner is
JUST big enough to do the job, then the compressor will run most of the
time, the evaporator coil will stay very cold and a lot of water will be
removed from the air. If the AC doesn't have to work very hard (it's too
big) then the evaporator coil never gets cold enough to condense any water.
It cools the air easily, but never removes any water.

An example of the first case is my SEM space. In south-central Pennsylvania
we have a lot of humidity in the summer with temperatures often in the upper
80s (32-33C). The room is about 16'x32' (5x10m) with a SSE exposure and 2
windows. With an SEM running and 3 bodies in the room my 7000 BTU air
conditioner just barely holds its own, but the humidity can easily drop to
65%, 60% or lower. On the other side of the building I have a 16'x16'
(5x5m) storage room with 2 windows with a NNW exposure. Unless I actually
turn the heat on, the 6000 BTU AC works so little that I often cannot get
the humidity below 80%.

A second option is to use a dehumidifier. These add heat to the room while
removing water, so your AC will need to be able to handle the additional
load. Of course, if it can't handle the additional load, then you will
probably find that it is already working hard enough that your humidity is
low.

The main thing is to not have any condensation in the power supplies. If
you're dry enough for that, you're dry enough.

Good luck,

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:yksze1970-at-yahoo.com]
Sent: Wednesday, July 21, 2004 8:28 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (yksze1970-at-yahoo.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday,
July 21, 2004 at 04:13:54
---------------------------------------------------------------------------

Email: yksze1970-at-yahoo.com
Name: Yuk

Title-Subject: [Microscopy] [Filtered] MListserver: Advice on water cooling

Question: Dear Colleagues,

I found some SEM systems require cooling water to cool pump system,
electron-optical lenes and electronic circuit boards in parallel branches
mode or in series mode. I understand that there are advantages of using
water cooling for the electronic boards : temperature stable and free from
fan vibration.

Is water cooling system in parallel branches mode better than in series
mode?

My laboratory is located at sub-tropical region (hot and high humidity) and
laboratory temperature is maintained by air-conditioner. I would appreciate
hearing from anyone who has used SEM with water-cooled electronic circuit
boards particularly on the precaution of water condensation on circuit
boards.

Please contact me directly at: yksze1970-at-yahoo.com

Thanks

Yuk

---------------------------------------------------------------------------

________________________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Wed Jul 21 22:22:01 2004

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Good morning colleagues
I just figured out that I started last box of tungsten filaments (type K,
JEOL) from my 10+ years old "savings". I need to consider: should I buy
native JEOL's filaments or other vendors are good as well (what is your own
experience?). Another consideration I need to do: should I try re-built
filaments, what company? Any input would be greatly appreciated. Thanks in
advance, Sergey

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 06:29:01 2004

Contents Retrieved from Microscopy Listserver Archives
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There are many glycerin or gelatin based media which are easy and fast to
use, stable (especially if you take the time to "ring" the edges to seal
the media) and can be redissolved in a little water.

Try googling this subject or try the RMS.

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 07:09:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

If you have an FEI microscope with a compustage that is available for
outside users, and you are near Chicago, please contact me (off-line).
Thanks.

-----------------------------------------------
Laurence Marks
Department of Materials Science and Engineering
Northwestern University
Evanston, IL 60201, USA
Tel: (847) 491-3996 Fax: (847) 491-7820
mailto:ldm2-at-risc4.numis.nwu.edu
http://www.numis.nwu.edu
-----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 08:52:56 2004

Contents Retrieved from Microscopy Listserver Archives
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sergey

as we stumble and bungle towards a core facility we deal with a mixture
of filament sources. i have used rebuilts on a Philips 201 for 20
years. in Canada, the distributor is Soquelec. however, i believe they
are actually from SPI. i get specialty filaments. simple pointed
filaments are half the price as FEI bent tungsten. they provide
significantly better electron emission (probably because they are the
pointed ones), brighter illumination at lower filament current (again,
better emission, pointed filaments) and they last 5-8x longer. my last
one ran approximately 300 hours. for the CM 10 and other 201 in this
awkward mixture the original departments insist on using FEI supplied
filaments. shorter life in the gun, lower emission, less illumination.

do not read this as a knock against FEI. their service people are quite
good, and they make good microscopes. beyond a doubt, part of what i
see is because i get specialty filaments, not just bent tungsten. but
you cannot beat the price. and no, i have no interest in any of the
three companies.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Work Phone: 204-789-3313
Pager: 204-931-954
Home Phone: 204-489-6924
Cell: 204-781-1502
Fax: 204-789-3926/204-489-6924

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 08:55:30 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Biomeda Corp. (Foster City, CA)is just one company that sells a number of
aqueous mounting media (i.e. Crystal/Mount-aqueous/dry mounting media for enzyme
immunohistochemistry and Gel/Mount- aquesous mounting media with anti-fading
agents) We have a need for them especially with fluourescent work.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Andre Dufresne [mailto:dufresne-at-Ms.UManitoba.CA]
Sent: Wednesday, July 21, 2004 6:03 PM
To: Microscopy List

Hi everyone,
I received a request from a the staff members of our department for a
water soluble mounting medium. He is working with algae and wants to
know if such a product exists. I am only familiar with Permount,
Harleco Synthetic Resin and Canada Balsam used with tissue that has
been processed and sectioned.
Does anyone have experience with such a product? Can you skip the
tissue dehydration process (just fix and cover slip)? What do your
slides look like? How stable is the product and how long does it last?
etc...
Once again I thank all the list supporters in advance for your
knowledgeable responses. If you wish, you may contact me directly at
dufresne-at-ms.umanitoba.ca. Merci.

André Dufresne

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 09:54:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Currently we have a posting for an experienced EM Tech.

The position is in a clinical pathology laboratory and requires
routine TEM. Salary and responsibility to commensurate with experience.
If you are interested or know of anyone who may be interested please
feel free to contact me directly, or check out the posting at

jobs. jhu.edu

Thanks

Lois Anderson
Johns Hopkins University
Dept. of Pathology
Laboratory Manager
EM/IF/Reference Histology
600 N. Wolfe Street/Pathology 709 A
Baltimore, MD 21287
(410) 955-2861/fax (410) 614-7110
landers-at-jhmi.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 10:51:55 2004

Contents Retrieved from Microscopy Listserver Archives
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Paul,

Just a minor correction. The rebuilt and specialty filaments you get
from Soquelec are actually manufactured by EBSciences. Soquelec is a
distributor for our products in Canada.

Michael R. Nesta
General Manager
Energy Beam Sciences, Inc.
800 992-9037
www.ebsciences.com

DISCLAIMER: Energy Beam Sciences manufactures and sells electron beam
sources and therefore has a financial interest in the accurate
representation of this information.

paul r hazelton wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 11:04:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Glacial acetic acid, or LOTS of vinegar is the tried and true
solution(sic) for lime deposits.

John Mardinly
Intel

-----Original Message-----
} From: John Twilley [mailto:jtwilley-at-sprynet.com]
Sent: Wednesday, July 21, 2004 10:07 AM
To: Frank.Karl-at-Degussa.com
Cc: microscopy-at-msa.microscopy.com

Frank,

I think that phosphoric acid may not be as effective on a lime deposit
as one would
wish, although it is probably less likely to cause corrosion than some
other
acids. Calcium phosphate is low in solubility and the initial amount
formed on a
heavy lime buildup may serve to inhibit attack on the material
underneath.

Another alternative that is effective on lime and relatively benign
toward metals
is sulfamic acid. This material is sold in hardware stores for uses
such as
cleaning lime scale from food service items like coffee makers and for
removing
lime scale in water wells. It is a granular solid (therefore no fumes),
soluble in
water up about 10%. I have no experience with using this in chiller
lines but it
has worked in a very controlled way in other cleaning roles and and has
a lot of
advantages over liquid or volatile alternatives.

John Twilley

Frank.Karl-at-degussa.com wrote:

}
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------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
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} On-Line Help
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-------
}
} Hi everyone,
} I have a poor cooling water flow in my Philips TEM. I cleaned
strainers,
} filter lines, but alas, I still have poor flow.
}
} On a previous position the TEM crew use to clean the pipes with some
sort
} of phosphoric acid cleaner. Any information would be welcome as well
as
} non-acid suggestions. I can use the scope until i get some flow
through
} it. It's a Phillip's 400 and its a bit sluggish right now.....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
} 330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 11:06:19 2004

Contents Retrieved from Microscopy Listserver Archives
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On Jul 21, 2004, at 8:29 PM, Sergey Ryazantsev wrote:

} I just figured out that I started last box of tungsten filaments (type
} K, JEOL) from my 10+ years old "savings". I need to consider: should
} I buy native JEOL's filaments or other vendors are good as well (what
} is your own experience?). Another consideration I need to do: should
} I try re-built filaments, what company? Any input would be greatly
} appreciated. Thanks in advance, Sergey
}
Dear Sergey,
Back in Albany on the HVEM we got the best results with both new and
rebuilt filaments from Energy Beam Sciences and new filaments from
Agar. I have no affiliation with either of these companies except as a
satisfied customer. The rebuilt filaments worked as well as the new
ones as long as the bases were not damaged or heavily coated with
tungsten.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 11:30:08 2004

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Cora,

You can use almost any standard embedding medium, as far as I know. We
routinely use Epon-Araldite or Epon-Spurrs, but any resin should work.

Just in case you're not aware of it, you have a couple options for
dealing with plated cells on coverslips. With Thermonox coverslips you
can indeed embed them directly into the resin and cut thin sections.
This will give you a cross section of the cells on the surface of the
slip, appearing as a line of cells along the straight edge of the
plastic.

The other option is to fill an embedding capsule to the brim with resin
with the open end up, then lay the cover slip on top with the cells down
(after processing the coverslip through the pure resin stage, of
course). Polymerize as usual, but stop before the resin is 100%
hard---it can still be a little sticky, usually 12 hours or overnight
will do it. Then drop the capsule with attached coverslip into liquid
nitrogen until it quits fizzing, pick it up and snap off the coverslip.
Usually it will snap off fairly cleanly, leaving a layer of cells in the
wide end of the resin block. If not, dunk it again. (Occasionally, the
resin may crack, but I've only had this happen once and was able to get
good sections anyway.) Put the blocks back in the oven and finish
polymerizing, and make sure you save the coverslips as backups. Now all
you have to do is use a microscope to find a good area with cells on the
block, trim your block face, and start cutting thins.

You have to start cutting ultrathins immediately, no thicks!, since you
only have a monolayer of cells, but there should be enough material for
lots of grids. This method has the advantage of giving you top-down
overall views of the cells, instead of itty-bitty edge-on cross
sections.

Apologies if you already knew about this, but we find this technique
very useful.

Good luck,

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.biotech.missouri.edu/emc/

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 12:29:29 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

Can anyone suggest an embedding epoxy for 200kV TEM?
Thanks in advance.

Ling

=====
Ling Pan, Ph.D.
195 Materials Research Institute
The Pennsylvania State University
University Park, PA 16802
Tel: (814) 863-1096
Fax: (814) 863-8561

__________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 13:00:17 2004

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Hello all,

We are looking for CL capability (in a SEM) for probing electronic materials with a bandgap range of 350 to 200 nm. We need to measure a small number of samples and would prefer, if possible, a facility in the CT area.

Any suggestions would be much appreciated.

Cheers!
Ann

****************
Ann H. Lehman
Trinity College EM Facility
Hartford, CT 06106
v. 860-297-4289

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 13:00:56 2004

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Hi Andre:

There are a number of do-it-yourself formulas, check John Kiernan's
website, any good histotechniques book, or you can buy a commercial
product. Making your own has several advantages, cheaper, you can make
just the amount you need, and you know exactly what is in it so you can
repeat your successes and not repeat your failures.
Aqueous mounts usually won't give as "crisp" an image as a
dehydrated and cleared specimen, due to different indices of refraction
between glass and aqueous materials.

Geoff

Andre Dufresne wrote:

} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hi everyone,
} I received a request from a the staff members of our department for a
} water soluble mounting medium. He is working with algae and wants to
} know if such a product exists. I am only familiar with Permount,
} Harleco Synthetic Resin and Canada Balsam used with tissue that has
} been processed and sectioned.
} Does anyone have experience with such a product? Can you skip the
} tissue dehydration process (just fix and cover slip)? What do your
} slides look like? How stable is the product and how long does it
} last? etc...
} Once again I thank all the list supporters in advance for your
} knowledgeable responses. If you wish, you may contact me directly at
} dufresne-at-ms.umanitoba.ca. Merci.
}
} André Dufresne
}
--

**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 15:06:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all,

We are considering adding UPS units to our instruments. All of the systems
I'm familiar with contain a number of lead-acid gel cell batteries. Right
now, we are considering putting the whole instrument (rather than just the
computer) on a UPS.

If you power the entire instrument through the UPS, the power draw is
significant. Since the gel-cells generally operate a 12 volts, there will
be a high current draw if all the power goes through the 12v circuit i.e. a
double-conversion system. This suggests that a UPS could be a significant
magnetic field generator.

Has anyone experienced problems of this sort? Also since we will need to
budget for battery replacement, what kind of lifetime do the battery packs
have?

Thanks,
Henk Colijn

Hendrik O. Colijn colijn.1-at-osu.edu
Campus Electron Optics Facility Ohio State University
(614) 292-0674 http://www.ceof.ohio-state.edu
Time is that quality of nature which keeps events from happening all at
once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 19:08:31 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (subramss-at-email.uc.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, July 22, 2004 at 18:38:51
---------------------------------------------------------------------------

Email: subramss-at-email.uc.edu
Name: Srinivas Subramaniam

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] M&M 04 Conference accomodations help

Question: Dear Friends,

I am a graduate student at the University of Cincinnati currently pursuing a Ph.D. in Materials Science & Engineering. I will be presenting my research at the Savannah conference.

Travel expenses and registration fees have severely my available funds.I would like to request assistance in obtaining economical accomodation due to the limited finances at my disposal. Any suggestions which can help in procurring economical stay would be greatly appreciated. I am also open to sharing lodging expenses with interested persons.

I would be greatful for any help in this matter.

Sincerely,

Jimble

Srinivas Subramaniam
Chemical & Materials Engineering
University of Cincinnati
Cincinnati OH 45221-0012

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 22:01:35 2004

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Begin forwarded message:

} From: Alberto Diaspro {diaspro-at-fisica.unige.it}
} Date: 23 luglio 2004 5:04:32 CET
} To: Confocal List Microscopy {CONFOCAL-at-LISTSERV.BUFFALO.EDU} ,
} 'Microscopy-at-MSA.Microscopy.Com' community
} {Microscopy-at-MSA.Microscopy.Com}
} Subject: [Microscopy] Villa Gualino School on Single Molecule Biophysics, Turin,
} Italy Sept 6-12
}
} Dear friends,
} in September will be held a SIngle Molecule Biophysics School in Turin.
} See you there!
} All my best
} Alby
}
}
}
} SINGLE MOLECULE BIOPHYSICS
} Villa Gualino, Turin, September 6-12
}
}
}
} Directors of the School :
}
} Franco Conti CNR-Istituto di Biofisica Via dei Marini, 6 16149 Genova
} Tel. 010-6475577 Fax 010-6475500 E-mail conti-at-ge.ibf.cnr.it
}
} Alberto Diaspro Universita' di Genova Dipartimento di Fisica Via
} Dodecaneso 33 16146 Genova Tel. 010-3536426/480 E-mail
} diaspro-at-fisica.unige.it
}
}
}
} Lecturers:
}
} M. Bolognesi (Universitŕ di Genova)
}
} G. Chirico (Universita’ di Milano Bicocca)
}
} D. Dunlap (Istituto Scientifico San raffaele, Milano)
}
} L. Finzi (Universita' Statale di Milano)
}
} A. Gliozzi (Universitŕ di Genova)
}
} E. Gratton (University of Illinois, Urbana, USA)
}
} J. Langowski (German Cancer Research Center,Heidelberg, Germany)
}
} C. Miller (Brandeis University, Waltham,USA)
}
} O. Moran (Istituto di Biofisica CNR, Genova )
}
} F. Pavone (Universitŕ di Firenze)
}
} B. Samorě (Universitŕ di Bologna)
}
} S. M. Simon, (Rockefeller University, New York, USA)
}
} H. Vogel (Institute de Science Biomoleculaire, Lausanne, Switzerland)
} SISTEMI DI NON
}
}
}
} Scientific Advisory board: Guido Boffetta (Universita' di Torino),
} Franco Conti (CNR- Istituto di Biofisica), Alberto Diaspro
} (Universita' di Genova) Francesco Pegoraro (Universita' di Pisa),
} Mario Rasetti (Politecnico di Torino), Elena Tresso (Politecnico di
} Torino), Angelo Vulpiani (Universita' di Roma)
}
} Organization: Fondazione I.S.I., c/o Villa Gualino Viale Settimio
} Severo, 65 - 10133 Torino Tel. +39-011-6603090 Fax. +39-011-6600049
} E-mail:segreteria-at-isi36a.isi.it
}
} website: http://www.isi.it/42/events_detail.html
}
} Sponsored by Fondazione Cassa di Risparmio di Torino, del Politecnico
} di Torino e della Regione Piemonte.
}
}
}
} -----------------------------------------------------------------------
} ----------------------------
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} Via Dodecaneso 33, 16146 Genova, Italy
} facsimile +39-010314218 - voice +39-0103536426/480/309
} URL: http://www.lambs.it
} http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
} -----------------------------------------------------------------------
} ---------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 22 22:15:08 2004

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Thank you all for sharing your expertise. I appreciate your comments and
pointers.

Cora Bucana

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 06:11:26 2004

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I had an overwhelming response for the free EMs. I have found new homes
for them. I apologize but I could not respond to every phone call and
email.

Thanks,

Steve Widing
Technical Coordinator
Biology Department
Temple University

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 07:45:48 2004

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Hello Jonathan,
Personnaly, I like the calendar published by the american registry of pathology. I do not remember who had sent an e-mail to this list concerning this calendar, but I have ordered it (it is free) and love it. (website : www.afip.org )
Could be an idea ...
Daničle

--------------------------------------------
Daničle Spehner, INSERM EPI 99-08 - EFS-Alsace
10 rue Spielmann - 67065 STRASBOURG
tel : 03 88 21 25 25 - fax : 03 88 21 25 44
e-mail : daniele.spehner-at-efs-alsace.fr
------------------------------------

-----Message d'origine-----
De : Jon Krupp [mailto:jmkrupp-at-cats.ucsc.edu]
Envoyé : jeudi 22 juillet 2004 00:10
Ŕ : microscopy-at-microscopy.com
Objet : Microscope souvenirs ?

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Hi:

We are having a new TEM installed in our lab. The PI in charge wants to
thank the staff who have helped with the project by having a 'scope
warming' event and pass out some kind of microscope souvenir, like a
keychain, miniature microscope, or something equally cheap, but thoughtful.

Probably fewer than 10 would be needed, anybody have ideas and/or where
such things could be found?

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 08:08:51 2004

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-----Original Message-----
} From: Hendrik O. Colijn [mailto:colijn.1-at-osu.edu]
Sent: Thursday, July 22, 2004 4:16 PM
To: Microscopy-at-MSA.Microscopy.Com

Hendrik,

This may not answer you whole need, but the turbo pump power on our
Hitachi S-900 has a battery back up that uses lead-acid cells. The
pump uses a magnetically levitated bearing, and the batteries are
only to maintain this for a brief power outage, or to spin down the
pump in case of a longer outage.
For us, the batteries are recommended to be replaced every year, but
actually last 18 months, maybe 2 years, if we're feeling adventurous.

Phil

} Hi all,
}
} We are considering adding UPS units to our instruments. All of the
} systems I'm familiar with contain a number of lead-acid gel cell
} batteries. Right now, we are considering putting the whole
} instrument (rather than just the computer) on a UPS.
}
} If you power the entire instrument through the UPS, the power draw
} is significant. Since the gel-cells generally operate a 12 volts,
} there will be a high current draw if all the power goes through the
} 12v circuit i.e. a double-conversion system. This suggests that a
} UPS could be a significant magnetic field generator.
}
} Has anyone experienced problems of this sort? Also since we will
} need to budget for battery replacement, what kind of lifetime do the
} battery packs have?
}
} Thanks,
} Henk Colijn
}
}
} Hendrik O. Colijn colijn.1-at-osu.edu
} Campus Electron Optics Facility Ohio State University
} (614) 292-0674 http://www.ceof.ohio-state.edu
} Time is that quality of nature which keeps events from happening all
} at once. Lately it doesn't seem to be working.

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 09:27:45 2004

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Dear All,
I suspect I am not alone in spending much of my time measuring
dimensions from micrographs. As we will soon have a new TEM with digital
image capture, I am starting to wonder whether there is some software which
will automate this to some extent. I am thinking of something which will be
able to recognise bands of (fairly) constant contrast, determine its
orientation (Hough transform?), determine how many different bands there
are, extract a line profile by averaging and measure the width of each based
on some criterion (e.g. mid-way between the two contrast levels). The same
of course applies to SEM, optical or indeed any other kind of image where
dimensions are measured. I know this is asking a lot from image processing,
but it seems quite feasible. Or I can just carry on using a ruler..

Any ideas?

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
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From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 10:23:42 2004

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My system currently runs with two Toshiba 1400xl Plus
6KVA dual conversion UPS units. These run from 120/208/240
VAC and output same voltages during run and backup.

One unit runs the SEM and its pumps while the other
unit runs the chiller and compressor. The PCs and all
other 120VAC units are run from the SEM's UPS. Output
voltage is regulated to +- 2% and can handle over voltage
and brownouts.

These UPS units use 18 12VDC 7.2Amp sealed lead acid
batteries all connected in series. There is a large
transformer in the UPS which is used to invert the
rectified line AC or directly from the batteries.
I find no stray magnetic interference from these systems
either when in AC operation or backup operation.

Battery life is between three to four years. From
Digikey, the batteries are about $16 each. With care,
they can be user replaced. Outside service typically
charges $30 per battery plus $125 per hour labor.

That said, I would not recommend the Toshiba units as
they are now difficult if not impossible to repair.
Battery replacement is OK but if an electronic problem
occurs, I have not located anyone who will service the
units. Perhaps check into Liebert units. They seem
to be more predominant in the states.

gary g.

At 05:11 AM 7/23/2004, you wrote:

} -----Original Message-----
} } From: Hendrik O. Colijn [mailto:colijn.1-at-osu.edu]
} Sent: Thursday, July 22, 2004 4:16 PM
} To: Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] UPS systems and magnetic fields
}
}
}
} Hi all,
}
} We are considering adding UPS units to our instruments. All of the systems
} I'm familiar with contain a number of lead-acid gel cell batteries. Right
} now, we are considering putting the whole instrument (rather than just the
} computer) on a UPS.
}
} If you power the entire instrument through the UPS, the power draw is
} significant. Since the gel-cells generally operate a 12 volts, there will
} be a high current draw if all the power goes through the 12v circuit i.e. a
} double-conversion system. This suggests that a UPS could be a significant
} magnetic field generator.
}
} Has anyone experienced problems of this sort? Also since we will need to
} budget for battery replacement, what kind of lifetime do the battery packs
} have?
}
} Thanks,
} Henk Colijn
}
}
} Hendrik O. Colijn colijn.1-at-osu.edu
} Campus Electron Optics Facility Ohio State University
} (614) 292-0674 http://www.ceof.ohio-state.edu
} Time is that quality of nature which keeps events from happening all at
} once. Lately it doesn't seem to be working.
} ---------------------------------------
}
} Hello Henk,
}
} I have (only) my computers on 1kVA UPS systems, so cannot speak from direct
} experience about one large enough to power the entire EM system. Some
} generalizations...
}
} While most small UPS systems do run on 12 volts, I think you will find that
} one of sufficient capacity to run your entire system will use a higher
} voltage - 24, 48, 120, or more. ...An obvious attempt to reduce current for
} a given power.
}
} Never the less, the systems employ "switching" technology which generates
} significant high frequency EMI. If properly designed, using steel cases
} (...possibly Mu metal shielding) and appropriate I/O filtering, they can be
} rather "quiet". Without proper shielding and filtering, they can be pretty
} good broadband transmitters.
}
} I would consult with the application department of the UPS suppliers you are
} considering and specifically ask about EMI radiation specifications for the
} units under consideration.
}
} Good Luck,
} Woody
}

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 11:02:41 2004

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Jonathan,
This is a beautiful calender I agree however a
donation was requested to cover the costs if they
are still available. It was quite some time ago
that I had received mine.
Pat Connelly
U of P , Biology
psconnel-at-sas.upenn.edu
++++++++++++++++++
} We are having a new TEM installed in our lab. The PI in charge wants to
} thank the staff who have helped with the project by having a 'scope
} warming' event and pass out some kind of microscope souvenir, like a
} keychain, miniature microscope, or something equally cheap, but thoughtful.
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu
} ==================
} Hello Jonathan,
} Personnaly, I like the calendar published by the
} american registry of pathology. I do not
} remember who had sent an e-mail to this list
} concerning this calendar, but I have ordered it
} (it is free) and love it. (website :
} www.afip.org )
} Could be an idea ...
}
} Daničle Spehner, INSERM EPI 99-08 - EFS-Alsace
} 10 rue Spielmann - 67065 STRASBOURG
} tel : 03 88 21 25 25 - fax : 03 88 21 25 44
} e-mail : daniele.spehner-at-efs-alsace.fr

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 12:05:59 2004

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Hello Everyone,
Thanks for your advice with our new(ish) XL30 ESEM W TMP from FEI. The
microscope was working for a week with the new power supply, but voltage
problems in our building I think killed the power supply and power
distribution board in the ESEM computer. I'm faced with either replacing
the power supply and distribution board or rebuilding the whole system.

I was wondering if anyone knew what systems I could go up to that the XL30
software would support? Anyone ever upgrade their computers? I was
thinking of going with Pentium 3 or 4 system and trying to reinstall the
software.

Again, any advice will be appreciated. We are setting up a Sola voltage
system to correct voltage problems.
Thanks,
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 13:03:35 2004

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Henk;
We have our JEOL 2010F on a UPS to protect the FEG tip, and the
UPS needs to be located a LONG distance from the TEM due to magnetic
fields. Something like 30 feet.

John Mardinly
Intel

-----Original Message-----
} From: Hendrik O. Colijn [mailto:colijn.1-at-osu.edu]
Sent: Thursday, July 22, 2004 1:16 PM
To: Microscopy-at-MSA.Microscopy.Com

Hi all,

We are considering adding UPS units to our instruments. All of the
systems
I'm familiar with contain a number of lead-acid gel cell batteries.
Right
now, we are considering putting the whole instrument (rather than just
the
computer) on a UPS.

If you power the entire instrument through the UPS, the power draw is
significant. Since the gel-cells generally operate a 12 volts, there
will
be a high current draw if all the power goes through the 12v circuit
i.e. a
double-conversion system. This suggests that a UPS could be a
significant
magnetic field generator.

Has anyone experienced problems of this sort? Also since we will need
to
budget for battery replacement, what kind of lifetime do the battery
packs
have?

Thanks,
Henk Colijn

Hendrik O. Colijn colijn.1-at-osu.edu
Campus Electron Optics Facility Ohio State University
(614) 292-0674 http://www.ceof.ohio-state.edu
Time is that quality of nature which keeps events from happening all at
once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 14:25:32 2004

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} Dear All,
}

We normally Clean the Wehnelt of our TEM with Trichlorofluoroethane with
alumina powder. The process takes some time. Does anybody know if there
is any other way to do it faster?

Thank you

Jafar

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 16:01:35 2004

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On Jul 23, 2004, at 3:32 PM, Jafar Al-Sharab wrote:

} We normally Clean the Wehnelt of our TEM with Trichlorofluoroethane
} with alumina powder. The process takes some time. Does anybody know
} if there is any other way to do it faster?
}
Dear Jafar,
Are you using W or LaB6 filaments? The former requires an abrasive
and I've used Pol and Wenol, which are pastes and may be faster than
Cl3F3Et + Al2O3. NH4OH will dissolve LaB6 without abrasive, and it is
a lot less work than using abrasive. Since NH4OH is easier to remove
than Al2O3, the total process should be quicker even though you will
have to leave the Wehnelt in the NH4OH for longer than it takes to
polish it with abrasive; furthermore, there is no chance of leaving
scratches with NH4OH.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 16:27:33 2004

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Sorry, I didn't make myself clear. What I want to do
is to embed my powder sample in some kind of epoxy and
then section it after it is cured. M-bond 610 is
usually used to make cross section samples, right?

Ling

--- Karin Pruessner {kpruessn-at-uno.edu} wrote:
}
} Hi Ling,
}
} it depends what you actually want to do and what
} your material is, but both
} M-Bond AE 15 and M-Bond 610 from Vishay (Measurement
} Group) in Raleigh, NC
} are suitable for use in a 200 kV TEM.
}
} Karin
}
}
}
}
} At 10:30 AM 7/22/2004 -0700, you wrote:
}
}
}
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
} -------------------------------------------------------------------------------
} }
} } Hi,
} }
} } Can anyone suggest an embedding epoxy for 200kV
} TEM?
} } Thanks in advance.
} }
} } Ling
} }
} } =====
} } Ling Pan, Ph.D.
} } 195 Materials Research Institute
} } The Pennsylvania State University
} } University Park, PA 16802
} } Tel: (814) 863-1096
} } Fax: (814) 863-8561
} }
} }
} }
} }
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From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 17:46:07 2004

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My advisor, Will Bigelow, taught me over 30 years ago (geez, has it been
that long?) that if you want to clean stainless steel, use stainless
steel cleaner. Revere Ware stainless steel cleaner is still available in
Home Depot, is aqueous, so it leaves no oily residue to outgas, and the
wehnelt ends up clean enough to eat off of..............

John Mardinly
Intel

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Friday, July 23, 2004 2:15 PM
To: microscopy-at-msa.microscopy.com

On Jul 23, 2004, at 3:32 PM, Jafar Al-Sharab wrote:

} We normally Clean the Wehnelt of our TEM with Trichlorofluoroethane
} with alumina powder. The process takes some time. Does anybody know
} if there is any other way to do it faster?
}
Dear Jafar,
Are you using W or LaB6 filaments? The former requires an
abrasive
and I've used Pol and Wenol, which are pastes and may be faster than
Cl3F3Et + Al2O3. NH4OH will dissolve LaB6 without abrasive, and it is
a lot less work than using abrasive. Since NH4OH is easier to remove
than Al2O3, the total process should be quicker even though you will
have to leave the Wehnelt in the NH4OH for longer than it takes to
polish it with abrasive; furthermore, there is no chance of leaving
scratches with NH4OH.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 19:15:23 2004

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Dear Jafar,

Three separate pieces of advice:

1. Get spare Wehnelt, clean it and store in the
hermetically sealed plastic bag. Use pre-cleaned
wehnelt to service the instrument and clean used one
at your convenience.

2. To ease cleaning, soak the used Wehnelt overnight
in diluted solution of the cleaner used for surgical
SST instruments, like Alconox or other. Rinse
thoroughly in DI water and then clean or polish as you
do usually. Concentration for the soaking solution
will have to be found empirically, as it depends on
the particular cleaner you use and contaminants.

3. Use high quality DI instead of tap water to dilute
your cleaner, works much better.

4. "Handbook of electron tube and vacuum techniques"
by Fred Rosebury, AVS Classics series, lists on page
15 few acid-based recipes for SST cleaning. SS-3,
based on HF and HNO3 at room temperature should
dissolve any contaminants, including tungsten, quite
rapidly, but I would rather prefer to use milder
cleaner and some polishing then deal with HF.

Hope it helps,

Valery Ray
Particle Beam Systems
& Technology, PBS&T
www.partbeamsystech.com

Jafar Al-Sharab {jafarhan-at-rci.rutgers.edu} wrote:

------------------------------------------------------------------------------
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Society of America

} Dear All,
}

We normally Clean the Wehnelt of our TEM with
Trichlorofluoroethane with
alumina powder. The process takes some time. Does
anybody know if there
is any other way to do it faster?

Thank you

Jafar

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 23 20:09:58 2004

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We are looking for a new epoxy for wedge prep to replace our G2 and
M-Bond. The epoxy should have high penetrating ability so that it can
flow into some 90nm trenches, can cure at room temperature, and will not
be softened by acetone. If there are any suggestions, please post them.
Thank you.

John Mardinly
Intel

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 24 09:46:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (chenhong-at-mailst.xjtu.edu.cn) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Saturday, July 24, 2004 at 03:29:24
---------------------------------------------------------------------------

Email: chenhong-at-mailst.xjtu.edu.cn
Name: Chen Hong

Organization: Xi'an JiaoTong Univ.

Education: Graduate College

Location: XI'an ShaanXi P.R.China

Question: Hello,
I am searching for a microscope to observe the specimen put in the middle of a 20*30*20cm water tank, the working distance should be about 7cm and the magnification should be about 150X.

Sincerely appreciated any help.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 24 11:24:25 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Caroline

--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 24 16:45:18 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (taylor-at-research.ge.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, July 24, 2004 at 16:11:28
---------------------------------------------------------------------------

Email: taylor-at-research.ge.com
Name: Seth Taylor

Organization: GE Research

Title-Subject: [Microscopy] [Filtered] MListserver: Embedding media for hydride particles

Question: Hi folks,

Can anyone suggest appropriate embedding media for room temperature microtomy of metal hydride particles? The hydride particles are highly reactive and foam extensively when placed in epoxy (presumably due to reaction with oxygen). I have also tried using paraffin as an embedding medium (for cryo-microtomy), but unfortunately that material is highly beam sensitive in the TEM. Ideally, I'd like to use something that won't react with the hydrides, can be microtomed at room temperature, and won't damage extensively under the electron beam. If carbon coating the microtomed sections is necessary, that won't be a problem.

Thanks in advance for any suggestions you might have.

Seth Taylor
Niskayuna, NY

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Jul 24 23:20:14 2004

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We are in the final phase of construction of a new material science and
chemical engineering building that will also accommodate a TEM facility
(JEOL-2010F & Topcon-002B). Much work and thought has gone into the design
of the facility; such as isolating the concrete foundation/floor slab, as
well as distancing 3-phase electrical services, large current devices, e.g.
motors, etc. and large vibration sources, e.g. elevator. However, there
remain a few areas of concern for which we are soliciting feedback.

1) Regarding TEM room air temperature stability, we noticed exhaust ducts in
lieu of the traditional return air ducts that are coupled with room air
supply ducts. We presented the JEOL installation requirements to the
building engineers prior to the ground breaking. However, we are concerned
whether sufficient attention to the necessary HVAC details have been
addressed. Subsequently, we are considering obtaining the services of a
consultant with the appropriate HVAC qualifications pertaining to room air
delivery and control for a TEM facility. Does anyone have a recommendation?

2) We have requested that any metal work (electrical systems, conduit,
ducts, fire sprinklers, etc.) not directly associated with the TEMs be
removed from within a 12-foot diameter floor-to-ceiling cylinder centered on
the TEM column. The question was raised whether the conduit for electrical,
smoke/fire detection systems attached to the 12-foot ceiling (concrete floor
above the column) would also need to be relocated. Can any one share their
knowledge and/or experience in this area?

3) Is anti-static flooring in a TEM room necessary? Is this more important
to those servicing the TEM compared to it being necessary for the TEM
operator?

We are requiring that JEOL perform a site survey to qualify the rooms before
relocating the TEMs to this new facility.

Thank you in advance for your responses.

Thomas A. Rawdanowicz
North Carolina State University
Department of Materials Science & Engineering
2142 Burlington Engineering Lab., Box 7916
Raleigh, North Carolina 27695-7916

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 25 09:26:40 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

} }
} } The Mount Sinai School of Medicine in New York invites applications for
} } the Director of the Microscopy Shared Research Facility. The facility
} } is one of 10 institutional Shared Research Facilities that bring
} } state-of-the-art instrumentation and methodologies crucial to modern
} } biomedical research within the reach of all faculty and graduate
} } students. The director will have a faculty appointment and advancement
} } in either the Research or Academic Track.
} }
} } This institutional multi-user, microscopy facility includes: a BioRad
} } Radiance multi-photon laser scanning microscopy system, 2 confocal
} } laser scanning microscopes (Zeiss 510 META and Leica TCS-SP-uv), a TEM
} } equipped with a CCD camera, ultramicrotomes, a cryoultramicrotome, 3
} } widefield fluorescence microscopes, a live-cell imaging system and
} } several computers with various image analysis and digital deconvolution
} } programs.
} }
} } The director will oversee and participate in microscopy-based projects,
} } consult with research scientists for experimental design and review of
} } results, train facility users in microscope operation & image analysis,
} } participate in grant writing, and supervise 2 full time technicians.
} } Teaching in the medical & graduate schools is also possible.
} }
} } Applicants should send a cv or resume including the names of two
} } references to
} }
} } Sandra K. Masur, PhD
} } Faculty Coordinator Shared Research Facilities
} } Dean for Faculty Development
} } Professor of Ophthalmology
} }
} } Mount Sinai School of Medicine
} } Box 1183
} } 1 Gustave Levy Place
} } New York NY 10029-6574
} } telephone: 212-241-0089
} } fax: 212-289-5945
} }
} } sandra.masur-at-mssm.edu

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 25 14:26:09 2004

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Dear Thomas,

2 cents on metal conduits in EM lab: keeping them
away
from the TEM will only help in any case. More
important however is to make sure that conduits will
not carry any ground loop currents. In some areas
code
requires to connect ground of electrical loads and
ground pins of the electrical outlets not only to the
dedicated ground wire, but ALSO to the metal
conduits.
If this is a case in your area, the conduit may carry
significant AC currents and become a source of strong
EMI.

Cheers,

Valery Ray
Particle Beam Systems
& Technology
} www.partbeamsystech.com

--- "Thomas A. Rawdanowicz" {tarawdan-at-unity.ncsu.edu}
wrote:

}
}
}
------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------
}
} We are in the final phase of construction of a new
} material science and
} chemical engineering building that will also
} accommodate a TEM facility
} (JEOL-2010F & Topcon-002B). Much work and thought
} has gone into the design
} of the facility; such as isolating the concrete
} foundation/floor slab, as
} well as distancing 3-phase electrical services,
} large current devices, e.g.
} motors, etc. and large vibration sources, e.g.
} elevator. However, there
} remain a few areas of concern for which we are
} soliciting feedback.
}
} 1) Regarding TEM room air temperature stability, we
} noticed exhaust ducts in
} lieu of the traditional return air ducts that are
} coupled with room air
} supply ducts. We presented the JEOL installation
} requirements to the
} building engineers prior to the ground breaking.
} However, we are concerned
} whether sufficient attention to the necessary HVAC
} details have been
} addressed. Subsequently, we are considering
} obtaining the services of a
} consultant with the appropriate HVAC qualifications
} pertaining to room air
} delivery and control for a TEM facility. Does anyone
} have a recommendation?
}
} 2) We have requested that any metal work (electrical
} systems, conduit,
} ducts, fire sprinklers, etc.) not directly
} associated with the TEMs be
} removed from within a 12-foot diameter
} floor-to-ceiling cylinder centered on
} the TEM column. The question was raised whether the
} conduit for electrical,
} smoke/fire detection systems attached to the 12-foot
} ceiling (concrete floor
} above the column) would also need to be relocated.
} Can any one share their
} knowledge and/or experience in this area?
}
} 3) Is anti-static flooring in a TEM room necessary?
} Is this more important
} to those servicing the TEM compared to it being
} necessary for the TEM
} operator?
}
} We are requiring that JEOL perform a site survey to
} qualify the rooms before
} relocating the TEMs to this new facility.
}
} Thank you in advance for your responses.
}
}
} Thomas A. Rawdanowicz
} North Carolina State University
} Department of Materials Science & Engineering
} 2142 Burlington Engineering Lab., Box 7916
} Raleigh, North Carolina 27695-7916
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 25 14:38:52 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Sylvain,

The easiest way of measuring high resistivity is to
use picoammeter and a voltage source to measure
leakage current flowing through high-resistivity
sample. I like Keithley 6487 model (no commercial
interest here), since it combines the picoammeter and
a voltage source in one unit. See this page:

http://www.keithley.com/servlet/Data?id=4645"} http://www.keithley.com/servlet/Data?id=4645

and also a "Low Level Measurements" book from Keithley
Instruments (it is a free literature) for the details
on high resistivity measurement techniques.

On the other note, I am not sure that mixing
conductive powder with the resin will reduce
resistivity before impacting the transparency. To
affect resistivity, conductive particles should be
close enough so some current will start tunneling
between them. By that time optical transparency could
be significantly impacted... .

Does anyone of listers aware of optically transparent
conductive glue? I'd be very interested to know if it
exists.

Back to the charging issue, why can't you use a FIB to
deposit a narrow conductive stripe (C, Pt, W, or Au,
whatever is available to you) between the die and a
sample holder? Use low current for deposition close to
the die to minimize overspray. If distance from the
sample holder to the die is prohibitive for FIB
deposition, use some sliver-paint, applied under a
microscope, to get close to the die first, and then
FIB deposition to connect the die to a silver paint.
Thin layer of carbon can also be deposited by imaging
in oil-contaminated SEM. Other approach to deal with
charging would be to image a die by ESEM in a water
vapor atmosphere.

Hope it helps,

Valery Ray
Particle Beam Systems
& Technology
www.partbeamsystech.com

The Microscopy ListServer -- Sponsor: The Microscopy
Society of America {BR} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver {BR} On-Line
Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html {BR} ------------------------------------------------------------------------------- {BR} {BR} Hi
all! {BR} {BR} To solve the charging phenomenon problem
of HR FESEM observations, in my {BR} application
(polished cross-sections of Silicium dies samples,
coated in {BR} epoxy resin, i'm trying to chargea very
little quantity of resin with a {BR} very little
quantity of metal powder (copper, silver graphite),
in {BR} order to keep the resin transparent, just enough
to evacuate charges. {BR} {BR} Is there a way to measure
the very high resistivity of this
charged {BR} resin? {BR} {BR} My goal is to obtain
resistivities { 10e12 ohm*cm... {BR} {BR} thanx in
advance {BR} {BR} Sylvain
MAURY {BR} {BR} {BR} {/BLOCKQUOTE} {/DIV} {/DIV} {/DIV} {/DIV} {/DIV} {/DIV}

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 25 15:19:11 2004

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Wow! That sounds really laborious, as I imagine you will be battling with the
evaporation of the tric while you're doing it.

I sonicate mine in a concentrated ammonia solution (about 30% of the lab
'concentrated') for about 10 minutes. This dissolves much of the deposit and softens
the rest.

Then I polish with household silver cleaner ('Silvo' brand). This is a slightly abrasive
runny cream. I have been told that the one for silver is less abrasive than the one for
brass ('Brasso').

Then I wash it under the hot tap, rinse with methanol, and dry it with tissues.

Takes about 30 minutes from go to whoa.

cheers

rtch

Date sent: Fri, 23 Jul 2004 15:32:14 -0700
To: microscopy-at-ns.microscopy.com
} From: Jafar Al-Sharab {jafarhan-at-rci.rutgers.edu}

So far I have received 8 automated 'Out of Office' replies to my posting of about two
hours ago, and I guess I'll receive a similar number from this one.

Guys, this is not reasonable, and it's a decided inhibition to making a posting.

On the XRF and Plasma listservers, subscribers who clutter the ether and posters'
inboxes with "Out of Office Auto Reply" messages are summararily unsubscribed.

If you're going away, how about temporarily unsubscribing from the list?

Nestor, do you have any policy/recommendations on this?

While I'm at it, I suppose I may as well make myself really unpopular ------ I think that
everyone who posts should identify themselves, as a courtesy.

Signatures are real easy to do.

Happy Monday morning, from one whose Mondays start before anyone else's.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 25 18:51:36 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Richie,

In short, the reason for the DP valve is:
How do you know what is plugged if you can't eliminate the DP line as a
possible cause of lower flow?
Yes, you could install three branch flow meters with individual shutoffs to
isolate the cause. With three meters you can instantly tell which line or
lines are plugged.

You now know where the blockage is. What do you do next? If the lens
lines are plugged, then how do you apply full or low partial back pressure
with an open DP line bypassing most of the flow? Isolating the DP line
means you can forward or backwards flush the lens lines without loss of
pressure or bypass through the DP line.

If you apply nitrogen, like you can on a Philips, then an open DP line will
again bypass the gas.

The DP valve gives your serviceman more options to control how he is going
to try to dislodge or cleanout the blockage. He can use nitrogen or water.
He can flush all lines or eliminate the DP line. He can vary the bypass
amount in the DP line with a partially closed DP valve.

Ditto all that with the lens end caps that fit onto the bulkhead union
water fittings on a Philips.

The DP valve is a clean install and easy to do. A Nupro brass valve with
tubing port connections works fine in the DP line.

Paul

From MicroscopyL-request-at-ns.microscopy.com Sun Jul 25 19:45:34 2004

Contents Retrieved from Microscopy Listserver Archives
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Richtie

Yes there is a policy, which has been in place for over decade, it is in the
Rules/FAQ that everyone receives, when they subscribe.

http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html

It deals both points that you raise, namely - it says
1.) people should identify themselves and
2.) not to use " Out of the Office", but unsubscribe.

Unfortunately, (for you) the out of office replies only go to the poster
they don't go to the list. This was they only way I can manage the system.
I can't realistically police this one. Unless I get reports of abuse, or mail loops start.
If this happens, then I step in and remove the individual. But I have to know about
the problem.

So... by making this posting I'll presumably get the same number of Out-of-the-Office
posting you just got.

Sigh...

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 04:47:35 2004

Contents Retrieved from Microscopy Listserver Archives
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We used to use cleaning paste etc until a service engineer
showed me an easier method. Now I sonicate in about 5%
Decon 90, rinse and sonicate in acetone.

Dave

On Fri, 23 Jul 2004 15:32:14 -0700 Jafar Al-Sharab
{jafarhan-at-rci.rutgers.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} } Dear All,
} }
}
} We normally Clean the Wehnelt of our TEM with Trichlorofluoroethane with
} alumina powder. The process takes some time. Does anybody know if there
} is any other way to do it faster?
}
} Thank you
}
} Jafar
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 07:03:49 2004

Contents Retrieved from Microscopy Listserver Archives
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Jafar,

If you use abrasive polishing, here is a labor saving hint.

Wooden shaft cotton swabs will fit a 3/32" collet for a "Dremel Tool" (small
rotary grinder). Cut the swab so that only a very short piece of shaft
protrudes from the collet or it will break off. Wear safety glasses.

I use POL or Wenol with the "high speed rotary q-tip" and it is very
effective.

Hint 2: To clean the ID of the hole, break (or cut) the swab shaft to a
taper and use only the tapered wooden shaft and some polishing compound.

Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Jafar Al-Sharab [mailto:jafarhan-at-rci.rutgers.edu]
Sent: Friday, July 23, 2004 6:32 PM
To: microscopy-at-ns.microscopy.com

} Dear All,
}

We normally Clean the Wehnelt of our TEM with Trichlorofluoroethane with
alumina powder. The process takes some time. Does anybody know if there
is any other way to do it faster?

Thank you

Jafar

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 07:31:15 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

One method I was taught years ago by a service tech was that any plated
parts could be cleaned by immersion in plain household ammonia, (not the
sudsy type) or a 5% solution of ammonium hydroxide. Depending on how
contaminated the cap is, it will take 5 to 20 minutes. The plus side of
this method is, a quick rinse in distilled water followed by alcohol or
acetone and the cap is ready for use.

Mannie Steglich
Tech Dir E M Lab
U T M D Anderson Cancer Center

Jafar Al-Sharab {jafarhan-at-rci.rutgers.edu}

07/23/2004 05:32 PM

To:
microscopy-at-ns.microscopy.com
cc:

} Dear All,
}

We normally Clean the Wehnelt of our TEM with Trichlorofluoroethane with
alumina powder. The process takes some time. Does anybody know if there
is any other way to do it faster?

Thank you

Jafar

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 08:03:50 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Gervais.Sawyer-at-bcuc.ac.uk) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, July 26, 2004 at 03:16:58
---------------------------------------------------------------------------

Email: Gervais.Sawyer-at-bcuc.ac.uk
Name: Gervais Sawyer

Organization: Forest Products Research Centre

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I have been asked to image 50 micron glass spheres used as filler in animal adhesive formulations to see if the adhesive has wetted the beads. Can anybody suggest a suitable microscopy technique? Any EM approach requiring drying regimes will surely only give artefacts.

Many thanks

Gervais Sawyer

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 09:24:13 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Gervais,
It is possible that viewing the beads through phase contrast
or Nomarski optics would let you distinguish beads that have been
coated with adhesive from those that havent. The latter technique
would be more useful if you expect that a poorly wet bead would have
a patchy distribution over the surface of the beads (as opposed to
all or nothing wetting). Whether these methods will actually work
would depend on the refractive index of the adhesive, how thick a
layer it forms, and what kind of a layer it forms, impossible for me
to predict from first principles, but easy enough to have a look
under the microscope.
Hope this helps
Tobias Baskin

} Monday, July 26, 2004 at 03:16:58
} ---------------------------------------------------------------------------
}
} Email: Gervais.Sawyer-at-bcuc.ac.uk
} Name: Gervais Sawyer
}
} Organization: Forest Products Research Centre
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: I have been asked to image 50 micron glass spheres used as
} filler in animal adhesive formulations to see if the adhesive has
} wetted the beads. Can anybody suggest a suitable microscopy
} technique? Any EM approach requiring drying regimes will surely only
} give artefacts.
}
} Many thanks
}
} Gervais Sawyer
}
} ---------------------------------------------------------------------------

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 11:56:24 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Jafar,

To answer your question, I sure do know how to clean a Wehnelt! After
almost
40 years in the business it seems to me that people still work with
techniques
that make this task far too complicated. Set out below is a technique that
was developed, like many good ideas, from an initial mistake. Try this out
and keep away from any technique that is going to take you hours to follow,
there is no real point!

The procedure, like may other maintenance tips, is found on our
"Monitoring and Maintaining the Electron Microscope" interactive CD.

There are two parts to an ideal cleaning procedure for an EM

1. Wet cleaning is by far the best route, no cotton, no particles, no
fiddling, just liquids doing the job.
2. Having a solvent for the media that you wish to remove (in this case
ammonia is a solvent for tungsten)

The Procedure For W
The cathode assembly is placed, aperture face upwards, in a beaker of stock
ammonia solution diluted 3 parts ammonia to one part water. The stock
solution is normally about 40% ammonia. After a maximum of 15 minutes in
the ultrasonic cleaner the beaker is placed under running water and
thoroughly flushed through. Care should taken to ensure that none of the
clamping or alignment screws have fallen out of the cathode assembly and
could be flushed away! The cathode is then washed with alcohol before being
dried with a hair drier. A new filament is fitted and centred. The
assembly is checked for cleanliness by observing with a 20X lens or
binocular microscope prior to re installation in the microscope. Total time
for this procedure less than 25 minutes.

Safety
Great care was taken not to allow the ammonia solution to make contact with
the skin or eyes of the operator. When flushing the solution through with
water its flow should be set so as not to splash the solution over the
operator prior to placing the beaker under the flow.

I know this works, try it?

Steve Chapman
Senior Consultant Protrain
Electron Microscopy Training and Consultancy World Wide
Tel +44 (0)1280 816512 Fax +44 (0)1280 814007 Mob +44 (0)7711 606967
www.emcourses.com

----- Original Message -----
} From: "Jafar Al-Sharab" {jafarhan-at-rci.rutgers.edu}
To: {microscopy-at-ns.microscopy.com}
Sent: Friday, July 23, 2004 11:32 PM

Another reason to NOT use the 'Out of office' feature in Outlook is that
it automatically replies to randomly generated spam, and sends a signal
that the address is a real, live account, in which case the address is
recorded, sold to other spammers, etc., which will dramatically increase
the amount of spam you get. In addition, your 'out of office' replies
are typically undeliverable, which gets you another message from your
server, and rapidly fill up your mailbox.

John Mardinly
Intel

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Sunday, July 25, 2004 4:27 PM
To: microscopy-at-ns.microscopy.com

So far I have received 8 automated 'Out of Office' replies to my posting
of about two
hours ago, and I guess I'll receive a similar number from this one.

Guys, this is not reasonable, and it's a decided inhibition to making a
posting.

On the XRF and Plasma listservers, subscribers who clutter the ether and
posters'
inboxes with "Out of Office Auto Reply" messages are summararily
unsubscribed.

If you're going away, how about temporarily unsubscribing from the list?

Nestor, do you have any policy/recommendations on this?

While I'm at it, I suppose I may as well make myself really unpopular
------ I think that
everyone who posts should identify themselves, as a courtesy.

Signatures are real easy to do.

Happy Monday morning, from one whose Mondays start before anyone else's.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext
87713
Microanalyst Fax : 64 9
3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 13:02:07 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Ritchie,
I agree with you partially. If I am going out of town for a week or more, I will unsubscribe, but not for a day or two. However, I want people where I work to know that I am not in the office if they send me a message. I can't edit Outlook to not send it in response to a listserver message -I've tried. I have put "out of office" as a search item to send such messages to a junk email location and then simply delete them later. It is the best solution that I came up with.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Sunday, July 25, 2004 7:27 PM
To: microscopy-at-ns.microscopy.com

So far I have received 8 automated 'Out of Office' replies to my posting of about two
hours ago, and I guess I'll receive a similar number from this one.

Guys, this is not reasonable, and it's a decided inhibition to making a posting.

On the XRF and Plasma listservers, subscribers who clutter the ether and posters'
inboxes with "Out of Office Auto Reply" messages are summararily unsubscribed.

If you're going away, how about temporarily unsubscribing from the list?

Nestor, do you have any policy/recommendations on this?

While I'm at it, I suppose I may as well make myself really unpopular ------ I think that
everyone who posts should identify themselves, as a courtesy.

Signatures are real easy to do.

Happy Monday morning, from one whose Mondays start before anyone else's.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 14:25:24 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

It seems that I have raised a few hackles, but I have received (real replies, not only the
inevitable Out of Office Auto Replies) roughly the same amount of support as of
opposition.

Here is a possible solution.

To avoid cluttering the ether and the inboxes of others with meaningless auto replies,
how's about getting your IT people to provide you with a new and different email alias
for list purposes?

Thus to the business world you could remain captainjameskirk-at-starship.com, and to
this and other lists you would jim-at-starship.com.

Or whatever rings your bell.

When you are out of the office, you can set your 'business' one to autoreply, while the
'list' address's inbox keeps all the list stuff accumulating until you return.

Sometimes my own brilliance terrifies me.

cheers

rtch

Date sent: Sun, 25 Jul 2004 19:56:49 -0500
To: microscopy-at-microscopy.com
} From: "Nestor J. Zaluzec" {zaluzec-at-microscopy.com}

On Jul 24, 2004, at 9:28 PM, Thomas A. Rawdanowicz wrote:

} 1) Regarding TEM room air temperature stability, we noticed exhaust
} ducts in
} lieu of the traditional return air ducts that are coupled with room air
} supply ducts. We presented the JEOL installation requirements to the
} building engineers prior to the ground breaking. However, we are
} concerned
} whether sufficient attention to the necessary HVAC details have been
} addressed. Subsequently, we are considering obtaining the services of
} a
} consultant with the appropriate HVAC qualifications pertaining to room
} air
} delivery and control for a TEM facility. Does anyone have a
} recommendation?
}
} 2) We have requested that any metal work (electrical systems, conduit,
} ducts, fire sprinklers, etc.) not directly associated with the TEMs be
} removed from within a 12-foot diameter floor-to-ceiling cylinder
} centered on
} the TEM column. The question was raised whether the conduit for
} electrical,
} smoke/fire detection systems attached to the 12-foot ceiling (concrete
} floor
} above the column) would also need to be relocated. Can any one share
} their
} knowledge and/or experience in this area?
}
} 3) Is anti-static flooring in a TEM room necessary? Is this more
} important
} to those servicing the TEM compared to it being necessary for the TEM
} operator?
}
} We are requiring that JEOL perform a site survey to qualify the rooms
} before
} relocating the TEMs to this new facility.
}
Dear Thomas,
1) We had consultants in to evaluate our A/C system, and, based on
the temperature stability and maximum air flow rate requirements, they
suggested ~60 ft^2 of exhaust manifold. Furthermore, the original A/C
setup was designed to use a baseboard exhaust that had been proposed
for the evacuation of SF6--apparently the designers thought that
combining the two functions would be more efficient. Unfortunately,
that design did not draw the air past the TEM column, so we had to redo
the A/C exhaust completely.
2) We did not relocate the conduit for lights, fire sprinklers, or
other electrical lines, but there is no measurable effect on EM stray
fields, nor was there any problem meeting the specs for the EM. It is
never a bad idea to move current-carrying wires away from the column,
and, if your scope operates at a voltage lower than 300 kV, you may see
effects from smaller fields than would affect our scope.
3) We did not put in anti-static flooring, and we have not seen any
problem.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 16:39:12 2004

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good idea on the surface. But I suspect that Nestor
won't like it.

As I found out some many months ago, Nestor has each
member's e-mail address linked to the group/list.
Each person can only have one address. I had tried
to get a second address subscribed but no go. perhaps
identical TLDs makes a difference. But probably not.

I would suggest that when Out of Office is turned on
that the Subject line include that. Not all do this. If
it is in the subject line, my incoming filter will delete
the whole Out of Office message. That is handy and
appreciated.

gary g.

At 12:39 PM 7/26/2004, you wrote:

} It seems that I have raised a few hackles, but I have received (real
} replies, not only the
} inevitable Out of Office Auto Replies) roughly the same amount of support
} as of
} opposition.
}
} Here is a possible solution.
}
} To avoid cluttering the ether and the inboxes of others with meaningless
} auto replies,
} how's about getting your IT people to provide you with a new and different
} email alias
} for list purposes?
}
} Thus to the business world you could remain captainjameskirk-at-starship.com,
} and to
} this and other lists you would jim-at-starship.com.
}
} Or whatever rings your bell.
}
} When you are out of the office, you can set your 'business' one to
} autoreply, while the
} 'list' address's inbox keeps all the list stuff accumulating until you return.
}
} Sometimes my own brilliance terrifies me.
}
} cheers
}
} rtch
}
}
}
}
} Date sent: Sun, 25 Jul 2004 19:56:49 -0500
} To: microscopy-at-microscopy.com
} } From: "Nestor J. Zaluzec" {zaluzec-at-microscopy.com}
} Subject: [Microscopy] Administrivia: Out of Office Replies..
}
} }
} }
} } ----------------------------------------------------------------------
} } -------- The Microscopy ListServer -- Sponsor: The Microscopy Society
} } of America To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------
} } ---------
} }
} }
} } Richtie
} }
} } Yes there is a policy, which has been in place for over decade, it is
} } in the Rules/FAQ that everyone receives, when they subscribe.
} }
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} } It deals both points that you raise, namely - it says
} } 1.) people should identify themselves and
} } 2.) not to use " Out of the Office", but unsubscribe.
} }
} } Unfortunately, (for you) the out of office replies only go to the
} } poster they don't go to the list. This was they only way I can manage
} } the system. I can't realistically police this one. Unless I get
} } reports of abuse, or mail loops start. If this happens, then I step in
} } and remove the individual. But I have to know about the problem.
} }
} } So... by making this posting I'll presumably get the same number of
} } Out-of-the-Office posting you just got.
} }
} } Sigh...
} }
} } Nestor
} } Your Friendly Neighborhood SysOp
} }
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 20:15:11 2004

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Gary

What you said below is not completely correct. It is true there is a problem
with your particular domain(s). That, however, is only a function of how you were
trying to use the system. Yours is a special case, which we never solved satisfactorially.

In any event, there are a number of people subscribed at multiple addresses.
I, for example, receive Listserver Email at 3 different addresses. I do this as
a monitoring as well as a convenience function, other people do it for reasons that
which have been discussed previously.

If someone wishes to subscribe 2 different Email address that is perfectly acceptable.
I only remind everyone that posting to the Listserver is only
permitted from a user whose "Email Header/Envelope" has a return address which
is on the master subscription list, and this address MUST be an EXACT match
with the subscription address.

If you are forced by your Employer to use out of the office protocols, then setting up
a 2nd Email address which only receives Listserver mail, could solve your problem.

The key to making this "solution" work is that these have to be 2 different "mailboxes",
not aliases to the same mailbox. Email addresses which point to the same destination
mailbox will not work. The reason for this is obvious, your Out of the Office message
is conntect to your "mailbox" not with your Email address.

The subtleness of this difference is beyond the bounds of this list and I do not wish
to bore the world with the details.

If someone has any more detailed questions, just contact me off-line

Cheers...

Nestor
Your Friendly Neighborhood SysOp

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 20:59:36 2004

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I'm driving to Savannah from Madison WI for mm2004. I could use another
rider from here or anywhere in between here and Savannah.
Pete

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 21:08:00 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jmurray-at-rjlg.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, July 26, 2004 at 09:24:13
---------------------------------------------------------------------------

Email: jmurray-at-rjlg.com
Name: Jeff

Organization: RJ Lee Group

Title-Subject: [Microscopy] [Filtered] MListserver: Optical Microscopy Image Software

Question: We are looking for image software which automatically overlays information (such as scale or some other relevant info) on optical microscopy images. Are there any products out there that currently have this capability?

I know you can add info with Photoshop, but I am looking for a more automated method which adds the info as photo is taken.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 21:09:39 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mccaulak-at-wfu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, July 26, 2004 at 12:38:18
---------------------------------------------------------------------------

Email: mccaulak-at-wfu.edu
Name: Anita McCauley

Organization: Wake Forest University

Title-Subject: [Microscopy] [Filtered] MListserver: CTB-biotin visualization

Question: I am looking for any suggestions regarding the visualization of the neural tracer cholera toxin subunit B, CTB, in tissue sections.

The CTB was injected into either the eye or the cortex and allowed to transport for 2 days. The tissue was fixed and sliced and now I am attempting to label the CTB with DAB. The CTB has biotin conjugated to it already. Since it already has biotin, I have tried proceeding with an ABC reaction (Vector Kit) and then DAB. Twice, varying the time in ABC, the reaction has not worked.

Besides CTB concentration and injection issues as possible causes of the failure, I am trying to determine if the visualization reaction I am trying to perform is correct. If anybody can make any suggestions for visualizing something already tagged with biotin, I would appreciate it.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 21:42:40 2004

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Sometimes the out of office replies are generated by an inhouse Microsoft
Exchange mail server. The IT person in charge of the server can set it to
send/not send out of office replies to the internet. Seems that most mail
admins don't turn off Microsoft's default to send OOF replies to the whole
world. The person using Outlook sometimes has no real control over this
function.

Bob

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 22:08:04 2004

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ImageJ and Photoshop both have methods for automation. Actually, most
imaging software can do this and you may already have these features in
the package you are using. However, ImageJ is both extremely powerful and
free and Photoshop is extremely popular.
-Michael

___________________________________
WORK: http://www.aecom.yu.edu/aif/
PERSONAL: http://www.art-studio.us/

On Mon, 26 Jul 2004, by way of MicroscopyListserver wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jmurray-at-rjlg.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, July 26, 2004 at 09:24:13
} ---------------------------------------------------------------------------
}
} Email: jmurray-at-rjlg.com
} Name: Jeff
}
} Organization: RJ Lee Group
}
} Title-Subject: [Microscopy] [Filtered] MListserver: Optical Microscopy Image Software
}
} Question: We are looking for image software which automatically overlays information (such as scale or some other relevant info) on optical microscopy images. Are there any products out there that currently have this capability?
}
} I know you can add info with Photoshop, but I am looking for a more automated method which adds the info as photo is taken.
}
} ---------------------------------------------------------------------------
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 22:19:30 2004

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Dear Gervais,

Sounds like a job for AFM. It can give you a topography image to show
where the adhesive is as well as an adhesive force measurement.

If you would like to discuss this further, please contact me off-line.

Best regards,

At 08:14 AM 7/26/2004, Gervais.Sawyer-at-bcuc.ac.uk wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Jul 26 22:35:03 2004

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At 10:28 PM 7/26/2004, Barbara Foster wrote:
} Dear Gervais,
}
} Sounds like a job for AFM. It can give you a topography image to show
} where the adhesive is as well as an adhesive force measurement.
}
} If you would like to discuss this further, please contact me off-line.
}
} Best regards,
} Barbara Foster

*******************************************************************************************************************
We've moved!
MME is now at:
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011

} At 08:14 AM 7/26/2004, Gervais.Sawyer-at-bcuc.ac.uk wrote:
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 00:20:29 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Gervais Sawyer wrote:
===========================================================
Question: I have been asked to image 50 micron glass spheres used as filler
in animal adhesive formulations to see if the adhesive has wetted the beads.
Can anybody suggest a suitable microscopy technique? Any EM approach
requiring drying regimes will surely only give artefacts.
=============================================================
This might sound a bit hairbrained, but some years ago we did something
similar.

Draw down (using, for example, a tooth pick) on some rigid surface some
ordinary 5 minute epoxy. When the epoxy is starting to harden but is still
very very tacky, sprinkle some of your glass spheres onto the surface of the
curing epoxy. The point is that the epoxy must be hard enough that the
glass beads won't sink into it and become submerged.

After it is completely cured, we used our own SPI "Wet Replica Kit" which is
our silicone based replication system, see URL
http://www.2spi.com/catalog/spec_prep/wet_rep_kits.shtml

The silicone system is spread over the now immobilized glass spheres and
when the silicone is removed (and it will lift off easily) there will be a
perfect replica of the glass beads and any coatings. The disadvantage of
this approach is that one can not go above 700x in the SEM before seeing
structure from the replication system. But this could be high enough
resolution to see the coating. I would also recommend making a "positive"
of the "negative" replica since the resulting micrographs will be so much
easier to understand.

If that method fails, you can Pt/C shadow the immobilized glass spheres and
then remove the replica, using poly acrylic acid (PAA) if necessary in order
to have an even better look. Or AFM might be useful (something we never did
ourselves).

For either of these two approaches to work, however, the glass beads ideally
would be submerged into the curing epoxy to their equatorial lines.

Disclaimer SPI Supplies offers the "Wet Replica Kit" to our commercial
customers.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 07:53:26 2004

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Torino 27 July 2004
(ITALY)

Hi all,
I’d like to study the anatomy and histology of a land snail.
I wonder how to kill or to anaesthetise the little creature without procure it any pain and do not damage the tissues.
Would be important that it could not withdraw into its shell.
Someone knows a web site where I could find anatomy charts and some instruction about their dissection?
Thank you,
Best Regards,
Massimo

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 07:55:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Take a 1-3 ul droplet of your biotinylated probe and spot it on a 0.5 cm
wide strip of nitrocellulose paper (get it from somebody who does western
blots). block the rest of the sites on the paper by incubation in 1% bsa
for several hours. incubate in your streptavidin-hrp or ABC kit and then
develop. you can do these steps in a microfuge tube or small glass
testtube. it should show a brown spot if it is working.

At 09:20 PM 07/26/04 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 08:13:26 2004

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Hello All,

Has anyone any experience trying to sputter coat* with pure niobium?
If so, what were your results?
*My coater is the common magnet loaded target, DC/argon plasma type
("magnatron", but not microwave tube) with rough pump only.

TIA,
Woody
BWXT Services

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 08:22:26 2004

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Hi Anita:

Is the DAB fresh? If has been around the lab more than a year I
would test it or get a fresh bottle.
Is the peroxide fresh? Hydrogen peroxide turns to water over time so get
a fresh bottle.
Call Vector and talk to them, I have found that they are an excellent
source of information, they can help you trouble shoot the reaction.

Geoff

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 11:04:26 2004

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Not having $100K to purchase a TEM digital camera system, I am
thinking of making my own. I would like to bounce these design ideas
off of the EM community.

The basic design would involve removing the bottom cover plate under
the film camera and having a machinist mill a port to accommodate a
leaded glass window (for example, a viewing port from a TEM). A
separate, thin glass plate coated with a phosphor would be placed
above the leaded glass (inside the vacuum). We would use a
peltier-cooled CCD (such as the Q Imaging system), focused on the
phosphor, to capture the image. The camera system has the necessary
software to capture the 2k x 2k image on a PC.

Obviously, this camera would lack all the wonderful features offered
by the TEM camera manufacturers, but I feel that we could build such
a system for $10-12K.

Something must be wrong with this design, since it seems too simple.
So, any comments and/or suggestions would be appreciated.

Thanks.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 12:44:01 2004

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On Jul 27, 2004, at 9:14 AM, John J. Bozzola wrote:

} Not having $100K to purchase a TEM digital camera system, I am
} thinking of making my own. I would like to bounce these design ideas
} off of the EM community.
}
} The basic design would involve removing the bottom cover plate under
} the film camera and having a machinist mill a port to accommodate a
} leaded glass window (for example, a viewing port from a TEM). A
} separate, thin glass plate coated with a phosphor would be placed
} above the leaded glass (inside the vacuum). We would use a
} peltier-cooled CCD (such as the Q Imaging system), focused on the
} phosphor, to capture the image. The camera system has the necessary
} software to capture the 2k x 2k image on a PC.
}
} Obviously, this camera would lack all the wonderful features offered
} by the TEM camera manufacturers, but I feel that we could build such a
} system for $10-12K.
}
} Something must be wrong with this design, since it seems too simple.
} So, any comments and/or suggestions would be appreciated.
}
Dear John,
Dave Barnard designed and constructed a good system for the HVEM in
Albany. He investigated many different types of camera, coupling,
phosphor, etc. and came up with a high-sensitivity system that would
give video-rate images at very low dose. That particular system was
designed for scanning grids and focussing, so you may want a different
camera, but the rest of his system could be very useful to you.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 14:46:02 2004

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John,

Your estimate is correct under following conditions:

a) 2K x 2K camera is not Peltier cooled,
b) no special TEM software is used,
c) you labor costs $0.00.

Peltier cooled 2K x 2K home-made TEM camera will somewhat exceed $20K,

Nothing is wrong with your idea. But it is not a design yet.

Contact me off-list for further details.

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "John J. Bozzola" {bozzola-at-siu.edu}
To: {Microscopy-at-msa.microscopy.com}
Sent: Tuesday, July 27, 2004 12:14 PM

Have you looked at the cameras sold by SIA, as advertised on pg 69 of the
July Microscopy Today? They are at www.sia-cam.com and 770-232-7785.

No financial interest other than the fact that SIA advertises in MT.

Ron Anderson
MT Editor

-----Original Message-----
} From: John J. Bozzola [mailto:bozzola-at-siu.edu]
Sent: Tuesday, July 27, 2004 12:15 PM
To: Microscopy-at-msa.microscopy.com

Not having $100K to purchase a TEM digital camera system, I am
thinking of making my own. I would like to bounce these design ideas
off of the EM community.

The basic design would involve removing the bottom cover plate under
the film camera and having a machinist mill a port to accommodate a
leaded glass window (for example, a viewing port from a TEM). A
separate, thin glass plate coated with a phosphor would be placed
above the leaded glass (inside the vacuum). We would use a
peltier-cooled CCD (such as the Q Imaging system), focused on the
phosphor, to capture the image. The camera system has the necessary
software to capture the 2k x 2k image on a PC.

Obviously, this camera would lack all the wonderful features offered
by the TEM camera manufacturers, but I feel that we could build such
a system for $10-12K.

Something must be wrong with this design, since it seems too simple.
So, any comments and/or suggestions would be appreciated.

Thanks.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 15:16:06 2004

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Dear Vladimir,
I have used ethylene glycol as a 'boat' solution for sectioning
precipitates and small mineral grains. It worked well - sections floated
off onto the liquid easily and the diamond knife edge stayed wet. The
sections take longer to dry than from a water solution and I found little
contamination. BUT prolonged exposure to ethylene glycol is not good for
you. It can be harmful by inhalation, ingestion or skin absorption. In
particular, I would be concerned about eye irritation and skin
irritation. We have devised a mini-fume hood (dryer hose attached to fume
hood) that stands close to the boat and I have shields in front of the boat
to avoid exposure as much as possible. Subsequently we discovered that
ethylene glycol is hygroscopic and absorbs water readily which made its
usage not practical for our application.
Regards, Susan

} ------------------------------------------------------------------------------
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Susan Belfry,
Microscopy and Microanalysis Facility,
University of New Brunswick, Fredericton, NB, Canada
Phone:(506) 447-3286/453-4887, Fax:(506) 453-3583, Email: belfry-at-unb.ca
www.unbf.ca/mmf

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 15:33:51 2004

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This reminds me a bit of the old Phillips EM 100, which had a
horizontal column, and you looked at the image through a screen at
the end. It looked a bit like the (even older) Bendix washing
machine (remember?)

The main problem that you might encounter is the resolution of the
phosphor screen. As you know, traditional em, where the electron
beam falls directly on film, allows you to make substantial
enlargements with little loss of resolution. The phosphor is
considerably coarser than photographic grain.

So, it depends primarily on how much resolution you need. For a
class of undergraduates, I rigged up something even cruder. We
mounted a commercial digital camera so that it would take pictures
through the viewport. This gave us distorted images which we were
able to correct with photoshop (in batch mode). Naturally, the
resolution was terrible, but we were able to get a set of digital
images that could be used for measurement, labels, etc. by a class of
neophytes. I wouldn't think of printing them at anything larger than
3"x4", even though they were taken at 2048X1500 pixels.

If you like, I can send you some examples.

One more thought...the Zeiss EM 10 used a fiber optic plate to
tranfer images through a vacuum seal so that it was not necessary to
insert film. They claimed pretty good resolution, as I remember. I
believe that such a plate is still available. Hmm.

Good luck with the project.

Joel

}
}
} ----------------------------------------------------------------------
} -------- The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America To Subscribe/Unsubscribe --
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} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
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} ---------
}
} Not having $100K to purchase a TEM digital camera system, I am
} thinking of making my own. I would like to bounce these design ideas
} off of the EM community.
}
} The basic design would involve removing the bottom cover plate under
} the film camera and having a machinist mill a port to accommodate a
} leaded glass window (for example, a viewing port from a TEM). A
} separate, thin glass plate coated with a phosphor would be placed
} above the leaded glass (inside the vacuum). We would use a
} peltier-cooled CCD (such as the Q Imaging system), focused on the
} phosphor, to capture the image. The camera system has the necessary
} software to capture the 2k x 2k image on a PC.
}
} Obviously, this camera would lack all the wonderful features offered
} by the TEM camera manufacturers, but I feel that we could build such a
} system for $10-12K.
}
} Something must be wrong with this design, since it seems too simple.
} So, any comments and/or suggestions would be appreciated.
}
} Thanks.
}
} --
} ##############################################################
} John J. Bozzola, Ph.D., Director
} I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
} 750 Communications Drive - MC 4402
} Southern Illinois University
} Carbondale, IL 62901 U.S.A.
} Phone: 618-453-3730
} Email: bozzola-at-siu.edu
} ##############################################################
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 16:00:14 2004

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Hello,
We may have some grounding problems in the wiring in our building. I was
wondering if anyone knew of techniques to check the quality of ground, or
improve its quality? I contacted the electricians here, but they said
they needed to do more research to figure out how to test the ground.
Thanks
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
Gordon Ante Vrdoljak Electron Microscope Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 17:45:45 2004

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Hi

I have an EDS detector, Be window, about 8 years old.

} From new, its vacuum slowly but inexorably deteriorated, until, after 5 years, it would no
longer make it through a weekend without a Sunday visit to top up the LN2.

So, at great expense (see where I live), I returned it to PGT, where it was pumped and
baked, including leak testing, and returned.

It's been OK, but still has the slow vacuum deterioration, and can still maintain its LN2
through a weekend, but not a long one.

Tolerable for those living on the same landmass as the manufacturer, but it's a major
logistical exercise for me to send it away, and the overall time (almost two months last
time) is a killer.

I am a bit annoyed about this, but

1
For how long should an EDS detector maintain its Dewar vacuum so that it can go for 3
days without a topup? Does anyone know if any particular manufacturers are better or
worse than others?

2
It seems that the leak must be slower than is detected by PGT's testing, so it seems
unlikely that anyone will be able to find the leak and fix it. Is this assumption correct?
Does anyone know of a 3rd party repairman who might succeed where the
manufacturer has failed?

3
I understand that repumping can, in theory, be done by the user, using the SEM's
vacuum system. Has anyone out there done this in the privacy and comfort of their own
lab, and would they be able to help me figure out whether I have the skill and resources
to do it myself?

Maybe I should just save my pennies to replace it.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 18:03:09 2004

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Hello John,

As a manufacturer of these cameras I can tell you that there is a lot more
involved than the picture you are painting in your email. It is certainly
doable and with the right resources you may be able to save some money, but
here are a few things that you need to take into consideration:

The phosphor itself on the glass needs to be optimized for acceleration
voltage
coupling of the phosphor plate to the lead glass to reduce reflections
lens for the camera (as distortion-free as possible, match resolution)
or fiber-optic and coupling to CCD sensor
camera cooling
X-ray shielding
vibration shielding

On the software side you probably need:

shading correction
gain correction
perhaps live FFT
etc.

Once you put all that in and add the cost for development and labor, you
will probably end up with considerably more than 12k.

Give me a call if you want to discuss some of the details.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: John J. Bozzola [mailto:bozzola-at-siu.edu]
Sent: Tuesday, July 27, 2004 10:15
To: Microscopy-at-msa.microscopy.com

Not having $100K to purchase a TEM digital camera system, I am
thinking of making my own. I would like to bounce these design ideas
off of the EM community.

The basic design would involve removing the bottom cover plate under
the film camera and having a machinist mill a port to accommodate a
leaded glass window (for example, a viewing port from a TEM). A
separate, thin glass plate coated with a phosphor would be placed
above the leaded glass (inside the vacuum). We would use a
peltier-cooled CCD (such as the Q Imaging system), focused on the
phosphor, to capture the image. The camera system has the necessary
software to capture the 2k x 2k image on a PC.

Obviously, this camera would lack all the wonderful features offered
by the TEM camera manufacturers, but I feel that we could build such
a system for $10-12K.

Something must be wrong with this design, since it seems too simple.
So, any comments and/or suggestions would be appreciated.

Thanks.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 19:50:50 2004

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Hi Ritchie,

1. I would have thought that the normal 6-7L LN2 dewar should last around 5
days.

2. Try an organisation called Gresham Scientific Instruments, they do
detector repairs and I was given their name a couple of years ago. I have
no affiliation with them. http://www.gsinst.com/

3. I've used a system involving a brass fitting that fits onto the sample
loading port of a Gatan Dual Ion Mill. This is connected via vacuum hose to
another brass fitting that slides over the evacuation port and seals with an
o-ring. The brass fitting also has a sliding (sealed via an o-ring) pin
with a short thread on the end that can slide upto the bung and screw in.
The bung is then pulled out and the detector evacuated using the TMP on the
Dual Ion mill.
The process is reversed to replace the bung, the hose is then vented and the
brass fitting removed. Hey presto!!...newly evacuated detector.

The problem is that you need to be very careful when putting the bung back
in and unscrewing the pin, to ensure that the bung stays and only the pin is
retracted. Its very difficult to check that all is in order.
But then again you might prefer to leave it all permanently connected up to
the EM vac system, with a suitable isolation valve.

Yes, I admit I blew the window out but it was an old detector that we used
as a spare as our primary was having issues. Nevertheless I was not a happy
camper!!

Hope this helps.

Regards
George

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Wednesday, 28 July 2004 09:00
To: MSA listserver

Dear John and Joel

On the personal note I think that it's very possible to create quite decent
home-made digital camera. Everything depends from the CCD chip. On my 1
Mpix 12-bit (non-peltier) BioScan 600W camera from Gatan chip itself is
about $20K on the market (a little bit outdated data, sorry). It's called
"scientific grade" CCD. So, you actually could not avoid this part of
total cost. From another hand, phosphor screens is used in all
commercially available EM digital cameras. I assume that the quality at
least commercial phosphor screens is quite good (and pricey - about
$5K). So, these two components are most expensive and you could not save
much on it. Perhaps, the design with "optical coupling" (like yours) is
most suitable for amateur EM digital camera. I don't see any principal
problems here. I was thinking about "home-made" camera a few years ago
thinking similarly to you. It appeared to me that the cost of components
would made such project unrealistic. Finally I got Gatan's camera (no
commercial interest, happy user only) at the very (really very) good
price. Talk to Gatan, they are very cooperative and helpful! Before
digital, we used to use about 1000 films per year (not much, I guess). For
the last few years going "digital" we did not spent any film at
all. Nevertheless I am keeping film in the scope and darkroom is
functioning (and technician still have his salary). The thing about
digital cameras: there is not much difference between 1 and 4 M-pix
camera. Because digital cameras are much more sensitive, you may use less
light and shorter exposure time (0.1 sec typically), so your sample is
stable under the beam. You may easily take 4 1 M-pix images and assemble
them into single 4 M-pix montage. You may use automatic functions
incorporated in many EM digital cameras software (like digital montage or
so) to collect images and assemble them into single image. You see my
point: 1 M-pix camera much, much less expensive... If so, you may find
that not so fancy (but functional) commercial EM digital camera may fit
your budget and you would be free from inventing the wheel. Sergey.

At 01:43 PM 7/27/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 20:35:39 2004

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Based on how the cameras look like, it's optically coupled cameras. Modern
cameras usually had direct coupling when camera attached to the phosphor
directly (through fiber-optic plate usually). Direct-coupled cameras
mostly distortion-free. Fiber optics provide better pixel-to-pixel
separation, so images sharper. Not interesting, I am sorry. Sergey

At 01:15 PM 7/27/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Jul 27 21:41:51 2004

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Many thanks for the replies so far.

I should add that I'm happy to be contacted by any 3rd-party service people who feel
confident that they can solve my problem.

cheers

rtch

} From: Ritchie Sims {rsims-at-glgnov2.auckland.ac.nz}
To: MSA listserver {Microscopy-at-MSA.Microscopy.Com}

thanx Valery for these informations...

i have to explain a little my work...

i'm studying a method to make SEM samples conductive, like
polished/sectionned silicium dies, coated in (insulating and
polymerizing) epoxy resin and stuck with some thermo-fusing (at T} 80°C)
glue (insulating too) on an aluminium SEM holder.

My first idea was to mix the resin with metal powder like copper, silver
or graphite powder...but these powders don't work very well when we want
to keep the resin transparent enough to see the die, at 10-20% mixing
rates.
Now i would try the Tin oxyde powder...but i can't preview the result.

We don't need a transparent glue so it's not as difficult as it can be
for the resin.

This study complements the fine metal coatings with Au/Pd or
Pt...because the charging phenomenon is still a little influent on SEM
observation of this kind of prepared samples, in spite of fine metal
sputter coating...

Any suggestions, listers?

Thanx in advance

Sylvain MAURY

Valery Ray a écrit :
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi Sylvain,
}
} The easiest way of measuring high resistivity is to
} use picoammeter and a voltage source to measure
} leakage current flowing through high-resistivity
} sample. I like Keithley 6487 model (no commercial
} interest here), since it combines the picoammeter and
} a voltage source in one unit. See this page:
}
} http://www.keithley.com/servlet/Data?id=4645"} http://www.keithley.com/servlet/Data?id=4645
}
} and also a "Low Level Measurements" book from Keithley
} Instruments (it is a free literature) for the details
} on high resistivity measurement techniques.
}
} On the other note, I am not sure that mixing
} conductive powder with the resin will reduce
} resistivity before impacting the transparency. To
} affect resistivity, conductive particles should be
} close enough so some current will start tunneling
} between them. By that time optical transparency could
} be significantly impacted... .
}
} Does anyone of listers aware of optically transparent
} conductive glue? I'd be very interested to know if it
} exists.
}
} Back to the charging issue, why can't you use a FIB to
} deposit a narrow conductive stripe (C, Pt, W, or Au,
} whatever is available to you) between the die and a
} sample holder? Use low current for deposition close to
} the die to minimize overspray. If distance from the
} sample holder to the die is prohibitive for FIB
} deposition, use some sliver-paint, applied under a
} microscope, to get close to the die first, and then
} FIB deposition to connect the die to a silver paint.
} Thin layer of carbon can also be deposited by imaging
} in oil-contaminated SEM. Other approach to deal with
} charging would be to image a die by ESEM in a water
} vapor atmosphere.
}
} Hope it helps,
}
} Valery Ray
} Particle Beam Systems
} & Technology
} www.partbeamsystech.com
}
} The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America {BR} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver {BR} On-Line
} Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html {BR} ------------------------------------------------------------------------------- {BR} {BR} Hi
} all! {BR} {BR} To solve the charging phenomenon problem
} of HR FESEM observations, in my {BR} application
} (polished cross-sections of Silicium dies samples,
} coated in {BR} epoxy resin, i'm trying to chargea very
} little quantity of resin with a {BR} very little
} quantity of metal powder (copper, silver graphite),
} in {BR} order to keep the resin transparent, just enough
} to evacuate charges. {BR} {BR} Is there a way to measure
} the very high resistivity of this
} charged {BR} resin? {BR} {BR} My goal is to obtain
} resistivities { 10e12 ohm*cm... {BR} {BR} thanx in
} advance {BR} {BR} Sylvain
} MAURY {BR} {BR} {BR} {/BLOCKQUOTE} {/DIV} {/DIV} {/DIV} {/DIV} {/DIV} {/DIV}

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 03:29:55 2004

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Torino 28 July 2004
(ITALY)

Thank you all for your kindly answers.

Just only a few specification:

I have in mind to kill the snail, to dissect it, to extract the interested parts, to fix them with a Bouin solution, ... ,wax inclusion, cutting by microtome, dye and then to perform the histological observations with an optical microscope in transmitted light.

Best Regards,

Massimo

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 05:03:08 2004

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Dear Gordon,

Just a few ideas:
-you could measure the quality of a certain ground point by running a new
thin wire from the 'real' groundpoint (the reference which is chosen for
your system, it should be a star point where all gnds of your system come
together) to the point you want to invesitate and then put an osciloscope
or spectrum analyzer between the new wire and the gnd under test. Just
make sure that the thin wire follows exactly the path of the real ground
wire, otherwise you create a loop which picks up all B-fields. (for safety
you may want to use a battery powered portable scope or a safety
transformer at the input of a normal scope (not sure this is required))

-all ground problems arise from not adhering to the star earth philosophy.
Each device should have its own gnd cable to the reference gnd. This is
very uncommon in electric installations since usualy (like in your home)
it doesn't matter too much and its expensive and creates bulky cable
booms. If for instance a dimmed light is attached to an outlet on the
microscope somewhere it might use the same ground as the microscope and
all the high frequency gnd current created by the lamp will also flow
trough the gnd wire of the microscope creating a voltage due to the
impedance of that wire. For higher frequencies this impedance can be high
and the effect could be a very bad ground. So making an up to date
(usually they are not) schematic and checking for gnds that are connected
in other places than the star point seems like the best but most tedious solution to me.

-a dirty solution would be to decrease the high frequency impedance of the
problematic gnd wire by paralling it with a gnd wire with a lot of strands
(like shielded Litze wire, better in terms of skin effect), making again
sure that it exactly follows the path of the main gnd wire (less critical
as in 1). Replacing
the ground wire with a considderable bigger cross section could also help
for
low frequency problems.

-Most ground problems also create magnetic field problems (and vice
versa, a bad grounding scheme is susceptible to magnetic fields). A handy
and inexpensive way to sniff around for these fields is by constructing a
loop (say diam 10cm) in solid shielded copper wire and soldering it to a
BNC connector
(you could also create a multi loop but single works quite well). Attach
this to a scope or spectrum analyser and 'sniff' around for fields. If
your gnd wires are creating a lot of B-field this also means that they are
carrying a lot of (high freq) current. By studying the frequency pattern
it is sometimes possible to detect where they are coming from (e.g. 50Hz
multiples from dimmers etc, TV monitors have their typical freq.,
switching power supplies of computers have their own freq)

Hopefully this gives some ideas in general to solve those nasty gnd
problems.

kind regards,
Jo

*************************************************************
* Dr. Jo Verbeeck *
* University of Antwerp *
* Dept. EMAT (Electron Microscopy for Materials Research) *
* Groenenborgerlaan 171 *
* B-2020 Antwerpen *
* e-mail: jo.verbeeck-at-ua.ac.be *
* tel: +32(0)3 265 32 49 *
* fax: +32(0)3 265 32 57 *
*************************************************************

On Tue, 27 Jul 2004, Gordon Vrololjak wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
} Hello,
} We may have some grounding problems in the wiring in our building. I was
} wondering if anyone knew of techniques to check the quality of ground, or
} improve its quality? I contacted the electricians here, but they said
} they needed to do more research to figure out how to test the ground.
} Thanks
} Gordon
}
} \/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\
} Gordon Ante Vrdoljak Electron Microscope Lab
} ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
} gvrdolja-at-nature.berkeley.edu UC Berkeley
} phone (510) 642-2085 Berkeley CA 94720-3330
} fax (510) 643-6207 cell (510) 290-6793
}

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 07:27:47 2004

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Jo gave a rather comprehensive reply, but to comment on one point...
Building line power grounds are "safety" grounds only. That is, they are
"ground" from DC to above 60 HZ, but not much above. As frequency
increases, the wavelength of any "noise" becomes shorter. This means that
at higher frequencies, the ground may not be ground at all.

For example, at 100 MHz (3 meter wave):
If a wire is "ground" at one end and is 0.75 (or any odd multiple * 1/4
wave) meters long, the other end is the equivalent of an open circuit.

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Gordon Vrololjak [mailto:gvrdolja-at-nature.Berkeley.EDU]
Sent: Tuesday, July 27, 2004 5:11 PM
To: microscopy-at-msa.microscopy.com

Hello,
We may have some grounding problems in the wiring in our building. I was
wondering if anyone knew of techniques to check the quality of ground, or
improve its quality? I contacted the electricians here, but they said
they needed to do more research to figure out how to test the ground.
Thanks
Gordon

\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/\/
\
Gordon Ante Vrdoljak Electron Microscope
Lab
ICQ 23243541 http://nature.berkeley.edu/~gvrdolja 26 Giannini Hall
gvrdolja-at-nature.berkeley.edu UC Berkeley
phone (510) 642-2085 Berkeley CA 94720-3330
fax (510) 643-6207 cell (510) 290-6793

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 09:21:42 2004

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Listers,

I recently posted a response to this note on TEM cameras referring people to
the SIA ad in the July issue of Microscopy Today.

What I should have done is refer the writer to ALL of the MT advertisers
that sell add-on cameras for TEMs. These include, based on their ads: 4pi
Analysis, Advanced Microscopy Techniques, EVEX, GATAN, and Soft Imaging
Systems. Other advertisers may well sell TEM cameras but did not mention
them in their July ads and there are also a number of advertisers offering
light-optical cameras.

As you might imagine, I have received a number of well-deserved,
appropriate, scoldings. I apologize to all of these fine manufacturers! I
shall have my head examined!

Ron Anderson, Editor
Microscopy Today

-----Original Message-----
} From: John J. Bozzola [mailto:bozzola-at-siu.edu]
Sent: Tuesday, July 27, 2004 12:15 PM
To: Microscopy-at-msa.microscopy.com

Not having $100K to purchase a TEM digital camera system, I am
thinking of making my own. I would like to bounce these design ideas
off of the EM community.

The basic design would involve removing the bottom cover plate under
the film camera and having a machinist mill a port to accommodate a
leaded glass window (for example, a viewing port from a TEM). A
separate, thin glass plate coated with a phosphor would be placed
above the leaded glass (inside the vacuum). We would use a
peltier-cooled CCD (such as the Q Imaging system), focused on the
phosphor, to capture the image. The camera system has the necessary
software to capture the 2k x 2k image on a PC.

Obviously, this camera would lack all the wonderful features offered
by the TEM camera manufacturers, but I feel that we could build such
a system for $10-12K.

Something must be wrong with this design, since it seems too simple.
So, any comments and/or suggestions would be appreciated.

Thanks.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 09:39:18 2004

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Sylvain,

Indium-Tin Oxide powder is transparent, conductive,
and available commercially:

http://www.reade.com/Products/Oxides/indium_tin_oxide.html
(no commercial interest here).

Try mixing nanoparticles grade with your epoxy resin.
Since this powder is inherently transparent, you
should still be able to see the die with quite high
mixing ratios.

Question: How large is your silicium die?

Valery Ray
www.partbeamsystech.com

--- sylvain maury {sylvain.maury-at-thalesgroup.com}
wrote:

}
}
}
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} Microscopy Society of America
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}
} thanx Valery for these informations...
}
} i have to explain a little my work...
}
} i'm studying a method to make SEM samples
} conductive, like
} polished/sectionned silicium dies, coated in
} (insulating and
} polymerizing) epoxy resin and stuck with some
} thermo-fusing (at T} 80°C)
} glue (insulating too) on an aluminium SEM holder.
}
} My first idea was to mix the resin with metal powder
} like copper, silver
} or graphite powder...but these powders don't work
} very well when we want
} to keep the resin transparent enough to see the die,
} at 10-20% mixing
} rates.
} Now i would try the Tin oxyde powder...but i can't
} preview the result.
}
} We don't need a transparent glue so it's not as
} difficult as it can be
} for the resin.
}
} This study complements the fine metal coatings with
} Au/Pd or
} Pt...because the charging phenomenon is still a
} little influent on SEM
} observation of this kind of prepared samples, in
} spite of fine metal
} sputter coating...
}
} Any suggestions, listers?
}
} Thanx in advance
}
} Sylvain MAURY
}
}
}
}
} Valery Ray a écrit :
} }
} }
}
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} Microscopy Society of America
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} } On-Line Help
}
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} }
} } Hi Sylvain,
} }
} } The easiest way of measuring high resistivity is
} to
} } use picoammeter and a voltage source to measure
} } leakage current flowing through high-resistivity
} } sample. I like Keithley 6487 model (no commercial
} } interest here), since it combines the picoammeter
} and
} } a voltage source in one unit. See this page:
} }
} }
}
http://www.keithley.com/servlet/Data?id=4645"} http://www.keithley.com/servlet/Data?id=4645
} }
} } and also a "Low Level Measurements" book from
} Keithley
} } Instruments (it is a free literature) for the
} details
} } on high resistivity measurement techniques.
} }
} } On the other note, I am not sure that mixing
} } conductive powder with the resin will reduce
} } resistivity before impacting the transparency. To
} } affect resistivity, conductive particles should be
} } close enough so some current will start tunneling
} } between them. By that time optical transparency
} could
} } be significantly impacted... .
} }
} } Does anyone of listers aware of optically
} transparent
} } conductive glue? I'd be very interested to know if
} it
} } exists.
} }
} } Back to the charging issue, why can't you use a
} FIB to
} } deposit a narrow conductive stripe (C, Pt, W, or
} Au,
} } whatever is available to you) between the die and
} a
} } sample holder? Use low current for deposition
} close to
} } the die to minimize overspray. If distance from
} the
} } sample holder to the die is prohibitive for FIB
} } deposition, use some sliver-paint, applied under a
} } microscope, to get close to the die first, and
} then
} } FIB deposition to connect the die to a silver
} paint.
} } Thin layer of carbon can also be deposited by
} imaging
} } in oil-contaminated SEM. Other approach to deal
} with
} } charging would be to image a die by ESEM in a
} water
} } vapor atmosphere.
} }
} } Hope it helps,
} }
} } Valery Ray
} } Particle Beam Systems
} } & Technology
} } www.partbeamsystech.com
} }
} } The Microscopy ListServer -- Sponsor: The
} Microscopy
} } Society of America {BR} To Subscribe/Unsubscribe --
} }
}
http://www.msa.microscopy.com/MicroscopyListserver {BR} On-Line
} } Help
} }
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html {BR} ------------------------------------------------------------------------------- {BR} {BR} Hi
} } all! {BR} {BR} To solve the charging phenomenon
} problem
} } of HR FESEM observations, in my {BR} application
} } (polished cross-sections of Silicium dies samples,
} } coated in {BR} epoxy resin, i'm trying to chargea
} very
} } little quantity of resin with a {BR} very little
} } quantity of metal powder (copper, silver
} graphite),
} } in {BR} order to keep the resin transparent, just
} enough
} } to evacuate charges. {BR} {BR} Is there a way to
} measure
} } the very high resistivity of this
} } charged {BR} resin? {BR} {BR} My goal is to obtain
} } resistivities { 10e12 ohm*cm... {BR} {BR} thanx in
} } advance {BR} {BR} Sylvain
} }
}
MAURY {BR} {BR} {BR} {/BLOCKQUOTE} {/DIV} {/DIV} {/DIV} {/DIV} {/DIV} {/DIV}
}
}

=====
Valery Ray

Particle Beam Systems
& Technology
www.partbeamsystech.com

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 10:38:41 2004

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Sergey, I took liberty to address couple of technical issues in point- I trust most subscribers will find it useful. More
information is available at http://www.gatan.com/ , http://www.tvips.com/ , http://www.amtimaging.com/ ,
http://www.soft-imaging.com/ , http://www.sia-cam.com/

} Based on how the cameras look like, it's optically coupled cameras.

Yes, they are.

} Modern
} cameras usually had direct coupling when camera attached to the phosphor
} directly (through fiber-optic plate usually).

Historically, TEM cameras started with fiber optic plate coupling (FOP). Lens coupling is more recent development. First CCD sensors
had too low S/N (signal-to-noise) specifications, demanding every possible photon to be used, not wasted. FOP has 2+ times
efficiency of the lens coupling. CCD sensors specifications improved dramatically over recent years. Of course, efficiency ratio of
both couplings remains the same. Yet lens coupling is working very well with modern sensors- low noise, short exposures.

} Direct-coupled cameras mostly distortion-free.

Decent aspherical lens has distortions less than 1% at the edge of the sensor (which is smaller than the lens maximum possible field
of view- that would make for 1% to 2 %, but is outside of the sensor). Distortion in the center is near zero. I believe that fits
definition "mostly distortion free" as well.

} Fiber optics provide better pixel-to-pixel separation, so images sharper.

This issue is not so straight forward. Fiber optics could do that ideally, if there was a way of attaching every fiber individually
to a single pixel, and fabricate defect free fibers. That would make for MTF = 100%. In addition, it would be nice to have pixels
and fibers as small as possible,
and as many of them, as possible. Such device would have an advantage of both very high spatial resolution (direct readout), and
very high sensitivity (binned readout). But in reality, the array of square pixels is coupled with the array of circles (well,
hexagons), which is how FOP looks like. Doesn't fit very well... The compromise is to use fibers much smaller than the pixels.
Minimum practical diameter of fibers is 6 um at the present time (could be twice less, but number of defects becomes prohibitive). I
am confident that it will be improved in short order, though. And maximum practical size of the pixels (between image resolution and
available sensors) is 24um. By combining these
two, a good compromise is achieved: MTF is elevated enough, and resolution is not reduced too much. Of course, many fibers feed
light to adjacent pixels (fibers which happened to be positioned on pixels borders). Thus, MTF will be much less than ideal 100%,
but
high enough to acquire good image.

Good quality lens does not have such a severe problem - it is capable of much higher MTF than FOP coupling, especially with 24um
pixels, in which case MTF is around 80% to 90%. Because of that, much smaller pixels can be used with the lens coupling, This
provides flexibility described above- high spatial resolution in direct readout mode, and high sensitivity in the binned readout
mode. With 9um pixels good lens delivers MTF about 35% to 60% depending on the size of the filed of view. Of course, lens coupled
camera will require
exposures about twice longer than FOP coupled camera, that uses identical sensor. But, with exposures durations from fractions of a
second to
several seconds, this is perfectly acceptable for many applications.

} Not interesting, I am sorry. Sergey

Between all TEM camera manufacturers which advertise (I counted 6) only one does not make lens coupled cameras. Others 5 do. That
could not be the case if this technology wasn't interesting, wouldn't it?

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
To: {Microscopy-at-microscopy.com}
Sent: Tuesday, July 27, 2004 9:46 PM

Hi Listers,

Our lab my be in the position (in a year or two) to purchase a new SEM.
I'd be
interested in hearing from those who have purchased a new scope in the
last two
years or so - likes dislikes, etc. I'm particularly curious about the
"newer" scope
manufacturers and your experiences with them. If you could provide some
feedback
(offlist) regarding the following items, I'd be grateful:

Brand and Model:
Ballpark purchase price:
Major use (discipline) of instrument:
Yearly service contract cost:
Reliability and performance of instrument:
Quality of service:
Cost of upgrades (i.e. computer acquisition section, if known):

Thanks in advance,

Jim

--

James M. Ehrman
Digital Microscopy Facility
Mount Allison University
Sackville, NB E4L 1G7
CANADA

phone: 506-364-2519
fax: 506-364-2505
email: jehrman-at-mta.ca
www: http://www.mta.ca/dmf

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 12:16:05 2004

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Dear John,
Before you dive too deep into your project, why not have a chat with
Hans Tietz (TVIPS, Munich) who is coming your way soon.
i.e.:
Microscopy & Microanalysis 2004
1-5 August, 2003
Savannah, Georgia, USA
www: www.microscopy.com/MSAMeetings/MM04/MMHomePage.html

He knows a lot about the design and possible pitfalls associated with
TEM digital cameras and should have helpful comments regarding your
proposed design. In the end perhaps, he might manage to sell you one of
his own!
Disclaimer: I have no commercial interest in TVIPS.
Cheers,

Jim

-----Original Message-----
} From: John J. Bozzola [mailto:bozzola-at-siu.edu]
Sent: Tuesday, July 27, 2004 6:15 PM
To: Microscopy-at-msa.microscopy.com

Not having $100K to purchase a TEM digital camera system, I am
thinking of making my own. I would like to bounce these design ideas
off of the EM community.

The basic design would involve removing the bottom cover plate under
the film camera and having a machinist mill a port to accommodate a
leaded glass window (for example, a viewing port from a TEM). A
separate, thin glass plate coated with a phosphor would be placed
above the leaded glass (inside the vacuum). We would use a
peltier-cooled CCD (such as the Q Imaging system), focused on the
phosphor, to capture the image. The camera system has the necessary
software to capture the 2k x 2k image on a PC.

Obviously, this camera would lack all the wonderful features offered
by the TEM camera manufacturers, but I feel that we could build such
a system for $10-12K.

Something must be wrong with this design, since it seems too simple.
So, any comments and/or suggestions would be appreciated.

Thanks.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 12:20:11 2004

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Hello,
does anybody know of the possibility to get the magnification and the
high tension values out of an Zeiss EM 10C and a Philips TEM EM 420 and
to make them available to a PC?
I would like to have these old TEMs interfaced with digital imaging and
need these values for the calibration of the images.

Yours,
Timo

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 12:20:33 2004

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Dear John,

Before you dive too deep into your camera project, why not have a chat
with Hans Tietz (TVIPS, Munich) who is coming your way very soon.
i.e.:
Microscopy & Microanalysis 2004
1-5 August, 2003
Savannah, Georgia, USA

He does know a lot about the design and possible pitfalls associated
with TEM digital cameras and should have helpful comments regarding your
proposed design. In the end, perhaps, he might manage to sell you one of
his own!
Disclaimer: I have no commercial interest in TVIPS.
Cheers,

Jim

-----Original Message-----
} From: John J. Bozzola [mailto:bozzola-at-siu.edu]
Sent: Tuesday, July 27, 2004 6:15 PM
To: Microscopy-at-msa.microscopy.com

Not having $100K to purchase a TEM digital camera system, I am
thinking of making my own. I would like to bounce these design ideas
off of the EM community.

The basic design would involve removing the bottom cover plate under
the film camera and having a machinist mill a port to accommodate a
leaded glass window (for example, a viewing port from a TEM). A
separate, thin glass plate coated with a phosphor would be placed
above the leaded glass (inside the vacuum). We would use a
peltier-cooled CCD (such as the Q Imaging system), focused on the
phosphor, to capture the image. The camera system has the necessary
software to capture the 2k x 2k image on a PC.

Obviously, this camera would lack all the wonderful features offered
by the TEM camera manufacturers, but I feel that we could build such
a system for $10-12K.

Something must be wrong with this design, since it seems too simple.
So, any comments and/or suggestions would be appreciated.

Thanks.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 12:39:22 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,
does anybody know of the possibility to get the magnification and the
high tension values out of an Zeiss EM 10C and a Philips TEM EM 420 and
to make them available to a PC?
I would like to have these old TEMs interfaced with digital imaging and
need these values for the calibration of the images.

Yours,
Timo

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 14:05:44 2004

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Sylvain: one of the tricks I use to ground samples encapsulated in
epoxy is to run a thin line of carbon paint (from somewhere on the
surface you wish to exam but not in the field of view) down the side of
the mount to the bottom of the mount. I also paint most of the exposed
surface epoxy with carbon paint, just leaving a small margin of
unpainted epoxy around my sample. I let this dry, usually in a 50ş C
oven for about 15 minutes. Then I flash the sample with my material of
choice and mount the whole block with carbon tape or carbon paint,
making sure the strip I painted from the top is in contact with this
mounting media. Now there is a conductive path from your sample surface
to the SEM stage. If I'm in a rush mode, I will take the flashed
sample, mount it on a stub, and then run a strip of carbon or copper
tape from the sample surface to the SEM stub. This method is less
elegant and not as efficient, but gets the job done.

I have one question: why are you using insulating glue to mount your
samples?

sylvain maury wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 14:13:08 2004

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On Jul 27, 2004, at 4:00 PM, Ritchie Sims wrote:

} I have an EDS detector, Be window, about 8 years old.

} } From new, its vacuum slowly but inexorably deteriorated, until, after
} } 5 years, it would no
} longer make it through a weekend without a Sunday visit to top up the
} LN2.
}
} So, at great expense (see where I live), I returned it to PGT, where
} it was pumped and
} baked, including leak testing, and returned.
}
} It's been OK, but still has the slow vacuum deterioration, and can
} still maintain its LN2
} through a weekend, but not a long one.
}
} Tolerable for those living on the same landmass as the manufacturer,
} but it's a major
} logistical exercise for me to send it away, and the overall time
} (almost two months last
} time) is a killer.
}
} I am a bit annoyed about this, but
}
} 1
} For how long should an EDS detector maintain its Dewar vacuum so that
} it can go for 3
} days without a topup? Does anyone know if any particular manufacturers
} are better or
} worse than others?
}
} 2
} It seems that the leak must be slower than is detected by PGT's
} testing, so it seems
} unlikely that anyone will be able to find the leak and fix it. Is this
} assumption correct?
} Does anyone know of a 3rd party repairman who might succeed where the
} manufacturer has failed?
}
} 3
} I understand that repumping can, in theory, be done by the user, using
} the SEM's
} vacuum system. Has anyone out there done this in the privacy and
} comfort of their own
} lab, and would they be able to help me figure out whether I have the
} skill and resources
} to do it myself?
}
} Maybe I should just save my pennies to replace it.
}
Dear Ritchie,
We had a Be window EDS detector on the HVEM in Albany for ~20 years,
and the vacuum in the dewar deteriorated in a time frame of ~1 mo. The
LN2 always lasted at least a week, but the resolution would deteriorate
when the vacuum got bad. It sounds like your vacuum leak is much
larger than ours. The detector was a Kevex, and, after pumpout the
resolution always returned to spec (148 eV) or better. I have no
experience with other detectors, so I can't say which is better.
toward the end of my stay in Albany, we had resolution problems and
sent the detector to a non-Kevex service person--I don't remember the
name, and, in any event, he is just as far from you as PGT would be.
We tried him because he was significantly cheaper than Kevex, and after
he baked out the system, the resolution returned to spec. Again, I
can't speak for other service companies, but in this one case, a third
party service was completely satisfactory.
1. With routine pumpout every few months or so our detector always
held LN2 for a week or longer.
2. We could find the occasional leak with a leak detector, and none
of those we found were sufficient to cause LN2 problems, so I'm
surprised that PGT couldn't find yours. I would hook your system up to
a leak detector and see what turns up--assuming you have the equipment.
If you can find someone on your land mass who provides third party
service, give it a try.
3. We installed a permanent branch off the column vacuum to pump our
detector, and we could definitely pump out the detector to the point
that resolution was restored--a much more stringent test than retaining
LN2--so you should be able to do this also. You may, however, have to
have the detector baked out once before you can do this, since there
may have been contaminants introduced through your leak.
Since our detector functioned quite well for 20 years (and still may
be working AFAIK), you shouldn't need to replace it. Of course, since
the newer systems have better functionality in many respects, you might
want to replace it for that reason. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 14:27:47 2004

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On Jul 27, 2004, at 6:36 PM, Sergey Ryazantsev wrote:

} I assume that the quality at least commercial phosphor screens is
} quite good (and pricey - about $5K). So, these two components are
} most expensive and you could not save much on it.

Dear Sergey,
I am not as certain about commercial phosphor screens--especially
since gain correction software can compensate for heterogeneities,
there is no pressure to produce homogeneous screens. At Albany we
poured our own by suspending phosphor, letting the larger grains
settle, then using the smaller grains for the screen. We had a mylar
film stretched and glued to a frame and poured the phosphor on than,
rather than on glass. The camera was lens-coupled, and the phosphor
was on the side of the mylar facing the lens. Fabrication of the frame
and mylar was ~$1000, and after that recoating was very cheap and took
only a few hours of labor, so the cost of the frame could be amortized
over many coatings.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 14:38:46 2004

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Vitaly
We had discussion on digital camera many times on this ListServer in the
past, so I could not add much new in this discussion. I am not good in
theory of digital imaging in EM and do believe there is not much theory
there. When I was shopping for my digital camera I ordered demos from
potential candidates, took pictures of the same sample at the same
conditions and compared them side-by-side. I do find that
optically-coupled cameras even having all advantages you described have
more blurry image than fiber-optic coupling. I don't know why, but this is
just a fact: with my particular sample, at my particular conditions. As a
user, I don't worry much about theory, I need practical results and results
were surprisingly vary in my test. Finally I bought the camera, which
satisfied my particular needs the best and had very good price/quality
ratio. This is a way how I usually shop.

As for MFT business, I would be happy to see what other vendors think about
it. In my particular camera, there are about 10 fibers per pixel
according to Gatan. Because each pixel separated from other, there is less
fiber's overlapping than you could think. I think the very important thing
is what is happening in the gap between sensor (fiber-optic plate) and
phosphor screen. Phosphor has granules which emit light in all
directions. If light from individual granules will overlap, it'll decrease
spatial resolution (and contrast). The ideology of fiber-optic system is
to keep this gap as smaller as possible, so to have less overlapping from
neighbor grains. Ideally you could put phosphor on top of the fiber-optic
plate. I am not quite sure how optical coupling system could handle this
issue. I think, when you are talking about MFT in optically coupled
systems, you are talking mostly about efficiency between lens and sensor,
not counting the specificity of EM - existence of phosphor screen with it's
own MFT if you permit me to call it so. I would think that MFT in optical
systems is quite good between lens and sensor but lens and screen. It
would be nice to discuss this issue with specialists.

As for why optical systems are still manufactured, I think this is because
such systems are much cheaper in production and manufacturer could make
more money from it. This is actually addressed to the original John's
question: why to pay so much money for such simple thing (OK, OK not such
simple). The answer (to me) is because manufacturers overpriced the optical
systems. FOP systems are much more expensive in production (mostly because
of price for the CCD chip), so they are less profitable. Nevertheless, I
think, most top-end systems for EM are FOP now. I would guess that
manufacturers even cover FOB system's production cost selling optical
systems at high price.
Have a good day, Sergey.

At 08:45 AM 7/28/2004, you wrote:
} Sergey, I took liberty to address couple of technical issues in point- I
} trust most subscribers will find it useful. More
} information is available at http://www.gatan.com/ , http://www.tvips.com/
} , http://www.amtimaging.com/ ,
} http://www.soft-imaging.com/ , http://www.sia-cam.com/
}
} } Based on how the cameras look like, it's optically coupled cameras.
}
} Yes, they are.
}
} } Modern
} } cameras usually had direct coupling when camera attached to the phosphor
} } directly (through fiber-optic plate usually).
}
} Historically, TEM cameras started with fiber optic plate coupling (FOP).
} Lens coupling is more recent development. First CCD sensors
} had too low S/N (signal-to-noise) specifications, demanding every possible
} photon to be used, not wasted. FOP has 2+ times
} efficiency of the lens coupling. CCD sensors specifications improved
} dramatically over recent years. Of course, efficiency ratio of
} both couplings remains the same. Yet lens coupling is working very well
} with modern sensors- low noise, short exposures.
}
} } Direct-coupled cameras mostly distortion-free.
}
} Decent aspherical lens has distortions less than 1% at the edge of the
} sensor (which is smaller than the lens maximum possible field
} of view- that would make for 1% to 2 %, but is outside of the sensor).
} Distortion in the center is near zero. I believe that fits
} definition "mostly distortion free" as well.
}
} } Fiber optics provide better pixel-to-pixel separation, so images sharper.
}
} This issue is not so straight forward. Fiber optics could do that ideally,
} if there was a way of attaching every fiber individually
} to a single pixel, and fabricate defect free fibers. That would make for
} MTF = 100%. In addition, it would be nice to have pixels
} and fibers as small as possible,
} and as many of them, as possible. Such device would have an advantage of
} both very high spatial resolution (direct readout), and
} very high sensitivity (binned readout). But in reality, the array of
} square pixels is coupled with the array of circles (well,
} hexagons), which is how FOP looks like. Doesn't fit very well... The
} compromise is to use fibers much smaller than the pixels.
} Minimum practical diameter of fibers is 6 um at the present time (could be
} twice less, but number of defects becomes prohibitive). I
} am confident that it will be improved in short order, though. And maximum
} practical size of the pixels (between image resolution and
} available sensors) is 24um. By combining these
} two, a good compromise is achieved: MTF is elevated enough, and resolution
} is not reduced too much. Of course, many fibers feed
} light to adjacent pixels (fibers which happened to be positioned on pixels
} borders). Thus, MTF will be much less than ideal 100%,
} but
} high enough to acquire good image.
}
} Good quality lens does not have such a severe problem - it is capable of
} much higher MTF than FOP coupling, especially with 24um
} pixels, in which case MTF is around 80% to 90%. Because of that, much
} smaller pixels can be used with the lens coupling, This
} provides flexibility described above- high spatial resolution in direct
} readout mode, and high sensitivity in the binned readout
} mode. With 9um pixels good lens delivers MTF about 35% to 60% depending on
} the size of the filed of view. Of course, lens coupled
} camera will require
} exposures about twice longer than FOP coupled camera, that uses identical
} sensor. But, with exposures durations from fractions of a
} second to
} several seconds, this is perfectly acceptable for many applications.
}
} } Not interesting, I am sorry. Sergey
}
} Between all TEM camera manufacturers which advertise (I counted 6) only
} one does not make lens coupled cameras. Others 5 do. That
} could not be the case if this technology wasn't interesting, wouldn't it?
}
} Vitaly Feingold
} Scientific Instruments and Applications
} 2773 Heath Lane, Duluth GA 30096
} (770)232-7785 ph.
} (770)232-1791 fax
} (678)467-0012 mobile
} www.sia-cam.com
}
} This message is made of 100% recycled electrons.
}
} This address can not receive messages larger than 15 kb without prior
} notification.
}
} ----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
} To: {Microscopy-at-microscopy.com}
} Sent: Tuesday, July 27, 2004 9:46 PM
} Subject: [Microscopy] Re: RE: TEM: home made digital camera question
}
}
} }
} }
} }
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} -------------------------------------------------------------------------------
} }
} } Based on how the cameras look like, it's optically coupled cameras. Modern
} } cameras usually had direct coupling when camera attached to the phosphor
} } directly (through fiber-optic plate usually). Direct-coupled cameras
} } mostly distortion-free. Fiber optics provide better pixel-to-pixel
} } separation, so images sharper. Not interesting, I am sorry. Sergey
} }
} } At 01:15 PM 7/27/2004, you wrote:
} }
} }
} } } -----------------------------------------------------------------------
} -------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } -----------------------------------------------------------------------
} --------
} } }
} } } Have you looked at the cameras sold by SIA, as advertised on pg 69 of the
} } } July Microscopy Today? They are at www.sia-cam.com and 770-232-7785.
} } }
} } } No financial interest other than the fact that SIA advertises in MT.
} } }
} } } Ron Anderson
} } } MT Editor
} } }
} } } -----Original Message-----
} } } } From: John J. Bozzola [mailto:bozzola-at-siu.edu]
} } } Sent: Tuesday, July 27, 2004 12:15 PM
} } } To: Microscopy-at-msa.microscopy.com
} } } Subject: [Microscopy] TEM: home made digital camera question
} } }
} } }
} } }
} } } -----------------------------------------------------------------------
} -----
} } } --
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } -----------------------------------------------------------------------
} -----
} } } ---
} } }
} } } Not having $100K to purchase a TEM digital camera system, I am
} } } thinking of making my own. I would like to bounce these design ideas
} } } off of the EM community.
} } }
} } } The basic design would involve removing the bottom cover plate under
} } } the film camera and having a machinist mill a port to accommodate a
} } } leaded glass window (for example, a viewing port from a TEM). A
} } } separate, thin glass plate coated with a phosphor would be placed
} } } above the leaded glass (inside the vacuum). We would use a
} } } peltier-cooled CCD (such as the Q Imaging system), focused on the
} } } phosphor, to capture the image. The camera system has the necessary
} } } software to capture the 2k x 2k image on a PC.
} } }
} } } Obviously, this camera would lack all the wonderful features offered
} } } by the TEM camera manufacturers, but I feel that we could build such
} } } a system for $10-12K.
} } }
} } } Something must be wrong with this design, since it seems too simple.
} } } So, any comments and/or suggestions would be appreciated.
} } }
} } } Thanks.
} } }
} } } --
} } } ##############################################################
} } } John J. Bozzola, Ph.D., Director
} } } I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
} } } 750 Communications Drive - MC 4402
} } } Southern Illinois University
} } } Carbondale, IL 62901 U.S.A.
} } } Phone: 618-453-3730
} } } Email: bozzola-at-siu.edu
} } } ##############################################################
} }
} } _____________________________________
} }
} } Sergey Ryazantsev Ph. D.
} } Electron Microscopy
} } UCLA School of Medicine
} } Department of Biological Chemistry
} } 10833 Le Conte Ave, Room 33-089
} } Los Angeles, CA 90095
} }
} } Phone: (310) 825-1144 (office)
} } (310) 206-1029 (Lab)
} } FAX (departmental): (310) 206-5272
} } mailto:sryazant-at-ucla.edu
} }
} }
} }
} }

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 15:18:29 2004

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Ron
I hate "political" (toward manufacturers in this context) correctness. You
have your own personal opinion and have rights to express this opinion on
this ListServer as long as you don't have anything to do with SIA
financially. If you really like SIA - why you could not share this
information with us? I think, this is very important to know good and bad
about manufacturers. Moreover, I think, this is a purpose of this forum -
to share useful information in microscopy area. Good or bad experience with
some vendors IS very valuable information. First, it helps us to avoid
mistakes somebody already done (I am too lazy to repeat other's mistakes, I
am sorry). Secondly, such feedback may help vendors to increase the
quality of product/service/etc. It seems to me that this forum drifted
towards pure "correctness". As a result I do notice that people just
afraid to present their own opinion on this forum anymore. I don't feel
it's right if I have to apply strict self-censure on every posting
(honestly, I just don't have time for censure). I think the posting should
be correct "factually" and ethically, that's it. I, also, think
manufacturers are "people" too. They have rights (as an individual, not
representing company's interest) to comment any posting. For instance, I
am quite sure that my postings contain a lot of factual mistakes because
lack of knowledge. I would be very glad if specialist will correct me, so
I'll understand better (and others will not be mistaken by my info). It
seems to me that "poor manufacturers" afraid to say any "word" at this
forum because of strict regulations... Too bad, the purpose of ANY public
forum is to SHARE knowledge and information, not restrict it. This is my
personal opinion.
Sergey

At 07:31 AM 7/28/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 16:18:01 2004

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Postdoctoral position available.

Our research focuses on the structure determination of macromolecular complexes
and their conformational changes by three-dimensional electron microscopy.
Currently one of our main projects is the determination of structure of
complexes in the mitochondrial respiratory chain by cryo-electron microscopy
and image processing. A second topic is the localization of their subunits
within the complexes by immunolabeling. The candidate we are looking for
should have a working knowledge of biochemistry and should carry out antibody
binding experiments, electron microscopy and image processing. To date the
samples are kindly provided by our collaborators; however, if the candidate
shows interest in protein purification some parts of the purification could
be transferred to our laboratory.

Our laboratory is equipped with a Tecnai 12 electron microscope equipped
for cryo-electron microscopy. Computing facilities include a 4-processor HP
alpha computer with several Tb of disk space, and access to an Opteron cluster.

Please send an application including CV to Dr. Michael Radermacher, University
of Vermont, College of Medicine, Dept. Mol. Physiol. and Biophysics,
HSRF Bldg. Rm 120, Burlington VT 05405.
e-mail: mraderma-at-physiology.med.uvm.edu.
Please arrange for three letters of reference to be sent.

The University of Vermont is an equal opportunity employer.

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 16:53:14 2004

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Sergey

I think you have misunderstood.

I don't think Ron intended to express any opinion that favoured SIA over the others, but
it was brought to his attention (by his other advertisers) that his first posting could have
been interpreted as such.

As editor of Microscopy Today, he is in a rather different position than you or me, and
quite properly can't be seen to endorse or denigrate products, even if he does have an
opinion. Which it didn't seem to me that he did have, in this case.

I agree with you about excessive political correctness, I live in a country which suffers a
great deal from it.

But this isn't a case of it.

cheers

rtch

Date sent: Wed, 28 Jul 2004 13:29:28 -0700
To: Microscopy-at-microscopy.com
} From: Sergey Ryazantsev {sryazant-at-ucla.edu}

It sounds like you are trying to image cross sections
of integrated circuits. Depending on the minimum feature
size, this is a routine process using either Buehler
mechanical polishing (} = .35u) or FIB (0.5u or less).
The mechanical polished specimens are mounted on
a 90 degree mount (e.g., Pella #15359) using mounting
wax and a #1 cover slip glass. Then, the edge of the
die is contacted using coloidal silver epoxy and the
sputter coating with Au/Pd or Pt. This works fine
up to 350KX using FESEM and can be done with VPSEM
without coating.

I do not see the point of embedding the specimen in
a large non-conductive mount. Are there other issues
that are not known?

gary g.

At 01:05 AM 7/28/2004, you wrote:

} thanx Valery for these informations...
}
} i have to explain a little my work...
}
} i'm studying a method to make SEM samples conductive, like
} polished/sectionned silicium dies, coated in (insulating and
} polymerizing) epoxy resin and stuck with some thermo-fusing (at T} 80°C)
} glue (insulating too) on an aluminium SEM holder.
}
} My first idea was to mix the resin with metal powder like copper, silver
} or graphite powder...but these powders don't work very well when we want
} to keep the resin transparent enough to see the die, at 10-20% mixing
} rates.
} Now i would try the Tin oxyde powder...but i can't preview the result.
}
} We don't need a transparent glue so it's not as difficult as it can be
} for the resin.
}
} This study complements the fine metal coatings with Au/Pd or
} Pt...because the charging phenomenon is still a little influent on SEM
} observation of this kind of prepared samples, in spite of fine metal
} sputter coating...
}
} Any suggestions, listers?
}
} Thanx in advance
}
} Sylvain MAURY
}

From MicroscopyL-request-at-ns.microscopy.com Wed Jul 28 19:58:23 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Friends,

Ritchie is exactly correct in all regards. I was wrong to make my original
posting the way I did. Can we please end the thread?

Thank you,

Ron

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Wednesday, July 28, 2004 6:07 PM
To: Sergey Ryazantsev; Microscopy-at-microscopy.com

Sergey

I think you have misunderstood.

I don't think Ron intended to express any opinion that favoured SIA over
the others, but
it was brought to his attention (by his other advertisers) that his first
posting could have
been interpreted as such.

As editor of Microscopy Today, he is in a rather different position than you
or me, and
quite properly can't be seen to endorse or denigrate products, even if he
does have an
opinion. Which it didn't seem to me that he did have, in this case.

I agree with you about excessive political correctness, I live in a country
which suffers a
great deal from it.

But this isn't a case of it.

cheers

rtch

Date sent: Wed, 28 Jul 2004 13:29:28 -0700
To: Microscopy-at-microscopy.com
} From: Sergey Ryazantsev {sryazant-at-ucla.edu}

Fellow Listmembers,

We apologize for any inconvenience this may cause, but the location for the
upcoming Cryoultramicrotomy for Materials Science Workshop, originally
scheduled at The University of Southern California in Los Angeles, has been moved to
**The University of California-Irvine.**

The Workshop will be held on the same dates and times as previously posted.

Some of the original attendees can't make it to the new location. There are
five open positions for people who would like to attend. Please see below for
instructions on how to RSVP.

Following is the modified posting with the new venue information:

***********************************************

Our Mini-Workshop Series on "Cryoultramicrotomy for Materials Sciences" is
coming to Irvine, California!

**When**:
Wednesday, August 18 through Thursday, August 19, 2004, 9:00am-4:00pm

**Where**:
University of California - Irvine
Henry Samueli School of Engineering
Dept. of Chemical Engineering & Materials Science
Building 303 (Engineering Tower)
Sixth Floor
Irvine, CA 92697

**Local contact for directions and UCI information.**:
Wen-an Chiou
Director, Materials Characterization Center
Tel. (949) 824-1567
Fax (949) 824-2541
{wchiou-at-uci.edu}

**Parking Notice**: All vehicles on campus require permits! Please see the
UCI Parking Page for details at:
{http://www.parking.uci.edu}

**What**:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair
probes), glass knife making, evaluation of glass knives, care and cleaning of
diamond knives and operation of the cryoultramicrotome.

If you wish to bring specimens, please let us know the nature of your
specimens when you
RSVP and reserve a place in the workshop.

**Background**:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing"at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

**Important Info**:

1. There is no charge for this workshop.

2. Meals and refreshments will be served!

3. Attendance is open to everyone for the presentations and demonstrations
on the first day. However, attendance is limited for the cryoultramicrotomy
hands-on sessions on the second day.

**RSVPs and Reservations**:
To RSVP and to reserve a spot for the hands-on sessions, please contact Kim
Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262).

**Sponsors and Organizers**:
University of California-Irvine
Henry Samueli School of Engineering
Department of Chemical Engineering & Materials Science
Materials Characterization Center
RMC Products Group, Boeckeler Instruments, Inc.

See you in Irvine!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 29 08:33:26 2004

Contents Retrieved from Microscopy Listserver Archives
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Post-doctoral position at Ryerson University

This project involves the development of fundamental, underlying
mechanisms to understand the concepts of self-assembly, as they pertain
to the development of processed foods. Structure development in
processed foods is a complex and multi-stage process that requires
cooperative changes in molecular conformation of key food constituent
(e.g., lipids, proteins, carbohydrates, water, etc.) to facilitate the
coordinated association of individual molecules into arrangements with a
well-defined three-dimensional order. Key techniques used include
atomic force microscopy, Raman confocal microscopy and multiphoton laser
scanning confocal microscopy.

The applicant must be a highly motivated individual with no more than
2-3 years of prior postdoctoral experience who has demonstrated the
ability to organise, execute and interpret complex experiments. A Ph.D.
in food science, physics, chemistry or related fields is desired; as is
a working understanding of atomic force microscopy or related microscopy
technique. Good communication skills and the ability to work effectively
within a multi-disciplinary team are required. The post is available
from September 1st, 2004, initially for a one year period, with a 1-year
extension possible.

For all enquiries, please email Dérick Rousseau (rousseau-at-ryerson.ca).
To apply, please send your application, comprising a full CV and contact
details for at least 2 referees to Dr. Dérick Rousseau, School of
Nutrition, Ryerson University, Toronto, Ontario, Canada, M5B 2K3. Fax
number is 416-979-5204.

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 29 08:52:50 2004

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thanx for all replies, listers...

Embedding the specimen in a non-conductive mount protects it against all
external "agressions" due to operator manipulations, like acidistic
treatments that reveal particular structures of the cross-sections, like
transistors, SiO2 layers.

i must tell that we grind the large epoxy mount until we obtain a tiny
"sandwitch" that looks like this ASCII cross-section :

___________________
{-- the glass plate (thickness ~150µm)
=================== {-- a small layer of epoxy resin (~5-10µm)
- - - - - - - - - - {-- active side (microelectronics)
/ / / / / /
/ / / / / {-- specimen of silicon die (silicon substrate)
(~100-300µm)
/ / / / /
/ / / / /
-------------------
+ + + + + + + + + +
+ + + + + + + + + {-- the rest of the mounting resin charged or not
with metal powder
+ + + + + + + + + +
------------------- thermo-fusing glue that permit to correct the
cross-section
___________________ {-- orientation before and during polishing...that
be replaced by
a
tripod holder

this "sandwitch" is stuck on an 90° aluminium holder with the glue, and
then is mechanically polished until we find the cross-section of
interest.
the very fine resulting layer of epoxy resin, charged with silver powder
(for example) may be enough fine to keep a good transparency in order to
see the sample active surface.
I did some experiments of resistance measurements of this mix today
between 2 disk electrodes of 1cm˛ , with a mixing ratio of 30% in
0.015ml of resin+silver powder : We obtained 5 Mohms ...
of 40% in 0.015ml of resin+silver poxder : 1.6 kOhms...

good results, i think if we are not considering the transparency...

please, be free to give any suggestions...

cheers!

Sylvain MAURY

Gary Gaugler a écrit :
}
} It sounds like you are trying to image cross sections
} of integrated circuits. Depending on the minimum feature
} size, this is a routine process using either Buehler
} mechanical polishing (} = .35u) or FIB (0.5u or less).
} The mechanical polished specimens are mounted on
} a 90 degree mount (e.g., Pella #15359) using mounting
} wax and a #1 cover slip glass. Then, the edge of the
} die is contacted using coloidal silver epoxy and the
} sputter coating with Au/Pd or Pt. This works fine
} up to 350KX using FESEM and can be done with VPSEM
} without coating.
}
} I do not see the point of embedding the specimen in
} a large non-conductive mount. Are there other issues
} that are not known?
}
} gary g.
}
} At 01:05 AM 7/28/2004, you wrote:
}
} } thanx Valery for these informations...
} }
} } i have to explain a little my work...
} }
} } i'm studying a method to make SEM samples conductive, like
} } polished/sectionned silicium dies, coated in (insulating and
} } polymerizing) epoxy resin and stuck with some thermo-fusing (at T} 80°C)
} } glue (insulating too) on an aluminium SEM holder.
} }
} } My first idea was to mix the resin with metal powder like copper, silver
} } or graphite powder...but these powders don't work very well when we want
} } to keep the resin transparent enough to see the die, at 10-20% mixing
} } rates.
} } Now i would try the Tin oxyde powder...but i can't preview the result.
} }
} } We don't need a transparent glue so it's not as difficult as it can be
} } for the resin.
} }
} } This study complements the fine metal coatings with Au/Pd or
} } Pt...because the charging phenomenon is still a little influent on SEM
} } observation of this kind of prepared samples, in spite of fine metal
} } sputter coating...
} }
} } Any suggestions, listers?
} }
} } Thanx in advance
} }
} } Sylvain MAURY
} }

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 29 16:17:29 2004

Contents Retrieved from Microscopy Listserver Archives
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Sylvain,

To avoid others having radically different results if trying to duplicate your
conductive epoxy mix: it's worth pointing out that the silver powder morphology has
a great deal to do with the conductivity than may be achieved. Silver for
conductive pastes can be flake or spherical or something in between. Unless one
knows which to use, the results may have as much to do with the type as the
proportions of silver to resin. One can always buy a commercial silver-filled
epoxy and have predictability.

John Twilley

sylvain maury wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} thanx for all replies, listers...
}
} Embedding the specimen in a non-conductive mount protects it against all
} external "agressions" due to operator manipulations, like acidistic
} treatments that reveal particular structures of the cross-sections, like
} transistors, SiO2 layers.
}
} i must tell that we grind the large epoxy mount until we obtain a tiny
} "sandwitch" that looks like this ASCII cross-section :
}
} ___________________
} {-- the glass plate (thickness ~150µm)
} =================== {-- a small layer of epoxy resin (~5-10µm)
} - - - - - - - - - - {-- active side (microelectronics)
} / / / / / /
} / / / / / {-- specimen of silicon die (silicon substrate)
} (~100-300µm)
} / / / / /
} / / / / /
} -------------------
} + + + + + + + + + +
} + + + + + + + + + {-- the rest of the mounting resin charged or not
} with metal powder
} + + + + + + + + + +
} ------------------- thermo-fusing glue that permit to correct the
} cross-section
} ___________________ {-- orientation before and during polishing...that
} be replaced by
} a
} tripod holder
}
}
} this "sandwitch" is stuck on an 90° aluminium holder with the glue, and
} then is mechanically polished until we find the cross-section of
} interest.
} the very fine resulting layer of epoxy resin, charged with silver powder
} (for example) may be enough fine to keep a good transparency in order to
} see the sample active surface.
} I did some experiments of resistance measurements of this mix today
} between 2 disk electrodes of 1cm˛ , with a mixing ratio of 30% in
} 0.015ml of resin+silver powder : We obtained 5 Mohms ...
} of 40% in 0.015ml of resin+silver poxder : 1.6 kOhms...
}
} good results, i think if we are not considering the transparency...
}
} please, be free to give any suggestions...
}
} cheers!
}
} Sylvain MAURY
}
} Gary Gaugler a écrit :
} }
} } It sounds like you are trying to image cross sections
} } of integrated circuits. Depending on the minimum feature
} } size, this is a routine process using either Buehler
} } mechanical polishing (} = .35u) or FIB (0.5u or less).
} } The mechanical polished specimens are mounted on
} } a 90 degree mount (e.g., Pella #15359) using mounting
} } wax and a #1 cover slip glass. Then, the edge of the
} } die is contacted using coloidal silver epoxy and the
} } sputter coating with Au/Pd or Pt. This works fine
} } up to 350KX using FESEM and can be done with VPSEM
} } without coating.
} }
} } I do not see the point of embedding the specimen in
} } a large non-conductive mount. Are there other issues
} } that are not known?
} }
} } gary g.
} }
} } At 01:05 AM 7/28/2004, you wrote:
} }
} } } thanx Valery for these informations...
} } }
} } } i have to explain a little my work...
} } }
} } } i'm studying a method to make SEM samples conductive, like
} } } polished/sectionned silicium dies, coated in (insulating and
} } } polymerizing) epoxy resin and stuck with some thermo-fusing (at T} 80°C)
} } } glue (insulating too) on an aluminium SEM holder.
} } }
} } } My first idea was to mix the resin with metal powder like copper, silver
} } } or graphite powder...but these powders don't work very well when we want
} } } to keep the resin transparent enough to see the die, at 10-20% mixing
} } } rates.
} } } Now i would try the Tin oxyde powder...but i can't preview the result.
} } }
} } } We don't need a transparent glue so it's not as difficult as it can be
} } } for the resin.
} } }
} } } This study complements the fine metal coatings with Au/Pd or
} } } Pt...because the charging phenomenon is still a little influent on SEM
} } } observation of this kind of prepared samples, in spite of fine metal
} } } sputter coating...
} } }
} } } Any suggestions, listers?
} } }
} } } Thanx in advance
} } }
} } } Sylvain MAURY
} } }

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 29 16:33:13 2004

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Hi Sylvain,

I believe you are making your sample prep more complex than necessary. I
have, for years, mounted the bare IC chip to my 90 deg. cross sectioning
block with mounting wax. I then grind/polish the cross section, with full
top view of the circuitry to see my site of interest approach the plane of
the section. I have used various wet and dry chemistries to "stain", or
delineate, structures of the transistors and wiring. The only time I have
attached a cover glass to the top surface, is when I had delamination
problems during the grind/polish operation. That usually only happens when
there are very large metal bus lines in the section plane. The exposure to
the chemistry is so short, that there is no "collateral damage" to my
sample. For SEM inspection, I carefully apply some carbon paint to the
outside corners of the polished section, away from the site of interest,
and down to the stub. That provides a path for the charge from the
circuitry, across the mounting wax, to the stub, and then the SEM stage.
Most of my imaging is done at low accelerating voltages these days, but if
needed, I will then apply a carbon, or metal, coating for further charge
control. I have often imaged without the carbon paint or coating, when I
did not need super fine detail.

Good Luck,
Darrell

sylvain maury {sylvain.maury-at-thalesgroup.com} wrote on 07/29/2004 10:02:11
AM:

}
}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.
} com/MicroscopyListserver
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}
} thanx for all replies, listers...
}
} Embedding the specimen in a non-conductive mount protects it against all
} external "agressions" due to operator manipulations, like acidistic
} treatments that reveal particular structures of the cross-sections, like
} transistors, SiO2 layers.
}
} i must tell that we grind the large epoxy mount until we obtain a tiny
} "sandwitch" that looks like this ASCII cross-section :
}
} ___________________
} {-- the glass plate (thickness ~150µm)
} =================== {-- a small layer of epoxy resin (~5-10µm)
} - - - - - - - - - - {-- active side (microelectronics)
} / / / / / /
} / / / / / {-- specimen of silicon die (silicon substrate)
} (~100-300µm)
} / / / / /
} / / / / /
} -------------------
} + + + + + + + + + +
} + + + + + + + + + {-- the rest of the mounting resin charged or not
} with metal powder
} + + + + + + + + + +
} ------------------- thermo-fusing glue that permit to correct the
} cross-section
} ___________________ {-- orientation before and during polishing...that
} be replaced by
} a
} tripod holder
}
}
} this "sandwitch" is stuck on an 90° aluminium holder with the glue, and
} then is mechanically polished until we find the cross-section of
} interest.
} the very fine resulting layer of epoxy resin, charged with silver powder
} (for example) may be enough fine to keep a good transparency in order to
} see the sample active surface.
} I did some experiments of resistance measurements of this mix today
} between 2 disk electrodes of 1cm˛ , with a mixing ratio of 30% in
} 0.015ml of resin+silver powder : We obtained 5 Mohms ...
} of 40% in 0.015ml of resin+silver poxder : 1.6 kOhms...
}
} good results, i think if we are not considering the transparency...
}
} please, be free to give any suggestions...
}
} cheers!
}
} Sylvain MAURY
}
}
} Gary Gaugler a écrit :
} }
} } It sounds like you are trying to image cross sections
} } of integrated circuits. Depending on the minimum feature
} } size, this is a routine process using either Buehler
} } mechanical polishing (} = .35u) or FIB (0.5u or less).
} } The mechanical polished specimens are mounted on
} } a 90 degree mount (e.g., Pella #15359) using mounting
} } wax and a #1 cover slip glass. Then, the edge of the
} } die is contacted using coloidal silver epoxy and the
} } sputter coating with Au/Pd or Pt. This works fine
} } up to 350KX using FESEM and can be done with VPSEM
} } without coating.
} }
} } I do not see the point of embedding the specimen in
} } a large non-conductive mount. Are there other issues
} } that are not known?
} }
} } gary g.
} }
} } At 01:05 AM 7/28/2004, you wrote:
} }
} } } thanx Valery for these informations...
} } }
} } } i have to explain a little my work...
} } }
} } } i'm studying a method to make SEM samples conductive, like
} } } polished/sectionned silicium dies, coated in (insulating and
} } } polymerizing) epoxy resin and stuck with some thermo-fusing (at T} 80°
C)
} } } glue (insulating too) on an aluminium SEM holder.
} } }
} } } My first idea was to mix the resin with metal powder like copper,
silver
} } } or graphite powder...but these powders don't work very well when we
want
} } } to keep the resin transparent enough to see the die, at 10-20% mixing
} } } rates.
} } } Now i would try the Tin oxyde powder...but i can't preview the result.
} } }
} } } We don't need a transparent glue so it's not as difficult as it can be
} } } for the resin.
} } }
} } } This study complements the fine metal coatings with Au/Pd or
} } } Pt...because the charging phenomenon is still a little influent on SEM
} } } observation of this kind of prepared samples, in spite of fine metal
} } } sputter coating...
} } }
} } } Any suggestions, listers?
} } }
} } } Thanx in advance
} } }
} } } Sylvain MAURY
} } }
}

From MicroscopyL-request-at-ns.microscopy.com Thu Jul 29 19:24:44 2004

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Hi all - we run this course every year or so, most participants are from
within Australia, but anyone from further afield would be very welcome.
cheers
Sally

The Australian National University Electron Microscopy Unit and Anaspec
Australia are offering two SEM Courses with Steve Chapman(Protrain):

Course 1
Monday 13th September until Wednesday 15th September 2004
A Basic Introduction to Scanning Electron Microscopy (3 days)

The course is based firmly upon the practical side of the instrument, with
theory introduced as and when it is required.

Cost AUS$300.00 plus GST

Course 2

Advanced Techniques in Scanning Electron Microscopy (2 days)
Thursday 16th September until Friday 17th September 2004

For scientists who need an introduction to high resolution SEM and energy
dispersive x-ray analysis or who have some experience but need to brush up
their skills. This is not a course for the SEM novice, however the Basic
SEM course should prepare the less experienced. Students are invited to
bring along one of their own problem specimens for investigation.

Cost AUS $200.00 plus GST

Or both Courses (5 days)

Monday 13th September until Friday 17th September 2004

Cost AUS$450.00 plus GST

Accommodation and meals are NOT included

For further information please contact

Ruth Grinan
Anaspec cc Australia
ruth-at-anaspec.co.za
Mob: 0438632470

or

Dr Sally Stowe
ANU EMU
Australian National University
sally.stowe-at-anu.edu.au

From MicroscopyL-request-at-ns.microscopy.com Fri Jul 30 11:53:40 2004

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University of Connecticut
Institute of Materials Science

Postdoctoral Position
SPM manipulation of carbon nanotubes and biological systems

A post-doctoral position is available immediately within the Institute
of Materials Science at UConn to work on SPM imaging, manipulation, and
lithography of carbon nanotubes and biological systems. The ideal
candidate will have experience with AFM measurements in liquid, SPM
lithography, and or SPM technique development. Experiments will be
conducted in the newly constructed NanoMeasurement labs, featuring two
new AFM systems for in vitro and air measurements with simultaneous
confocal microscopy, as well as a UHV AFM/STM.

This position is a one-year appointment, with funding available for
further years. To apply, please send a complete resume, together with a
list of publications and contact details for 3 references, to Prof.
Bryan Huey (bhuey-at-ims.uconn.edu). Screening of applications will begin
immediately, and will continue until the position is filled.
Applications are encouraged from under-represented groups, including
minorities, women, and people with disabilities.

Bryan D. Huey
The Institute of Materials Science
University of Connecticut
97 N. Eagleville Road, unit 3136
Storrs, CT 06269 USA
office: (860) 486 3284
fax: (860) 486 4745
http://www.ims.uconn.edu/
bhuey-at-uconn.edu

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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Name: Juan

Title-Subject: [Microscopy] [Filtered] Export EDX spectrum

Question:
Hi,

I took some EDX spectrum by using EDAX Phoenix 1998 Revision 3.1, but
I can not export the spectrum into a data file. Does anybody know
the method? Any suggestion would be highly appreciated.

Juan

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Name: daniele gazzola

Organization: Biomed dept. -at-Brown Univ., Providence, RI, USA -
Engineering dept. -at-Genova University, Italy

Title-Subject: [Microscopy] [Filtered] hybrid AFM-optical microscope

Question: I am trying to set up a hybrid microscope in order to use
AFM (atomic force microscope) along with light microscopy(phase) on
unstained biological samples.

The AFM that I am using adds two lenses to the optical path just
above the sample. Unfortunately I neither know the specifications of
those lenses, nor the characteristics of the other optical elements.
I know that the plane of the sample is conjugated to a plane 32mm
above the top lens. The whole AFM is practically a tube about 10cm
long and 1cm of diameter.

I am trying to get informations about the optical elements of a long
working distance condenser. Can anyone please send me a diagram?

I think that the AFM will add one conjugate focal plane to the
system. Do you think that this will be a problem?
What about using reflected light (for brightfield, phase, or DIC)?

I would like any comment or idea about this.
thanks a lot,
daniele

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Name: Frida Maiers

Organization: Hennepin County Medical Center

Title-Subject: [Microscopy] [Filtered] MListserver: TEM photographic supplies available

Question: Due to digital camera installation we have the following
available for a nominal fee: 1 case of D19 developer, 11 boxes of EM
film (Kodak 4489, new formulation), 15 liquid kits of Kodak fixer,
and 17 boxes Kodak Polymax II RC photographic paper (100 sheets
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on Sunday, August 1, 2004 at 14:15:07
---------------------------------------------------------------------------

Email: Gsalaj7-at-aol.com
Name: Sally Thomas Graziano

Organization: Orlando Science Center

Education: Undergraduate College

Location: Orlando Florida

Question: In my work on the SEM here at OSC. Along with our
educational programs we have an ongoing research project. In that
regard I have a very small eye cyst from a swan which I need to look
at. As you can see most of my specimens are larger biological
specimens. How should I mount it on the SEM stub. I use carbon tape
for most things but am afraid the cyst will get lost in one of the
bubbles of the tape.Also how long to coat. Any sugestions would be
most helpful. Sally Graziano

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Juan,

You wrote:

} I took some EDX spectrum by using EDAX Phoenix 1998 Revision 3.1, but I
} can not export the spectrum into a data file. Does anybody know the method?
} Any suggestion would be highly appreciated.
}
EDAX have a free spectrum viewer that can be downloaded from:
http://www.edax.com/support/EDS_Spectrum_Viewer.html

You can cut and paste the channel data from this programmme.

Alternatively, I have written an application which will display EDAX .spc
files - as well as Noran, Link/Oxford and EMSA file formats - which allows
export of data as well. Let me know if you want a copy.

David Vowles
Electron Microscope Unit
Dept of Materials Science and Metallurgy
University of Cambridge
Pembroke St Cambridge
UK CB2 3QZ
Tel: +44 (0)1223 334325
Fax: +44 (0)1223 334567
Email: djv23-at-cam.ac.uk

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Hey Listers,

We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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Hi

Can someone point me in the direction of online information regarding
techniques for the identification of asbestos by SEM and by other
techniques?

thanks

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599
ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

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Let us know if you find something that is suitable and *inexpensive*.
Microscopy supply vendors sell plastic boxes, but at the rate I go through
samples, I would go broke and run out of storage room as well.

No inexpensive vials, jars, etc. that I have found protect the prepared
surface well - no mounting method. The best compromise is to use a snugly
fitting "Cap Plug" (poly closure used to close pipe ends, other holes) and
partially insert the mount into it.

If nothing else fits, I stuff the large mounts into a locking closure
plastic bag. It is likely that if fragile or coated, this will harm the
specimen, however.

A great solution (not my idea) for 1/2" (12mm) pin-mounts is an "Opticlear"
25 dram glass vial with a closed bottom poly cap. Punch or cut a snug hole
in the bottom (inside) of the cap, shove the stub pin in and place in
vial...

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Giles, Bill [mailto:William.Giles-at-TIMET.com]
Sent: Monday, August 02, 2004 1:39 PM
To: 'Microscopy-at-microscopy.com'

Hey Listers,

We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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Bill:

We have some containers that are ideal for this application. You can
see an image of them on our website at www.southbaytech.com. Do a
keyword search for "containers". You will also find them listed with
our extensive range of metallographic consumables under the
"consumables" button. I will contact you off-line with pricing.

Best regards-

David

Giles, Bill wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
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South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

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Toll-free in the USA: +1-800-728-2233
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Hello Microscopy folks,
I am trying to resurrect an old spectroscopy system that uses a Tracor
Northern TN-6500 box for controlling a linear diode readout. Anyone out
there with a manual for the TN-6500? I am happy to pay photocopy charges
or do anything (reasonable!) to get my hands on one. Thanks again.
Greg Mulhollan
-----------------------------------
Gregory Mulhollan, Ph.D.
Saxet Surface Science
1001 S. Sunset Canyon Drive
Dripping Springs, TX 78620
(512)858-2841 office
(512)694-4879 cell
mulhollan-at-saxetsurfacescience.com
www.saxetsurfacescience.com

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

William Giles wrote:
============================================================================
==============
We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?
============================================================================
==============
SPI Supplies has manufactured for some years our special mount storage box
for 1" mounts, see URL
http://www.2spi.com/cataelog/boxes/speci_box.shtml

This would be our SPI #02020-AB and each one holds eight mounts. There are
inserts for desiccating capsules. And once the samples are loaded into the
box, and the lid closed, some ordinary Scotch Tape is put around the lip of
the closed box to seal out air or anything else that might seep in and
damage samples.

Disclaimer: SPI Supplies is the manufacturer of this special kind of
storage box.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

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Thanks for all the responses; I'll filter thru all the suggestions.

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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We use the "Cap Plugs" Woody has suggested and I find they work well if
you're looking for inexpensive (a few cents per piece) individual sample
storage.

The caps come in a variety of shapes and sizes, and I'm sure there are
many sources for such items. The vendor we ordered from has a good page
with drawings and dimensions for each:
http://www.niagaracapsandplugs.com/nonthreaded_caps.htm

Regards,

Steven T Szewczyk
Materials Science Contractor
US Army Research Lab
Aberdeen Proving Ground, MD

-----Original Message-----
} From: White, Woody N. [mailto:nwwhite-at-bwxt.com]
Sent: Monday, August 02, 2004 4:08 PM
To: 'Giles, Bill'; 'Microscopy-at-microscopy.com'

Let us know if you find something that is suitable and *inexpensive*.
Microscopy supply vendors sell plastic boxes, but at the rate I go
through samples, I would go broke and run out of storage room as well.

No inexpensive vials, jars, etc. that I have found protect the prepared
surface well - no mounting method. The best compromise is to use a
snugly fitting "Cap Plug" (poly closure used to close pipe ends, other
holes) and partially insert the mount into it.

If nothing else fits, I stuff the large mounts into a locking closure
plastic bag. It is likely that if fragile or coated, this will harm the
specimen, however.

A great solution (not my idea) for 1/2" (12mm) pin-mounts is an
"Opticlear" 25 dram glass vial with a closed bottom poly cap. Punch or
cut a snug hole in the bottom (inside) of the cap, shove the stub pin in
and place in vial...

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Giles, Bill [mailto:William.Giles-at-TIMET.com]
Sent: Monday, August 02, 2004 1:39 PM
To: 'Microscopy-at-microscopy.com'

Hey Listers,

We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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Hello Microscopists !

Quite some time ago, in anticipation of a congenial meeting of interested
parties at a common-ground investigation of several broken steel bolts in
the Cleveland, Ohio, area, I asked about suitable SEM labs in the area.
I received an excellent response from The List, which indicates that it is
the primary means of rapid and effective communication in the micrsocopy
community. Alas, there was a slower response from the above-referenced
interested parties, and so no agreement about protocol or venue was
reached until we had all retired to our own offices. Later on, we wound up
going back to the place selected originally by one of the parties way back
at the beginning of the project, where 1000X is about the limit of useful
magnification. I am sure any one of you could have done better.

Thanks to all who reponded.

Best regards,
George Langford, Sc.D.
Principal Consultant
Amenex Associates, Inc.
amenex-at-amenex.com
http://www.amenex.com/

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Mr. Chapman,
When you say "stock ammonia solution", are you talking about standard
Ammonia(NH3)?

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Email: cnorton-at-wis-inc.net
Name: chris norton

Organization: Wafer Inspection Services, Inc.

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: We are searching for service engineers with KLA-Tencor
service and applications experience on all models.
Prometrix UV1250/1280; RS 75; 6420; AIT; Starlight; 8100 CD SEMS; etc.

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (garyeaston-at-scannerscorp.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, August 3, 2004 at 13:34:53
---------------------------------------------------------------------------

Email: garyeaston-at-scannerscorp.com
Name: Gary M. Easton

Organization: Scanners Corporation

Title-Subject: [Microscopy] [Filtered] Cambridge/Leica/LEO S360 SEM

Question: I just picked up a used Cambridge S360 that gives me an
error code 307(defective LAB6 switch). Does anyone out there that
has a complete list of the software error codes and their
explanation? The operator's manual offers no help. Also, if anyone
has the setup software (mag cal,
etc) for this series SEM and is willing to part with a copy, it would
be greatly appreciated. Please reply offline to
garyeaston-at-scannerscorp.com. Thanks in advance.

Gary M. Easton

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Hi all
I am looking at Leica ultra-microtomes. The new version (the UC6b) has
two controllers, the key pad or the touch screen. I would appreciate
any input or comments on these. I am especially interested in reasons
to get one or the other.
Thanx
David

_____________________

David Elliott Ph.D.
Research Assistant Professor
Department of Cell Biology and Anatomy
PO Box 245004
Tucson, AZ 85724

Voice: 520-626-7870
Fax: 520-626-2097

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Hi all, I am co-chair of a workshop being given on algae identification at
the North American Lakes Management Society International Symposium in
Victoria Canada. The workshop is being offered November 2,
2004. Normally, its not a problem to get the scopes, but I can't find a
source in Canada. I need 10 teaching scopes with Phase and 400 objectives
and 1 BX60 with Phase at 200 and 400 with a trinoc head and a digital
camera. Can anyone help? I'm located in Michigan, United States. Thanks
much, Ann.

Ann St. Amand, Ph.D.
President
PhycoTech, Inc.
620 Broad St., Suite 100
St. Joseph, Michigan 49085 USA

269-983-3654 (voice)
269-983-3653 (fax)
mailto:astamand-at-phycotech.com
www.phycotech.com

Specializing in Aquatic Sample Analysis and Microscope Accessories

Director, Region V, North American Lake Management Society, www.nalms.org

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Hi David
Keypad does not have all features, touch screen has. It's quite
confusing. For instance if you go with touch pad, you need to buy $5K
interface (whichever it called) for their new cryo-attachment and so on. As
far as I understand, touch-screen is sort of "standard" and they "invented"
key-pad to make cheaper version of the ultratome. You need to check the
compatibility issue, because UC6 is not compatible with previous generation
stuff, like UCT, FSC etc. Good luck with shopping. Sergey

At 08:09 AM 8/4/2004, you wrote:

} ------------------------------------------------------------------------------
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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (matthew.salanga-at-childrens.harvard.edu) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html#form
on Wednesday, August 4, 2004 at 15:15:22
---------------------------------------------------------------------------

Email: matthew.salanga-at-childrens.harvard.edu
Name: Matthew Salanga

Organization: Children's Hospital Boston

Education: Graduate College

Location: Boston, MA

Question: Greetings!

Does anybody know where I can obtain CFP-YFP FRET control slides. Or
transfected a stable FRET positive cell line. Ideally I am looking
for cells grown on coverslips which have tagged CFP and YFP proteins
that are known to elicit a FRET response.

Thanks!

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (sspence-at-flemingc.on.ca) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Wednesday, August 4, 2004 at 19:41:48
---------------------------------------------------------------------------

Email: sspence-at-flemingc.on.ca
Name: Susan Spence

Organization: Tottenham Public School

Education: 6-8th Grade Middle School

Location: Tottenham, Ontario Canada

Question: I have a very ruly group of grade 8's, very few
microscopes, and even fewer quality slides from which to view
organelles and unicellular organisms. DO you have any suggestions as
to where I may find good images, either from a light microscope or an
electron microscope? I want to show them what cells really look like
through a microscope without actually having them to touch one.
Thanks for your suggestions!

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The Leica ultra-microtome ....?!
This brings back memories of the original one, based on the design by
Humberto Fernandez-Moran about 50 years ago. Anyone still remember it?
Its design was absolutely unique in that the specimen chuck was mounted
in a motor-driven massive cylinder which performed complete rotations in
the horizontal plane over two pairs of huge flat sapphire bearings
placed in a "V" orientation. I imagine that it must have been a "cow of
a thing" to set up! It was possibly developed to utilize the newly
invented diamond knives (also invented by F-M, whose genius contributed
so much to new developments in the early days of TEM). I only ever saw
advertising brochures of the ultra-microtome, so would be interested to
learn of users' experiences from those times and perhaps also something
about the fate of these now-historic instruments.

-----Original Message-----
} From: David Elliott [mailto:David.Elliott-at-yale.edu]
Sent: Wednesday, August 04, 2004 5:09 PM
To: Microscopy ListServer

Hi all
I am looking at Leica ultra-microtomes. The new version (the UC6b) has
two controllers, the key pad or the touch screen. I would appreciate
any input or comments on these. I am especially interested in reasons
to get one or the other.
Thanx
David

_____________________

David Elliott Ph.D.
Research Assistant Professor
Department of Cell Biology and Anatomy
PO Box 245004
Tucson, AZ 85724

Voice: 520-626-7870
Fax: 520-626-2097

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I do remember setting up something like that. Except my recollection
is that it was designed by Sjostrand. The cylindrical chuck unit had
a groove around it so that you would mount the motor on the wall, and
run a long V-belt from the motor to the microtome. This was to
minimize vibration. The other feature that I remember is that the
cutting speed was quite fast, not at all like what we use today.

Joel

I am using a Reichart-Jung MT 6000 ultramicrotome for standard EM
sectioning. After the specimen goes through the cutting range there is a
beep and the microtome electronics will freeze up, I have tried reseting the
knife and specimen advancements but the problem still persists, does anyone
have a recommendation?

Thanks,

Todd Hamm
Research Technician
Oklahoma Medical Research Foundation
tmhamm09-at-yahoo.com

_________________________________________________________________
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On my search for the possibility to get high tension and magnification
values out of older Philips and Zeiss TEMs I got no answer from the group
and finally found after an extensive search of the web the following
interface-cards for these TEMs:

For Philips EM 400, 410, 420: http://www.stefan-diller.com/rem_tem3_en.htm
For Zeiss TEMs EM 10 A, B and C: http://www.stefan-diller.com/rem_tem4_en.htm

I hope this is useful for somebody having the same problems with wrong
mag-values and doing new reference images after changing the HT-value on an
old TEM...

--
Timo Junker Holografie
Lindenstr. 10
97297 Waldbźttelbrunn
Tel: ++49 (0)931 4520655
Fax: ++49 (0)931 4520657
www.holografie.com

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Dear Joel,

Thanks for your comments. The ultra-microtome as such was of course invented by Fritiof Sjostrand and I agree that his first models had a remote motor, just as you describe. I did not realize that his design also originally had 360ˇ rotation of the specimen chuck holder. As far as I know his design was developed in conjunction with LKB-Produkter, Bromma Sweden whereas the slightly later Fernandez-Moran instrument was developed with Ernst Leitz, Wetzlar Germany. I seem to recollect that an example of the F-M instrument found its way to Dunedin, New Zealand, but there must have been others too.
Perhaps others might be interested in taking the story further from here....
Cheers,

Jim

-----Original Message-----
} From: Joel Sheffield [mailto:jbs-at-temple.edu]
Sent: Thursday, August 05, 2004 3:05 PM
To: James Chalcroft; Microscopy ListServer

Dear Jim,

I saw the Sjostrand microtome when I taught a course at Rutgers,
Camden, in the 1970's. We actually got it set up and running. They
also had a (barely) working RCA EMU-2 scope. I doubt if they have
kept either.

The other thread in this history, of course, was the system developed
by Keith Porter. In the original models of what eventually became
the Porter-Blum microtome, the block followed the famous
parallelogram path, but advance was thermal. We had a goosneck lab
light mounted over the rod that held the specimen, and you sat there
flashing the light with each pass of the block. If you were good,
you could get beautiful ribbons of silver --but woe betide anyone who
walked past you while you were sectioning!

Later on, Keith developed the offset gimble mechanical advance that
led to the Sorval series of MT microtomes.

The other interesting approach to microtomy was that of Huxley, who
used flexible springs for all of the hinge points, to replace
bearings and reduce vibration. This machine was originally made by
Cambridge, and later distributed by LKB.

} Dear Joel,
}
} Thanks for your comments. The ultra-microtome as such was of course
} invented by Fritiof Sjostrand and I agree that his first models had a
} remote motor, just as you describe. I did not realize that his design
} also originally had 360ˇ rotation of the specimen chuck holder. As far
} as I know his design was developed in conjunction with LKB-Produkter,
} Bromma Sweden whereas the slightly later Fernandez-Moran instrument
} was developed with Ernst Leitz, Wetzlar Germany. I seem to recollect
} that an example of the F-M instrument found its way to Dunedin, New
} Zealand, but there must have been others too. Perhaps others might be
} interested in taking the story further from here.... Cheers,
}
} Jim
}
} -----Original Message-----
} From: Joel Sheffield [mailto:jbs-at-temple.edu]
} Sent: Thursday, August 05, 2004 3:05 PM
} To: James Chalcroft; Microscopy ListServer
} Subject: [Microscopy] Re: RE: Leica ultra-microtome (History)
}
} I do remember setting up something like that. Except my recollection
} is that it was designed by Sjostrand. The cylindrical chuck unit had
} a groove around it so that you would mount the motor on the wall, and
} run a long V-belt from the motor to the microtome. This was to
} minimize vibration. The other feature that I remember is that the
} cutting speed was quite fast, not at all like what we use today.
}
} Joel
}
}
} Subject: [Microscopy] RE: Leica ultra-microtome (History)
} Date sent: Thu, 5 Aug 2004 10:08:02 +0200 From:
} "James Chalcroft" {jchalcro-at-neuro.mpg.de} To: "David
} Elliott" {David.Elliott-at-yale.edu} Copies to: "Microscopy
} ListServer" {Microscopy-at-MSA.Microscopy.Com}
}
} }
} }
} } --------------------------------------------------------------------
} } -- -------- The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------
} } -- ---------
} }
} } The Leica ultra-microtome ....?!
} } This brings back memories of the original one, based on the design
} } by Humberto Fernandez-Moran about 50 years ago. Anyone still
} } remember it? Its design was absolutely unique in that the specimen
} } chuck was mounted in a motor-driven massive cylinder which performed
} } complete rotations in the horizontal plane over two pairs of huge
} } flat sapphire bearings placed in a "V" orientation. I imagine that
} } it must have been a "cow of a thing" to set up! It was possibly
} } developed to utilize the newly invented diamond knives (also
} } invented by F-M, whose genius contributed so much to new
} } developments in the early days of TEM). I only ever saw advertising
} } brochures of the ultra-microtome, so would be interested to learn of
} } users' experiences from those times and perhaps also something about
} } the fate of these now-historic instruments.
} }
} } -----Original Message-----
} } } From: David Elliott [mailto:David.Elliott-at-yale.edu]
} } Sent: Wednesday, August 04, 2004 5:09 PM
} } To: Microscopy ListServer
} } Subject: [Microscopy] Leica ultra-microtome
} }
} }
} }
} } --------------------------------------------------------------------
} } -- -- ------ The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------
} } -- -- -------
} }
} } Hi all
} } I am looking at Leica ultra-microtomes. The new version (the UC6b)
} } has two controllers, the key pad or the touch screen. I would
} } appreciate any input or comments on these. I am especially
} } interested in reasons to get one or the other. Thanx David
} }
} }
} } _____________________
} }
} } David Elliott Ph.D.
} } Research Assistant Professor
} } Department of Cell Biology and Anatomy
} } PO Box 245004
} } Tucson, AZ 85724
} }
} } Voice: 520-626-7870
} } Fax: 520-626-2097
} }
} }
} }
} }
}
} Joel B. Sheffield, Ph.D
} Department of Biology
} Temple University
} Philadelphia, PA 19122
} Voice: 215 204 8839
} e-mail: jbs-at-temple.edu
}
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

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Leica ultratomes originated from Ultracut series by Reichert-Jung. Am I
correct? It seems to me, Leica did not have their own ultratome
development (would be nice to know details if they did). They just bought
Reichert-Jung and LKB both. They killed SuperNova (LKB) and continued
Ultracut. Sergey

At 01:08 AM 8/5/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

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Aha! Joel, Sergey and anyone else interested in historical matters,

I got motivated after reading your interesting comments and actually located here an old Leica brochure (53-12b, in German) dated June 1964, which described the original "Leica Ultra-Mikrotom nach Fern‡ndez-Mor‡n". It was equipped with a Rawyler diamond knife "of highest quality" and was apparently designed to cut just about anything. The accompanying TEM images show sectioned cells in Vestopal and Methacrylate also an Al/Ag alloy. The 3 kg steel rotor was belt-driven with 2 motors situated below the desk (one was used for the sectioning phase of rotation and cutting speed could be controlled from 50 down to 3 mm/sec, while the fast second motor took over for the rest of the rotation cycle).
The object chuck was at the front of a long diametrically placed cylindrical invar holder (fastened at its back end to the back of the rotor) which had an inbuilt heating element, and the free front end moved by thermal expansion towards the knife for up to 30 mins. After that period the complete holder was removed and allowed to cool down for 15 mins, during which time a second holder could be used for sectioning.
Visualization during sectioning was done with a 72x (Leitz Greenough-type?) stereomicroscope and associated fluorescent lamp. A plexiglas hood was supplied to protect the system from air movements and temperature fluctuations during sectioning.
Other statistics: Weight (+ table) was 148 kg. Power draw-off was 130 W.
The images shown corresponded to typical good quality methacylate sections of the 1950/60s but the instrument never became popular. I imagine that this brochure was one of the last that Leitz issued.
It would seem that the main advantage of this instrument design was that complete 360ˇ rotation obviated the need for specimen retraction. Retraction during the upwards stroke is absolutely necessary for any reciprocating system in order to prevent wetting of the knife front or even breakage of the delicate cutting edge when the specimen moves upwards after cutting because all thermal expansion systems have great inherent inertia and advance cannot be stopped successfully for such short time periods.
One possible disadvantage of the system is the need for rotational bearings.
I do remember vaguely another old ultra-microtome brochure from Leica which had a graph showing the excellent reproducibility of specimen position during cutting from one cycle to the next. This may be so (since German precision workmanship in those years was unbeatable) but the inherent fine-scale bearing rumbling, even if reproducible, would result in a slightly corrugated cut as the specimen would oscillate a little forwards and backwards with respect to the knife during cutting. Perhaps it would need only 10 nm lateral movements in a 100 mm thick section to be noticeable when highest quality ultra-thin sections were examined. Perhaps I am talking somewhat off the top of my head in this case but it would now be interesting to hear from others the real reason(s) for the unpopularity of this long-discontinued instrument - the very FIRST Leica Ultra-Microtome.
Best regards & good sectioning to you all ...

Jim

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Hello folks,

I have a Gatan mod. 681 Ion Beam Coater and I'm looking for targets for
it. I'm on a limited budget so I'd rather not pay Gatan's prices.
Anyone have sources or ideas for Au and Ti targets?

Jerry

--
Gerald Bourne
Major Analytical Instrumentation Center
Department of Materials Science and Engineering
University of Florida
100 Rhines Hall
P.O. Box 116400
Gainesville, FL 32611
(352) 392-6985
(352) 392-0390 fax

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Dear all,

We have a QImaging camera Retiga 1300i 12 bits. The company we deal with for
the image acquisition (with a motorized microscope) uses the 16 bit format.
So, they transform the 12 bit images to 16 bit images.

We want to use deconvolution on these images. Will the transformation to 16
bits impair image quality?

Thank you, have a good week-end!

Marie-Claude Belanger

_________________________________________________________________
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Jerry:

While we do make our own Ion Beam Sputter Deposition and Etching System,
we can supply targets for the Gatan system as well. You will find our
prices to be *very* reasonable. Please contact me off-line about your
specific requirements and I will send you a quote.

Best regards-

David

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

Gerald Bourne wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hello folks,
}
} I have a Gatan mod. 681 Ion Beam Coater and I'm looking for targets
} for it. I'm on a limited budget so I'd rather not pay Gatan's
} prices. Anyone have sources or ideas for Au and Ti targets?
} Jerry
}

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Image quality is highest using the 16-bit format.
Since the original image is 12-bits, image
quality would suffer (mostly due to loss of dynamic
range) if converted to 8-bits. The conversion
from 12-bits to 16-bits is typically accomplished
by zero filling the four high order bits. Consequently,
the image data is in all eight bits of the low order
byte and in the four low order bits of the high order byte.

If your deconvolution program can handle 16-bit images,
there should be no image degradation. Be advised that,
depending on the app itself, your memory requirements
may be more than you have available. Very often one
can get "Out of Memory" error messages. With modest
pixel density and 16-bit TIFF files, you should be OK.

gary g.

At 10:04 AM 8/6/2004, you wrote:

} Dear all,
}
} We have a QImaging camera Retiga 1300i 12 bits. The company we deal with
} for the image acquisition (with a motorized microscope) uses the 16 bit
} format. So, they transform the 12 bit images to 16 bit images.
}
} We want to use deconvolution on these images. Will the transformation to
} 16 bits impair image quality?
}
} Thank you, have a good week-end!
}
} Marie-Claude Belanger

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Hendrik

We also have our 2010F running on a UPS system. I have just done some
measurements and while, yes, there is a very large field at the unit
(} 500mG rms - off scale for my EMF meter) this decays away rapidly and
drops below 1mG rms seven feet from the unit. In our case the column is
about 15' from the UPS and we see no effect.

We are still using the same batteries as delivered in 1998. The 50% life
time in the case of a power failure has diminished but they still provide
sufficient protection for the field emission tip. The battery
specifications from the manufacturer states 200 complete full load
discharges - we were told a typical life was 4-5 years depending on the
number of excursions. Through the manufacturer replacement of all the
batteries was quoted at $5K.

One thing to beware of, on multi-phase UPS systems if you are prone to one
phase ONLY dying you can fry the UPS control board and you will need a
voltage regulator before the UPS unit to protect the UPS.

Regards

Alan

At 11:08 AM 7/23/2004 -0700, Mardinly, John wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Alan W Nicholls, PhD
Director of Research Service Facility (Electron Microscopy)
Research Resources Center - East (M/C 337)
Room 100 Science and Engineering South Building
The University of Illinois at Chicago
845 West Taylor St
Chicago, IL 60607-7058

Tel: 312 996 1227
Fax: 312 996 8091
Office: Room 110

Web site www.rrc.uic.edu

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Robert:

We have a ArtixScan 2500. (as well as two Agfa Duoscan's). The
software interface was a little cumbersome to use, but the image quality was
very good.

However, I strongly recommend against Microtek. On the 2500 the lamp
stays on all the time (i.e. no standby) - o.k., not a problem just wear on the
lamp. The lamp burned out after 8 months - o.k., no problem we replaced
many lamps in previsouly years on several scanners - 5 minutes later lamp in
hand. . . Can NOT get a replacment lamp. We've been looking every where.
Microtek will NOT sell the lamps, they wanted us to send the scanner (67 lbs)
to across country and they would sell us a new shipping box. Fine - but 7
additional months later they can't come up with a shipping box, nor can they
come up with a price for the lamp replacment and NOW they are telling us
we're out of the 12 month warranty.

So here we sit - $3k scanner useless and for a $30 part.

}
} I am looking for comment on overall functionallity of the Microtek
} ArtixScan 1800f scanner. Reliability, resoultion, speed. Will use this
} to scan EM neg. etc.
}
} Thanks
}
} Robert J. Kayton, Ph.D.
} C.R.O.E.T. L606
} Oregon Health & Science Univ.
} kayton-at-ohsu.edu
} 503-494-2504-Lab
} 503-703-3938-Cell
} www.ohsu.edu/croet/facilities/emicroscopy
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

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University of Connecticut
Institute of Materials Science

Postdoctoral Position
SPM manipulation of carbon nanotubes and biological systems

A post-doctoral position is available immediately within the Institute
of Materials Science at UConn to work on SPM imaging, manipulation, and
lithography of carbon nanotubes and biological systems. The ideal
candidate will have experience with AFM measurements in liquid, SPM
lithography, and or SPM technique development. Experiments will be
conducted in the newly constructed NanoMeasurement labs, featuring two
new AFM systems for in vitro and air measurements with simultaneous
confocal microscopy, as well as a UHV AFM/STM.

This position is a one-year appointment, with funding available for
further years. To apply, please send a complete resume, together with a
list of publications and contact details for 3 references, to Prof.
Bryan Huey (bhuey-at-ims.uconn.edu). Screening of applications will begin
immediately, and will continue until the position is filled.
Applications are encouraged from under-represented groups, including
minorities, women, and people with disabilities.

Bryan D. Huey
The Institute of Materials Science
University of Connecticut
97 N. Eagleville Road, unit 3136
Storrs, CT 06269 USA
office: (860) 486 3284
fax: (860) 486 4745
http://www.ims.uconn.edu/
bhuey-at-uconn.edu

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Email: gazzzoman-at-yahoo.com
Name: daniele gazzola

Organization: Biomed dept. -at-Brown Univ., Providence, RI, USA -
Engineering dept. -at-Genova University, Italy

Title-Subject: [Microscopy] [Filtered] hybrid AFM-optical microscope

Question: I am trying to set up a hybrid microscope in order to use
AFM (atomic force microscope) along with light microscopy(phase) on
unstained biological samples.

The AFM that I am using adds two lenses to the optical path just
above the sample. Unfortunately I neither know the specifications of
those lenses, nor the characteristics of the other optical elements.
I know that the plane of the sample is conjugated to a plane 32mm
above the top lens. The whole AFM is practically a tube about 10cm
long and 1cm of diameter.

I am trying to get informations about the optical elements of a long
working distance condenser. Can anyone please send me a diagram?

I think that the AFM will add one conjugate focal plane to the
system. Do you think that this will be a problem?
What about using reflected light (for brightfield, phase, or DIC)?

I would like any comment or idea about this.
thanks a lot,
daniele

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Name: Frida Maiers

Organization: Hennepin County Medical Center

Title-Subject: [Microscopy] [Filtered] MListserver: TEM photographic supplies available

Question: Due to digital camera installation we have the following
available for a nominal fee: 1 case of D19 developer, 11 boxes of EM
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and 17 boxes Kodak Polymax II RC photographic paper (100 sheets
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July 30, 2004 at 22:47:04
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Email: juan-at-nanostellar.com
Name: Juan

Title-Subject: [Microscopy] [Filtered] Export EDX spectrum

Question:
Hi,

I took some EDX spectrum by using EDAX Phoenix 1998 Revision 3.1, but
I can not export the spectrum into a data file. Does anybody know
the method? Any suggestion would be highly appreciated.

Juan

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on Sunday, August 1, 2004 at 14:15:07
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Email: Gsalaj7-at-aol.com
Name: Sally Thomas Graziano

Organization: Orlando Science Center

Education: Undergraduate College

Location: Orlando Florida

Question: In my work on the SEM here at OSC. Along with our
educational programs we have an ongoing research project. In that
regard I have a very small eye cyst from a swan which I need to look
at. As you can see most of my specimens are larger biological
specimens. How should I mount it on the SEM stub. I use carbon tape
for most things but am afraid the cyst will get lost in one of the
bubbles of the tape.Also how long to coat. Any sugestions would be
most helpful. Sally Graziano

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Juan,

You wrote:

} I took some EDX spectrum by using EDAX Phoenix 1998 Revision 3.1, but I
} can not export the spectrum into a data file. Does anybody know the method?
} Any suggestion would be highly appreciated.
}
EDAX have a free spectrum viewer that can be downloaded from:
http://www.edax.com/support/EDS_Spectrum_Viewer.html

You can cut and paste the channel data from this programmme.

Alternatively, I have written an application which will display EDAX .spc
files - as well as Noran, Link/Oxford and EMSA file formats - which allows
export of data as well. Let me know if you want a copy.

David Vowles
Electron Microscope Unit
Dept of Materials Science and Metallurgy
University of Cambridge
Pembroke St Cambridge
UK CB2 3QZ
Tel: +44 (0)1223 334325
Fax: +44 (0)1223 334567
Email: djv23-at-cam.ac.uk

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Hey Listers,

We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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Hi

Can someone point me in the direction of online information regarding
techniques for the identification of asbestos by SEM and by other
techniques?

thanks

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599
ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

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Let us know if you find something that is suitable and *inexpensive*.
Microscopy supply vendors sell plastic boxes, but at the rate I go through
samples, I would go broke and run out of storage room as well.

No inexpensive vials, jars, etc. that I have found protect the prepared
surface well - no mounting method. The best compromise is to use a snugly
fitting "Cap Plug" (poly closure used to close pipe ends, other holes) and
partially insert the mount into it.

If nothing else fits, I stuff the large mounts into a locking closure
plastic bag. It is likely that if fragile or coated, this will harm the
specimen, however.

A great solution (not my idea) for 1/2" (12mm) pin-mounts is an "Opticlear"
25 dram glass vial with a closed bottom poly cap. Punch or cut a snug hole
in the bottom (inside) of the cap, shove the stub pin in and place in
vial...

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Giles, Bill [mailto:William.Giles-at-TIMET.com]
Sent: Monday, August 02, 2004 1:39 PM
To: 'Microscopy-at-microscopy.com'

Hey Listers,

We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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Bill:

We have some containers that are ideal for this application. You can
see an image of them on our website at www.southbaytech.com. Do a
keyword search for "containers". You will also find them listed with
our extensive range of metallographic consumables under the
"consumables" button. I will contact you off-line with pricing.

Best regards-

David

Giles, Bill wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

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Hello Microscopy folks,
I am trying to resurrect an old spectroscopy system that uses a Tracor
Northern TN-6500 box for controlling a linear diode readout. Anyone out
there with a manual for the TN-6500? I am happy to pay photocopy charges
or do anything (reasonable!) to get my hands on one. Thanks again.
Greg Mulhollan
-----------------------------------
Gregory Mulhollan, Ph.D.
Saxet Surface Science
1001 S. Sunset Canyon Drive
Dripping Springs, TX 78620
(512)858-2841 office
(512)694-4879 cell
mulhollan-at-saxetsurfacescience.com
www.saxetsurfacescience.com

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

William Giles wrote:
============================================================================
==============
We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?
============================================================================
==============
SPI Supplies has manufactured for some years our special mount storage box
for 1" mounts, see URL
http://www.2spi.com/cataelog/boxes/speci_box.shtml

This would be our SPI #02020-AB and each one holds eight mounts. There are
inserts for desiccating capsules. And once the samples are loaded into the
box, and the lid closed, some ordinary Scotch Tape is put around the lip of
the closed box to seal out air or anything else that might seep in and
damage samples.

Disclaimer: SPI Supplies is the manufacturer of this special kind of
storage box.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

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Thanks for all the responses; I'll filter thru all the suggestions.

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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We use the "Cap Plugs" Woody has suggested and I find they work well if
you're looking for inexpensive (a few cents per piece) individual sample
storage.

The caps come in a variety of shapes and sizes, and I'm sure there are
many sources for such items. The vendor we ordered from has a good page
with drawings and dimensions for each:
http://www.niagaracapsandplugs.com/nonthreaded_caps.htm

Regards,

Steven T Szewczyk
Materials Science Contractor
US Army Research Lab
Aberdeen Proving Ground, MD

-----Original Message-----
} From: White, Woody N. [mailto:nwwhite-at-bwxt.com]
Sent: Monday, August 02, 2004 4:08 PM
To: 'Giles, Bill'; 'Microscopy-at-microscopy.com'

Let us know if you find something that is suitable and *inexpensive*.
Microscopy supply vendors sell plastic boxes, but at the rate I go
through samples, I would go broke and run out of storage room as well.

No inexpensive vials, jars, etc. that I have found protect the prepared
surface well - no mounting method. The best compromise is to use a
snugly fitting "Cap Plug" (poly closure used to close pipe ends, other
holes) and partially insert the mount into it.

If nothing else fits, I stuff the large mounts into a locking closure
plastic bag. It is likely that if fragile or coated, this will harm the
specimen, however.

A great solution (not my idea) for 1/2" (12mm) pin-mounts is an
"Opticlear" 25 dram glass vial with a closed bottom poly cap. Punch or
cut a snug hole in the bottom (inside) of the cap, shove the stub pin in
and place in vial...

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Giles, Bill [mailto:William.Giles-at-TIMET.com]
Sent: Monday, August 02, 2004 1:39 PM
To: 'Microscopy-at-microscopy.com'

Hey Listers,

We are looking for a source of individual metallographic sample storage
containers. Our mounts are typically 1" diameter and 0.5-1" tall.

Anyone have a source for these?

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

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Hello Microscopists !

Quite some time ago, in anticipation of a congenial meeting of interested
parties at a common-ground investigation of several broken steel bolts in
the Cleveland, Ohio, area, I asked about suitable SEM labs in the area.
I received an excellent response from The List, which indicates that it is
the primary means of rapid and effective communication in the micrsocopy
community. Alas, there was a slower response from the above-referenced
interested parties, and so no agreement about protocol or venue was
reached until we had all retired to our own offices. Later on, we wound up
going back to the place selected originally by one of the parties way back
at the beginning of the project, where 1000X is about the limit of useful
magnification. I am sure any one of you could have done better.

Thanks to all who reponded.

Best regards,
George Langford, Sc.D.
Principal Consultant
Amenex Associates, Inc.
amenex-at-amenex.com
http://www.amenex.com/

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Mr. Chapman,
When you say "stock ammonia solution", are you talking about standard
Ammonia(NH3)?

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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Tuesday, August 3, 2004 at 13:34:53
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Email: garyeaston-at-scannerscorp.com
Name: Gary M. Easton

Organization: Scanners Corporation

Title-Subject: [Microscopy] [Filtered] Cambridge/Leica/LEO S360 SEM

Question: I just picked up a used Cambridge S360 that gives me an
error code 307(defective LAB6 switch). Does anyone out there that
has a complete list of the software error codes and their
explanation? The operator's manual offers no help. Also, if anyone
has the setup software (mag cal,
etc) for this series SEM and is willing to part with a copy, it would
be greatly appreciated. Please reply offline to
garyeaston-at-scannerscorp.com. Thanks in advance.

Gary M. Easton

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Email: cnorton-at-wis-inc.net
Name: chris norton

Organization: Wafer Inspection Services, Inc.

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: We are searching for service engineers with KLA-Tencor
service and applications experience on all models.
Prometrix UV1250/1280; RS 75; 6420; AIT; Starlight; 8100 CD SEMS; etc.

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Hi all
I am looking at Leica ultra-microtomes. The new version (the UC6b) has
two controllers, the key pad or the touch screen. I would appreciate
any input or comments on these. I am especially interested in reasons
to get one or the other.
Thanx
David

_____________________

David Elliott Ph.D.
Research Assistant Professor
Department of Cell Biology and Anatomy
PO Box 245004
Tucson, AZ 85724

Voice: 520-626-7870
Fax: 520-626-2097

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Hi all, I am co-chair of a workshop being given on algae identification at
the North American Lakes Management Society International Symposium in
Victoria Canada. The workshop is being offered November 2,
2004. Normally, its not a problem to get the scopes, but I can't find a
source in Canada. I need 10 teaching scopes with Phase and 400 objectives
and 1 BX60 with Phase at 200 and 400 with a trinoc head and a digital
camera. Can anyone help? I'm located in Michigan, United States. Thanks
much, Ann.

Ann St. Amand, Ph.D.
President
PhycoTech, Inc.
620 Broad St., Suite 100
St. Joseph, Michigan 49085 USA

269-983-3654 (voice)
269-983-3653 (fax)
mailto:astamand-at-phycotech.com
www.phycotech.com

Specializing in Aquatic Sample Analysis and Microscope Accessories

Director, Region V, North American Lake Management Society, www.nalms.org

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Hi David
Keypad does not have all features, touch screen has. It's quite
confusing. For instance if you go with touch pad, you need to buy $5K
interface (whichever it called) for their new cryo-attachment and so on. As
far as I understand, touch-screen is sort of "standard" and they "invented"
key-pad to make cheaper version of the ultratome. You need to check the
compatibility issue, because UC6 is not compatible with previous generation
stuff, like UCT, FSC etc. Good luck with shopping. Sergey

At 08:09 AM 8/4/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

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Below is the result of your feedback form (NJZFM-ultra-55). It was
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on Wednesday, August 4, 2004 at 15:15:22
---------------------------------------------------------------------------

Email: matthew.salanga-at-childrens.harvard.edu
Name: Matthew Salanga

Organization: Children's Hospital Boston

Education: Graduate College

Location: Boston, MA

Question: Greetings!

Does anybody know where I can obtain CFP-YFP FRET control slides. Or
transfected a stable FRET positive cell line. Ideally I am looking
for cells grown on coverslips which have tagged CFP and YFP proteins
that are known to elicit a FRET response.

Thanks!

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on Wednesday, August 4, 2004 at 19:41:48
---------------------------------------------------------------------------

Email: sspence-at-flemingc.on.ca
Name: Susan Spence

Organization: Tottenham Public School

Education: 6-8th Grade Middle School

Location: Tottenham, Ontario Canada

Question: I have a very ruly group of grade 8's, very few
microscopes, and even fewer quality slides from which to view
organelles and unicellular organisms. DO you have any suggestions as
to where I may find good images, either from a light microscope or an
electron microscope? I want to show them what cells really look like
through a microscope without actually having them to touch one.
Thanks for your suggestions!

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The Leica ultra-microtome ....?!
This brings back memories of the original one, based on the design by
Humberto Fernandez-Moran about 50 years ago. Anyone still remember it?
Its design was absolutely unique in that the specimen chuck was mounted
in a motor-driven massive cylinder which performed complete rotations in
the horizontal plane over two pairs of huge flat sapphire bearings
placed in a "V" orientation. I imagine that it must have been a "cow of
a thing" to set up! It was possibly developed to utilize the newly
invented diamond knives (also invented by F-M, whose genius contributed
so much to new developments in the early days of TEM). I only ever saw
advertising brochures of the ultra-microtome, so would be interested to
learn of users' experiences from those times and perhaps also something
about the fate of these now-historic instruments.

-----Original Message-----
} From: David Elliott [mailto:David.Elliott-at-yale.edu]
Sent: Wednesday, August 04, 2004 5:09 PM
To: Microscopy ListServer

Hi all
I am looking at Leica ultra-microtomes. The new version (the UC6b) has
two controllers, the key pad or the touch screen. I would appreciate
any input or comments on these. I am especially interested in reasons
to get one or the other.
Thanx
David

_____________________

David Elliott Ph.D.
Research Assistant Professor
Department of Cell Biology and Anatomy
PO Box 245004
Tucson, AZ 85724

Voice: 520-626-7870
Fax: 520-626-2097

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I do remember setting up something like that. Except my recollection
is that it was designed by Sjostrand. The cylindrical chuck unit had
a groove around it so that you would mount the motor on the wall, and
run a long V-belt from the motor to the microtome. This was to
minimize vibration. The other feature that I remember is that the
cutting speed was quite fast, not at all like what we use today.

Joel

I am using a Reichart-Jung MT 6000 ultramicrotome for standard EM
sectioning. After the specimen goes through the cutting range there is a
beep and the microtome electronics will freeze up, I have tried reseting the
knife and specimen advancements but the problem still persists, does anyone
have a recommendation?

Thanks,

Todd Hamm
Research Technician
Oklahoma Medical Research Foundation
tmhamm09-at-yahoo.com

_________________________________________________________________
Express yourself instantly with MSN Messenger! Download today - it's FREE!
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On my search for the possibility to get high tension and magnification
values out of older Philips and Zeiss TEMs I got no answer from the group
and finally found after an extensive search of the web the following
interface-cards for these TEMs:

For Philips EM 400, 410, 420: http://www.stefan-diller.com/rem_tem3_en.htm
For Zeiss TEMs EM 10 A, B and C: http://www.stefan-diller.com/rem_tem4_en.htm

I hope this is useful for somebody having the same problems with wrong
mag-values and doing new reference images after changing the HT-value on an
old TEM...

--
Timo Junker Holografie
Lindenstr. 10
97297 Waldbźttelbrunn
Tel: ++49 (0)931 4520655
Fax: ++49 (0)931 4520657
www.holografie.com

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Dear Joel,

Thanks for your comments. The ultra-microtome as such was of course invented by Fritiof Sjostrand and I agree that his first models had a remote motor, just as you describe. I did not realize that his design also originally had 360ˇ rotation of the specimen chuck holder. As far as I know his design was developed in conjunction with LKB-Produkter, Bromma Sweden whereas the slightly later Fernandez-Moran instrument was developed with Ernst Leitz, Wetzlar Germany. I seem to recollect that an example of the F-M instrument found its way to Dunedin, New Zealand, but there must have been others too.
Perhaps others might be interested in taking the story further from here....
Cheers,

Jim

-----Original Message-----
} From: Joel Sheffield [mailto:jbs-at-temple.edu]
Sent: Thursday, August 05, 2004 3:05 PM
To: James Chalcroft; Microscopy ListServer

Dear Jim,

I saw the Sjostrand microtome when I taught a course at Rutgers,
Camden, in the 1970's. We actually got it set up and running. They
also had a (barely) working RCA EMU-2 scope. I doubt if they have
kept either.

The other thread in this history, of course, was the system developed
by Keith Porter. In the original models of what eventually became
the Porter-Blum microtome, the block followed the famous
parallelogram path, but advance was thermal. We had a goosneck lab
light mounted over the rod that held the specimen, and you sat there
flashing the light with each pass of the block. If you were good,
you could get beautiful ribbons of silver --but woe betide anyone who
walked past you while you were sectioning!

Later on, Keith developed the offset gimble mechanical advance that
led to the Sorval series of MT microtomes.

The other interesting approach to microtomy was that of Huxley, who
used flexible springs for all of the hinge points, to replace
bearings and reduce vibration. This machine was originally made by
Cambridge, and later distributed by LKB.

} Dear Joel,
}
} Thanks for your comments. The ultra-microtome as such was of course
} invented by Fritiof Sjostrand and I agree that his first models had a
} remote motor, just as you describe. I did not realize that his design
} also originally had 360ˇ rotation of the specimen chuck holder. As far
} as I know his design was developed in conjunction with LKB-Produkter,
} Bromma Sweden whereas the slightly later Fernandez-Moran instrument
} was developed with Ernst Leitz, Wetzlar Germany. I seem to recollect
} that an example of the F-M instrument found its way to Dunedin, New
} Zealand, but there must have been others too. Perhaps others might be
} interested in taking the story further from here.... Cheers,
}
} Jim
}
} -----Original Message-----
} From: Joel Sheffield [mailto:jbs-at-temple.edu]
} Sent: Thursday, August 05, 2004 3:05 PM
} To: James Chalcroft; Microscopy ListServer
} Subject: [Microscopy] Re: RE: Leica ultra-microtome (History)
}
} I do remember setting up something like that. Except my recollection
} is that it was designed by Sjostrand. The cylindrical chuck unit had
} a groove around it so that you would mount the motor on the wall, and
} run a long V-belt from the motor to the microtome. This was to
} minimize vibration. The other feature that I remember is that the
} cutting speed was quite fast, not at all like what we use today.
}
} Joel
}
}
} Subject: [Microscopy] RE: Leica ultra-microtome (History)
} Date sent: Thu, 5 Aug 2004 10:08:02 +0200 From:
} "James Chalcroft" {jchalcro-at-neuro.mpg.de} To: "David
} Elliott" {David.Elliott-at-yale.edu} Copies to: "Microscopy
} ListServer" {Microscopy-at-MSA.Microscopy.Com}
}
} }
} }
} } --------------------------------------------------------------------
} } -- -------- The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America To Subscribe/Unsubscribe --
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} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------
} } -- ---------
} }
} } The Leica ultra-microtome ....?!
} } This brings back memories of the original one, based on the design
} } by Humberto Fernandez-Moran about 50 years ago. Anyone still
} } remember it? Its design was absolutely unique in that the specimen
} } chuck was mounted in a motor-driven massive cylinder which performed
} } complete rotations in the horizontal plane over two pairs of huge
} } flat sapphire bearings placed in a "V" orientation. I imagine that
} } it must have been a "cow of a thing" to set up! It was possibly
} } developed to utilize the newly invented diamond knives (also
} } invented by F-M, whose genius contributed so much to new
} } developments in the early days of TEM). I only ever saw advertising
} } brochures of the ultra-microtome, so would be interested to learn of
} } users' experiences from those times and perhaps also something about
} } the fate of these now-historic instruments.
} }
} } -----Original Message-----
} } } From: David Elliott [mailto:David.Elliott-at-yale.edu]
} } Sent: Wednesday, August 04, 2004 5:09 PM
} } To: Microscopy ListServer
} } Subject: [Microscopy] Leica ultra-microtome
} }
} }
} }
} } --------------------------------------------------------------------
} } -- -- ------ The Microscopy ListServer -- Sponsor: The Microscopy
} } Society of America To Subscribe/Unsubscribe --
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} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } --------------------------------------------------------------------
} } -- -- -------
} }
} } Hi all
} } I am looking at Leica ultra-microtomes. The new version (the UC6b)
} } has two controllers, the key pad or the touch screen. I would
} } appreciate any input or comments on these. I am especially
} } interested in reasons to get one or the other. Thanx David
} }
} }
} } _____________________
} }
} } David Elliott Ph.D.
} } Research Assistant Professor
} } Department of Cell Biology and Anatomy
} } PO Box 245004
} } Tucson, AZ 85724
} }
} } Voice: 520-626-7870
} } Fax: 520-626-2097
} }
} }
} }
} }
}
} Joel B. Sheffield, Ph.D
} Department of Biology
} Temple University
} Philadelphia, PA 19122
} Voice: 215 204 8839
} e-mail: jbs-at-temple.edu
}
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

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Leica ultratomes originated from Ultracut series by Reichert-Jung. Am I
correct? It seems to me, Leica did not have their own ultratome
development (would be nice to know details if they did). They just bought
Reichert-Jung and LKB both. They killed SuperNova (LKB) and continued
Ultracut. Sergey

At 01:08 AM 8/5/2004, you wrote:

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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-089
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

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Aha! Joel, Sergey and anyone else interested in historical matters,

I got motivated after reading your interesting comments and actually located here an old Leica brochure (53-12b, in German) dated June 1964, which described the original "Leica Ultra-Mikrotom nach Fern‡ndez-Mor‡n". It was equipped with a Rawyler diamond knife "of highest quality" and was apparently designed to cut just about anything. The accompanying TEM images show sectioned cells in Vestopal and Methacrylate also an Al/Ag alloy. The 3 kg steel rotor was belt-driven with 2 motors situated below the desk (one was used for the sectioning phase of rotation and cutting speed could be controlled from 50 down to 3 mm/sec, while the fast second motor took over for the rest of the rotation cycle).
The object chuck was at the front of a long diametrically placed cylindrical invar holder (fastened at its back end to the back of the rotor) which had an inbuilt heating element, and the free front end moved by thermal expansion towards the knife for up to 30 mins. After that period the complete holder was removed and allowed to cool down for 15 mins, during which time a second holder could be used for sectioning.
Visualization during sectioning was done with a 72x (Leitz Greenough-type?) stereomicroscope and associated fluorescent lamp. A plexiglas hood was supplied to protect the system from air movements and temperature fluctuations during sectioning.
Other statistics: Weight (+ table) was 148 kg. Power draw-off was 130 W.
The images shown corresponded to typical good quality methacylate sections of the 1950/60s but the instrument never became popular. I imagine that this brochure was one of the last that Leitz issued.
It would seem that the main advantage of this instrument design was that complete 360ˇ rotation obviated the need for specimen retraction. Retraction during the upwards stroke is absolutely necessary for any reciprocating system in order to prevent wetting of the knife front or even breakage of the delicate cutting edge when the specimen moves upwards after cutting because all thermal expansion systems have great inherent inertia and advance cannot be stopped successfully for such short time periods.
One possible disadvantage of the system is the need for rotational bearings.
I do remember vaguely another old ultra-microtome brochure from Leica which had a graph showing the excellent reproducibility of specimen position during cutting from one cycle to the next. This may be so (since German precision workmanship in those years was unbeatable) but the inherent fine-scale bearing rumbling, even if reproducible, would result in a slightly corrugated cut as the specimen would oscillate a little forwards and backwards with respect to the knife during cutting. Perhaps it would need only 10 nm lateral movements in a 100 mm thick section to be noticeable when highest quality ultra-thin sections were examined. Perhaps I am talking somewhat off the top of my head in this case but it would now be interesting to hear from others the real reason(s) for the unpopularity of this long-discontinued instrument - the very FIRST Leica Ultra-Microtome.
Best regards & good sectioning to you all ...

Jim

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Hello folks,

I have a Gatan mod. 681 Ion Beam Coater and I'm looking for targets for
it. I'm on a limited budget so I'd rather not pay Gatan's prices.
Anyone have sources or ideas for Au and Ti targets?

Jerry

--
Gerald Bourne
Major Analytical Instrumentation Center
Department of Materials Science and Engineering
University of Florida
100 Rhines Hall
P.O. Box 116400
Gainesville, FL 32611
(352) 392-6985
(352) 392-0390 fax

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Dear all,

We have a QImaging camera Retiga 1300i 12 bits. The company we deal with for
the image acquisition (with a motorized microscope) uses the 16 bit format.
So, they transform the 12 bit images to 16 bit images.

We want to use deconvolution on these images. Will the transformation to 16
bits impair image quality?

Thank you, have a good week-end!

Marie-Claude Belanger

_________________________________________________________________
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contribuez Žliminer les virus destructeurs susceptibles dây tre intŽgrŽs.
http://join.msn.com/?pgmarket=fr-ca&page=features/virus Commencez dŹs
maintenant profiter de tous les avantages de MSN Premium et obtenez les
deux premiers mois GRATUITS*.

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Jerry:

While we do make our own Ion Beam Sputter Deposition and Etching System,
we can supply targets for the Gatan system as well. You will find our
prices to be *very* reasonable. Please contact me off-line about your
specific requirements and I will send you a quote.

Best regards-

David

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

Gerald Bourne wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hello folks,
}
} I have a Gatan mod. 681 Ion Beam Coater and I'm looking for targets
} for it. I'm on a limited budget so I'd rather not pay Gatan's
} prices. Anyone have sources or ideas for Au and Ti targets?
} Jerry
}

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Image quality is highest using the 16-bit format.
Since the original image is 12-bits, image
quality would suffer (mostly due to loss of dynamic
range) if converted to 8-bits. The conversion
from 12-bits to 16-bits is typically accomplished
by zero filling the four high order bits. Consequently,
the image data is in all eight bits of the low order
byte and in the four low order bits of the high order byte.

If your deconvolution program can handle 16-bit images,
there should be no image degradation. Be advised that,
depending on the app itself, your memory requirements
may be more than you have available. Very often one
can get "Out of Memory" error messages. With modest
pixel density and 16-bit TIFF files, you should be OK.

gary g.

At 10:04 AM 8/6/2004, you wrote:

} Dear all,
}
} We have a QImaging camera Retiga 1300i 12 bits. The company we deal with
} for the image acquisition (with a motorized microscope) uses the 16 bit
} format. So, they transform the 12 bit images to 16 bit images.
}
} We want to use deconvolution on these images. Will the transformation to
} 16 bits impair image quality?
}
} Thank you, have a good week-end!
}
} Marie-Claude Belanger

{/x-flowed}

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Hendrik

We also have our 2010F running on a UPS system. I have just done some
measurements and while, yes, there is a very large field at the unit
(} 500mG rms - off scale for my EMF meter) this decays away rapidly and
drops below 1mG rms seven feet from the unit. In our case the column is
about 15' from the UPS and we see no effect.

We are still using the same batteries as delivered in 1998. The 50% life
time in the case of a power failure has diminished but they still provide
sufficient protection for the field emission tip. The battery
specifications from the manufacturer states 200 complete full load
discharges - we were told a typical life was 4-5 years depending on the
number of excursions. Through the manufacturer replacement of all the
batteries was quoted at $5K.

One thing to beware of, on multi-phase UPS systems if you are prone to one
phase ONLY dying you can fry the UPS control board and you will need a
voltage regulator before the UPS unit to protect the UPS.

Regards

Alan

At 11:08 AM 7/23/2004 -0700, Mardinly, John wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Alan W Nicholls, PhD
Director of Research Service Facility (Electron Microscopy)
Research Resources Center - East (M/C 337)
Room 100 Science and Engineering South Building
The University of Illinois at Chicago
845 West Taylor St
Chicago, IL 60607-7058

Tel: 312 996 1227
Fax: 312 996 8091
Office: Room 110

Web site www.rrc.uic.edu

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Robert:

We have a ArtixScan 2500. (as well as two Agfa Duoscan's). The
software interface was a little cumbersome to use, but the image quality was
very good.

However, I strongly recommend against Microtek. On the 2500 the lamp
stays on all the time (i.e. no standby) - o.k., not a problem just wear on the
lamp. The lamp burned out after 8 months - o.k., no problem we replaced
many lamps in previsouly years on several scanners - 5 minutes later lamp in
hand. . . Can NOT get a replacment lamp. We've been looking every where.
Microtek will NOT sell the lamps, they wanted us to send the scanner (67 lbs)
to across country and they would sell us a new shipping box. Fine - but 7
additional months later they can't come up with a shipping box, nor can they
come up with a price for the lamp replacment and NOW they are telling us
we're out of the 12 month warranty.

So here we sit - $3k scanner useless and for a $30 part.

}
} I am looking for comment on overall functionallity of the Microtek
} ArtixScan 1800f scanner. Reliability, resoultion, speed. Will use this
} to scan EM neg. etc.
}
} Thanks
}
} Robert J. Kayton, Ph.D.
} C.R.O.E.T. L606
} Oregon Health & Science Univ.
} kayton-at-ohsu.edu
} 503-494-2504-Lab
} 503-703-3938-Cell
} www.ohsu.edu/croet/facilities/emicroscopy
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

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Colleagues

The July Archives are now on-line at

http://www.microscopy.com/MicroscopyListserver

Nestor
Your Friendly Neighborhood SysOp

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Hi All,

We have a Reichert Jung Ultracut microtome in need of a part,
specifically the clutch assembly in the fine advance. If anyone could
tell us where we could get such a part it would be greatly appreciated.
In Australia would be best but we'll get it from any part of the globe
if we have to!

Thank you very much for your help and it's great to be back working in
microscopy again after a few years "sabbatical" on other projects!!

Cheers

Colin Veitch

Electron Microscopist

CSIRO Textile and Fibre Technology

PO Box 21, BELMONT, Vic. 3216. Australia.

E-mail: colin.veitch-at-csiro.au

Web: http://www.tft.csiro.au

Tel: +61 (0) 3 5246 4000
Mob: 0438 538 475
Fax: +61 (0) 3 5246 4811

The information contained in this e-mail message may be privileged or
confidential information. If you are not an intended recipient, you may
not copy, distribute or take any action in reliance on it. If you have
received this message in error, please telephone CSIRO Textile and Fibre
Technology on +61 3 5246 4000.

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (castrj01-at-endeavor.med.nyu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, August 10, 2004 at 07:38:02
---------------------------------------------------------------------------

Email: castrj01-at-endeavor.med.nyu.edu
Name: George Castro

Organization: New York University Medical Center

Title-Subject: [Microscopy] [Filtered] siemens elmiskop 1a

Question: }
} I am writing in the hope that
} you might refer us to someone able to repair and service a Siemens
} Elmiskop 1A. I have obtained a limited amount of contacts through the
} web, but with no knowledge of this scope because of its age. Perhaps
} among your members there is a better chance.
} I am very grateful for your time and attention.
} George Castro
}
} George Castro
} Dept. of Surgery
} New York University Medical Center
} 520 First Ave. #421
} New York, NY 10016
} Tel 212 263 6777
} fax 212 263 0227
} castrj01-at-popmail.med.nyu.edu
}

---------------------------------------------------------------------------

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Hi,

Since the end of last year the idea of a Human Cytome Project has been
discussed at several meetings. At the F.O.M. meeting
(http://www.focusonmicroscopy.org/2004/program.html) this year the idea
of a Human cytome Project was discussed in public for the first time.

The next occasion will be the European Microscopy Meeting
(http://www.emc2004.be/) in Antwerp at the end of this month (Friday
August 27, Session LS 18. Round table: The Human Cytome project).

I hope it will be an interesting discussion and I look forward to meet
you at the meeting.

An interesting article on the idea of a Human Cytome Project:
Cytomics - New Technologies: Towards a Human Cytome Project
Valet G., T‡rnok A.
Cytometry 59A:167-171 (2004)

Some links on the topic:

http://www.biochem.mpg.de/valet/cytompr1.html
http://www.biochem.mpg.de/valet/cytompr2.html
http://ourworld.compuserve.com/homepages/pvosta/humcyt.htm
http://www.cytomics.info/

Regards,

Peter Van Osta

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Dear Gerald,
I have found that Abe Dayani of Refining Systems Inc. gives good prices and
service on sputtering and deposition targets of all types. He specializes in
targets. You can contact him at:
Refining Systems Inc.
PO Box 72466
Las Vegas, NV 89170
phone: 702-368-0579, fax: 702-368-0933
www.refiningsystems.com
I am just a satisfied customer.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Gerald Bourne" {grb-at-ufl.edu}
To: "Microscopy ListServer" {Microscopy-at-msa.microscopy.com}
Sent: Friday, August 06, 2004 8:05 AM

Article in today's New York Times about joys of microscopy for children
etc. If the link is still up:
http://nytimes.com/2004/08/10/science/10essa.html?8hpib

____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/

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Hello Everyone
We had a wonderful time in Savannah at the M&M meeting. Many thanks
to all the organisers, vendors and particpants who made it so
worthwhile for me.

But one piece of news I heard at the meeting was that Spurr resin is
supposed to be going off the market next year. As far as I understand
it one of the ingredients is being removed. Has anyone got any
comments about this or heard of an alternative ingredient?
Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

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George,
Peter Stolzenberg of Pesto Inc. had serviced the Siemens in the past but I
received word after I returned from the M&M 2004 meeting that he had recently
passed away. He was the serviceman for my Philips 200 and I received the
message so quickly because I had requested that he do a routine for me when I
returned. Consequently I am also looking for someone who can help me service my
TEM if I get stuck.

A few years ago there was a serviceman working for JEOL whom I had first met at
Temple University when he was servicing a Siemens Elmiskop there. Unfortunately
I can not remember his name.

Pat Connelly
Univ. of PA, Biology
Philadelphia, PA 19104-6018
psconnel-at-sas.upenn.edu
=========================
} Organization: New York University Medical Center
} Title-Subject: [Microscopy] siemens elmiskop 1a
} } I am writing in the hope that
} } you might refer us to someone able to repair and service a Siemens
} } Elmiskop 1A. I have obtained a limited amount of contacts through the
} } web, but with no knowledge of this scope because of its age. Perhaps
} } among your members there is a better chance.
} } I am very grateful for your time and attention.
} }
} } George Castro
} } Dept. of Surgery
} } New York University Medical Center
} } 520 First Ave. #421
} } New York, NY 10016
} } Tel 212 263 6777
} } fax 212 263 0227
} } castrj01-at-popmail.med.nyu.edu

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Dear Listers,

I am just catching up after a holiday so apologies for any delay. There has
been a lot of interesting info regarding early Leitz and Reichert
ultramicrotomes. I can add a little more to this dialogue.

During my time with Reichert-Jung UK as EM product specialist I was offered
several old ultramicrotomes before they were to be thrown into the Skip
(Dumpster in the US?). At one time I had around a dozen of these dinosaurs
cluttering up my house but most of them are now thankfully residing in the
Archive Building of the Science Museum in London.

Some of those I had were as follows:

Sorvall MT1 and MT2
Reichert Om U1 a design by Prof. H Sitte taken up by that company
LKB Sjostrand - the original ultramicrotome from LKB on which I learned
ultramicrotomy
Leitz - after a design by Fernandez-Moran, a massive but beautifully made
unit
Philips - yes even this company dabbled in ultramicrotomes
Cambridge Rocker - a factory modified microtome for ultra thin sectioning
Cooke and Perkins - a simple English ultramicrotme from the fifties
Cambridge Huxley
Si-ro-flex - an excellent microtome with superbly novel and advanced
features made by the Fairey Aviation in Australia

For those interested the first attempts to cut "ultrathin" were a bit of a
cheat as the idea was to cut cake-type slice from a specimen and try to
image cells at the thinnest part of the wedge. Not entirely successful.
There was an early diversion with high speed microtomes in the forties
particularly in the USA with massive rotational speeds up to 57,000 rpm but
cost and probably aerodynamics (or lack of them) led to there demise.

For anyone who might be as 'barmy' as I am with the history of these things
I was once talked into writing a short article for "Microscopy and
Analysis". The reference is:

The Thin End of The Wedge - A personal View of The Development of The
Ultramicrotome by T W Cooper, Microscopy and Analysis, January 1990.

I have no electronic copy of this dry old missive, but for anyone unable to
track it down I do still have a few reprints available that I would happily
send one to any interested party,

Best regards

Terry Cooper
TAAB Laboratories Equipment Ltd
3 Minerva House, Calleva Park
Aldermaston, Berks, RG7 8NA, England
Tel ++44 (0)118 981 7775 Fax ++44 (0)118 981 7881
e-mail sales-at-taab.co.uk
www.taab.co.uk

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So sad to hear of Peter Stolzenberg's passing. He lived and had his
offices in Cold Spring Harbor, NY (on Long Island) when I was a grad
student at the CW Post campus of LIU, and he kept our ancient Hitachi
Hu-11A in fine running order. I got to know Peter quite well during
the protracted period of time it took to track down one circuit in
the HV cabinet that would short out in a very unpredictable fashion.
It was always fun to be working at the scope and hear what sounded
like a crack of lightening followed by total loss of HV. It was a
matter of having Peter there with his meters in the right place at
the right moment. Since his home was just a few miles down the road
from the campus, he would stop by in the morning on his way out to
other calls and then again on his way home at the end of the day.
This went on for about 2 weeks or so. We were finally lucky, he
found the problem and even had the right tube (yes, it was all vacuum
tubes, remember those?) in stock.
I learned a lot of what I know about the inner workings of an EM from
Peter, and with his coaching and coaxing, got past my uneasiness
about tackling mechanically-related problems with that old beast.
Skills that I've carried with me.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

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Terry's mention of the high speed microtomes reminded me of a talk by
the then semi-retired Keith Porter that I was lucky enough to attend
in which he discussed the early years of EM work at the Rockefeller
University. One of the things he described was just such a
microtome. He said that the cutting speed was very fast, and that
the sections flew off the knife ( steel, if I remember correctly) and
were caught against a wire screen cage surrounding the microtome.
The sections were manually retrieved from the screen.
I hope I've remembered this correctly. Dr. Porter's description was
so animated, it created a very vivid impression.
Talk about doing things the hard way!

Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

{/x-flowed}

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Good Morning Elaine and all other microscopy listservers whom are
interested in the Spurrs resin and its "whereabouts". Although it is
true that one of the constituents is being dwindled from the market
ERL-4206 (due to safety issues) for the past 2 years all of our
Scientific team at Electron Microscopy Sciences has been doing
comparitive testing of like and similar resins to find the one that best
works as the original. Over the 2 years of testing we have been able to
come up with one and modify it to the point where it is basically
undistinguishable from the original 4206. We call it the ERL
4221(catalog number EMS 15004). Formulas do not have to change and the
4221 will become an exact replacement fo the 4206 and none of us will
ever know the difference. Blocks, sectioning, staining all will remian
unchanged. So this is the good news. At this time there is no bad news
at all.
If you have any questions or I may be of any assistance please do not
hesitate to contact us. We look forward to hearing from you

Sincerely

Stacie Kirsch
Electron Microscopy Sciences
Tel: 215-412-8400
Fax: 215-412-8450
E-mail: sgkcck-at-aol.com
Website: www.emsdiasum.com
-----Original Message-----
} From: Elaine Humphrey [mailto:ech-at-interchange.ubc.ca]
Sent: Tuesday, August 10, 2004 3:34 PM
To: microscopy-at-msa.microscopy.com

Hello Everyone
We had a wonderful time in Savannah at the M&M meeting. Many thanks
to all the organisers, vendors and particpants who made it so
worthwhile for me.

But one piece of news I heard at the meeting was that Spurr resin is
supposed to be going off the market next year. As far as I understand
it one of the ingredients is being removed. Has anyone got any
comments about this or heard of an alternative ingredient? Elaine

--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

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Oh, I'm sorry to hear that! Mr. Stolzenberg was just here a couple of
weeks ago to service our old Zeiss EM 10-he did a great job. Please
send my condolences.

Does anyone know of anyone who can service our Zeiss EM 10CA? It's OK
now, but we will certainly need someone in the future.

Thanks,
Kathleen Roberts
Principal Lab Technician
Neurotoxicology Labs
Dept. of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

psconnel-at-sas.upenn.edu wrote:

} ------------------------------------------------------------------------------
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Colleagues

I have spoken with Eric Ambrose concerning this message. In my opinion it
is not an advertisement and is definitely of interest and importance to the Microscopy Community.

Eric , thank you again for first checking with me on this.

Nestor
Your Friendly Neighborhood SysOp

----------------------------------------------------

Hi,

For the M & M Education Outreach program next year in Hawaii, we would
like to gather information on the various curriculum available for
teaching electron microscopy in the high schools. One of the drawbacks
of doing this, is that each of us must develop exercises and curriculum
to make it available to the high school teacher. This is very time
consuming. Rather than re-inventing the wheel, we are trying to find
those involved in these types of outreach activities who would be
willing to share some of their materials or let us know if it is
available for purchase. Even finding out the logistics of how you teach
the courses in the high school would be helpful.

This would be really helpful to percolate the excitement about
microscopy to high school students.

You can email me off-line.

Thank you so much in advance, for any assistance you can be.

Judy Murphy
Stockton, CA

murphyjudy-at-comcast.net

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 13 11:29:01 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (morillm-at-mail.rockefeller.edu) from http://microscopy.org/MicroscopyListserver/MLFormMail.html on Friday, August 13, 2004 at 11:26:17
---------------------------------------------------------------------------

Email: morillm-at-mail.rockefeller.edu
Name: Marivel Morillo

Organization: Rockefeller University

Title-Subject: [Microscopy] [Filtered] full-time electron microscopist position open

Question: Attention all Electron Microscopists!

The Laboratory of Developmental Genetics at The Rockefeller University
seeks a full-time electron microscopist to assist in studies of nervous
system development and cell death in the nematode C. elegans.

Work will involve preparing specimens for TEM, serial sectioning, and 3-D
image reconstructions. The successful candidate will become an integral part
of ongoing scientific efforts in the lab, and could also pursue independent
research. Previous experience with TEM is required, and experience with
serial sectioning experience a plus. Applicants must hold a minimum of a
Bachelor's degree.

We offer a competitive salary, comprehensive benefits, a gracious working
environment, and tuition reimbursement. For immediate consideration, send
resume/C.V. to: Ms. Kara R. Marshak, Senior Employment Specialist, The
Rockefeller University via fax (212)-327-7079 or email
{mailto:marshak-at-rockefeller.edu} marshak-at-rockefeller.edu. For more information about ongoing research in
this laboratory, please visit our website located at
{http://www.rockefeller.edu/labheads/shaham/shaham-lab.php} http://www.rockefeller.edu/labheads/shaham/shaham-lab.php.

An Affirmative Action/Equal Opportunity Employer. The Rockefeller
University appreciates all responses and will contact candidates selected
for further consideration.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Aug 14 02:15:49 2004

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I have just received a box full of wax blocks I made about 18 years ago for a study of reproductive biology and zooxanthellae of Millepora platyphylla, fire coral. I don't have a microtome, but thanks to the generosity of a microscopist cleaning out a lab, I have a steel microtome knife. I surely cannot afford a microtome, or especially the shipping, but I remember some plans from some discarded library material some years ago, for microtomes. One used a candle to heat a long metal rod, effectuating a gradual lengthening, for example.

Can anyone suggest whether hand sections are worth while to try of wax blocks. The blocks were made with paraplast. Being several years old, even though I have to assume they are still ok, should I take any special steps with storage or rejuvenation?

I'm afraid to ruin them. The study broke some ground, has not been published, and deserves to be followed through. Even though my notes have been lost through years of sore neglect, typhoons, and ex-spousal neglect, there are some hopeful clues in these specimens that would still be worthwhile, and dates of collection and other information are still recoverable for the most part, through existence of a parallel labelled collection of hard parts, with dates written on them. So... any suggestions on long term care of wax blocks, as well as suggestions for hand-sectioning, would be welcome.

I have a hand microtome, with German inscriptions, that may be useful.

Thank you,

Alan Davis
Kagman High School
Saipan, N. Mariana Islands
aedavis-at-eccomm.com

From MicroscopyL-request-at-ns.microscopy.com Sat Aug 14 15:55:53 2004

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Alan,

Having made more Paraplast embeddings than I care to remember..... The only
thing I can think of is to keep them in a cool dry place; otherwise, they
should last a very long time. The other question about how to section is an
interesting one. You already have a hand microtome and it might be worth a
try although I don't know how it is to be set up. You have a microtome
blade but do you have a handle for it? If not, it should be a low cost item
to acquire and I have the name of a local place that may have some.

I made a hand microtome using a screw type micrometer gauge, cutting off the
arch portion and mounting the screw portion to a steel cylinder with a hole
in it through which the screw part would push the tissue sample out by a
known amount. The top of the cylinder of course was ground to a reasonably
fine polish. The exposed sample was then cut using a microtome blade on a
handle. I used it primarily for fresh plant samples that I would sandwich
between some soft material like balsa, or Sambucus pith, cork, etc before
inserting it into the hole.

Damian Neuberger Ph.D.

I have just received a box full of wax blocks I made about 18 years ago for
a study of reproductive biology and zooxanthellae of Millepora platyphylla,
fire coral. I don't have a microtome, but thanks to the generosity of a
microscopist cleaning out a lab, I have a steel microtome knife. I surely
cannot afford a microtome, or especially the shipping, but I remember some
plans from some discarded library material some years ago, for microtomes.
One used a candle to heat a long metal rod, effectuating a gradual
lengthening, for example.

Can anyone suggest whether hand sections are worth while to try of wax
blocks. The blocks were made with paraplast. Being several years old, even
though I have to assume they are still ok, should I take any special steps
with storage or rejuvenation?

I'm afraid to ruin them. The study broke some ground, has not been
published, and deserves to be followed through. Even though my notes have
been lost through years of sore neglect, typhoons, and ex-spousal neglect,
there are some hopeful clues in these specimens that would still be
worthwhile, and dates of collection and other information are still
recoverable for the most part, through existence of a parallel labelled
collection of hard parts, with dates written on them. So... any
suggestions on long term care of wax blocks, as well as suggestions for
hand-sectioning, would be welcome.

I have a hand microtome, with German inscriptions, that may be useful.

Thank you,

Alan Davis
Kagman High School
Saipan, N. Mariana Islands
aedavis-at-eccomm.com

From MicroscopyL-request-at-ns.microscopy.com Sun Aug 15 10:31:27 2004

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Hello everybody
      I am looking for advice on representing 2D and 3D vector data. Namely, the image I collect from the microscope is either two dimensional vector (dx,dy) at each point, or three dimensional vector (dx,dy,dz). For example, it is in-plane polarization (or magnetization) vector or full 3D polarization vector. The data is collected in the form of ASCII files.
      I have seen numerous examples in which such data is represented as color-coded images (e.g., EBSD) and I will appreciate advice on how it can be done best (e.g., how to relate (dx, dy) and RGB color intensities, etc). I am currently using the straightforward approach of importing data files into Mathematika (they are generated by custom LabView based software) and assigning color values using RGBColor function.
      Thank you in advance
      Sergei

--
Sergei V. Kalinin,
Wigner Fellow and Research Staff Member
Oak Ridge National Laboratory,
1 Bethel Valley Rd,
Bldg. 3025, MS6030,
Oak Ridge, TN 37831
Phone: (865) 241-0236
FAX: (865) 574-4143
URL: sergei2.kalininweb.com
New: http://nanotransport.ornl.gov

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 16 07:17:48 2004

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NIST, AVS and MAS will co-sponsor a Workshop on Modeling Electron Transport
for Applications in Electron and X-ray Analysis and Metrology at NIST
(Gaithersburg, Maryland, November 8-10, 2004) to highlight progress and
determine directions for future development of electron-simulation
techniques and the needs for electron-interaction data. This Workshop will
bring together experts in the physical theory and data that support the
simulation techniques as well as scientists and engineers who develop
models and obtain results for specific applications. Applications will
include x-ray microanalysis of particles, rough and layered surfaces, Auger
analysis of near-surface features, testing of matrix-correction procedures
for bulk analysis, metrology of sub-micrometer scale features in SEM
images, low-voltage and ultra-low-voltage microscopy simulation, radiation
physics, etc. A planned poster session will include demonstrations of
relevant software and databases.

Further information on the Workshop can be found at
http://www.nist.gov/electron. We are now inviting the submission of
abstracts for the Workshop, the deadline being October 8. Enquiries should
be directed to dale.newbury-at-nist.gov

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 16 09:38:32 2004

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Hello, I work for a small research lab, and we plan to do TEM on mouse
tissue. We will fix the tissue in Trump's which is 4% formaldehyde + 1%
glutaraldehyde in a phosphate buffer. Has anyone use this fixative before?
Any pitfalls that we should avoid? Any comments will be very helpful.
Thanks alot!

Scott
Beth Israel Deaconess Medical Center
Boston, MA

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 16 12:01:15 2004

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} Good Morning -
}
} There is a great job opening in my area. The work is very interesting and
} the work environment is casual.
} Thousand Oaks (T.O.) is 1 hour NW of LA in beautiful Ventura County. The
} hiking trails are everywhere and we are 8 miles north of Malibu Beach.
} T.O. was recently rated safest city over 100,000 in the US. If interested
} you can email me directly or go thru the Amgen website and click on
} careers.
regards
} Gianni Torraca
} 805-447-7445
} gtorraca-at-amgen.com
}
} Title: Research Scientist/Assoc Scientist
} Department: 3760 - Analytical Sciences
} Location: Thousand Oaks CA
} Job ID: amge-00004427
} HR Recruiter: Ernest Allen
} (805) 447-6072
} ernesta-at-amgen.com
}
} Requirements:
} Strong skills in microscopy and micro-particle handling are needed.
} Experience in optical microscopy, FT-IR microscopy, and SEM-EDS is
} preferred. Experience in micro-particle identification and sizing and
} manufacturing incident investigation is desired. Experience in techniques
} commonly used for PSDA, such as light-obscuration techniques, as well as
} other skills relevant to the structural characterization of
} pharmaceuticals or biopharmaceuticals, is a plus. Excellent problem
} solving skills and good written and verbal communication skills are
} required.
} Educational requirements:
} M.S. or equivalent with extensive experience in Physical Chemistry,
} Analytical Chemistry, Biochemistry or related field.
}
} Job Summary:
} This position is for a scientist in the structural characterization group.
} A key responsibility will be analytical support of investigations by
} identification of adventitious micro-particles. Support of process
} development and support of incident investigations for both clinical and
} commercial drug products will be required. This position requires hands on
} work in the lab and may require supervision of scientific staff as the
} group grows. The position will also involve some particle size
} distribution analysis of resins, inclusion bodies, and similar objects.
} Experience:
} Relevant experience in the pharmaceutical or biopharmaceutical industry is
} desirable; other relevant experience may be acceptable. Experience in
} development and implementation of emerging technologies is desirable, and
} supervision of scientific staff is a plus.
}
****************************************************************************
**********************

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 16 13:59:47 2004

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Phosphate fixes can result in fine calcium precipitates. I prefer HEPES or
PIPES.

At 10:59 AM 08/16/04 -0400, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 16 21:10:56 2004

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I use modified Trump's fixative with 0.1M sodium cacodylate buffer
without problems with most kinds of tissue. I also use 0.1M phosphate
buffer without artifact problems as long as I wash in buffer 3X after
fixation prior to osmification (1% osmium in 0.1M buffer for 60 minutes)
followed by 3X rinse in buffer and additional 3X rinse in water prior to
dehydration in ethanol series. My problem had been "osmium peppering" -- a
fine precipitate contaminating samples run up in phosphate buffer when not
thoroughly washed. Na-cacodylate avoids this problem, but I always rinse
thoroughly when running up samples for TEM.
I run up tissue at room temperature because of a superstition
acquired as a graduate student that cold temperature promotes the
disassembly of microtubules. Does anyone have thoughts pro or con about
running up tissue on ice vs. room temperature?

Dean Abel
Biological Sciences 143 BB
University of Iowa
Iowa City IA 52242-1324

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 16 21:22:24 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (frah0010-at-umn.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, August 16, 2004 at 19:54:57
---------------------------------------------------------------------------

Email: frah0010-at-umn.edu
Name: Ellery Frahm

Organization: University of Minnesota Electron Microprobe Lab

Title-Subject: [Microscopy] [Filtered] MListserver: Cameca timeline question

Question: Greetings,

Does anyone know approximately when Cameca SU30 SEMprobes were manufactured?

Thanks,
Ellery

--------------------
Ellery E. Frahm
Research Fellow & Manager
Electron Microprobe Laboratory
University of Minnesota - Twin Cities
Department of Geology & Geophysics
Lab Website: http://probelab.geo.umn.edu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 17 02:07:43 2004

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Dear all,

I'm looking for a staining method to prepare an ultramicrotomed
polyurethane polymer for a TEM investigation. Contrast is needed between
the hard and soft segements of the polymer. The functional groups of the
soft segments are mainly carbonates, and of the hard segments amides or
urea. Both segments also have a different urethane content.

Are there staining methods recommended for polyurethane polymers with
such a combination of functional groups (for certain urethanes, OsO4 or
RuO4 may be used)? Can such polymers be imaged by coherent phase
contrast alone?

Thanks in advance

Thomas Keller

--
---------------------------------------------------
Dr. Thomas Keller
Institute of Materials Science and Technology (IMT)
Friedrich-Schiller-University Jena
Löbdergraben 32
D-07743 Jena
Germany
Phone: ++ 49 3641 947742
Fax: ++ 49 3641 947732
Mobile: ++ 49 170 1439522
Internet: t.keller-at-uni-jena.de
---------------------------------------------------
Visit us under http://www.uni-jena.de/matwi/

"Making Materials Science Work 4 U"
---------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 17 09:33:17 2004

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Dean,
I have used a combination fixative of 1% glutaraldehyde,1% OsO4 in
0.05M Phosphate Buffer -at-6.2pH ON ICE and kept dark for 45min. for
many tissues. There are many microtubules present.
Perhaps the microtubules were stablized by the osmium before
they were able to disassemble in the cold temperature.

The only problem I had with this fixative was with bacteria inside
tissue cultured macrophages. It did not wash out as easily/quickly
as I expected. As a result I had the "peppering" of the osmium in and
around the bacteria itself when the TEM beam hit the bacteria.

Pat Connelly
Univ. of PA, Biology
Philadelphia, PA
psconnel-at-sas.upenn.edu
=======================
Quoting Dean Abel {dean-abel-at-uiowa.edu} :
} I use modified Trump's fixative with 0.1M sodium cacodylate buffer
} without problems with most kinds of tissue. I also use 0.1M phosphate
} buffer without artifact problems as long as I wash in buffer 3X after
} fixation prior to osmification (1% osmium in 0.1M buffer for 60 minutes)
} followed by 3X rinse in buffer and additional 3X rinse in water prior to
} dehydration in ethanol series. My problem had been "osmium peppering" -- a
} fine precipitate contaminating samples run up in phosphate buffer when not
} thoroughly washed. Na-cacodylate avoids this problem, but I always rinse
} thoroughly when running up samples for TEM.
} I run up tissue at room temperature because of a superstition
} acquired as a graduate student that cold temperature promotes the
} disassembly of microtubules. Does anyone have thoughts pro or con about
} running up tissue on ice vs. room temperature?
}
} Dean Abel
} Biological Sciences 143 BB
} University of Iowa
} Iowa City IA 52242-1324

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 17 09:57:44 2004

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Hi, Thomas,

Specifically what information are you trying to obtain? If you are looking
for location of specific functional groups, you might try scanning
tunneling microscopy instead. I just sat in on a demo where Kim
Kangasniemi discussed some work like this, as part of his Master's
thesis. He can be reached at Kim-at-nt-america.com.

Hope this is helpful.

Barbara Foster
Microscopy/Microscopy Education
We've Moved!
313 S Jupiter Road, Suite 100
Allen, TX 75002
PH: 972-954-8011 FX: 972-954-8018 Web: www.MicroscopyEducation.com

~-at-~-at-~~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-
Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit
www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-

At 12:29 AM 8/17/04, Thomas Keller wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Tue Aug 17 11:14:03 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi, Thomas
Depending on the size of "soft" and "hard" regions, the best way to image them can be variants of phase-sensitive AFM (phase mode), force modulation mode, or acoustic or ultrasonic force microscopy. Basically, all these techniques are sensitive to hardness and losses at the tip-surface junction; the variation is primarily in frequency range and modulation/detection mechanism. Resolution is primarily limited by the tip-surface contact area and can be as small as few nanometers. Please feel free to contact me directly if this sounds useful.
Sergei

--
Sergei V. Kalinin,
Wigner Fellow and Research Staff Member
Oak Ridge National Laboratory,
1 Bethel Valley Rd,
Bldg. 3025, MS6030,
Oak Ridge, TN 37831
Phone: (865) 241-0236
FAX: (865) 574-4143
URL: sergei2.kalininweb.com

-----Original Message-----
} From: Barbara Foster [mailto:bfoster-at-mme1.com]
Sent: Tuesday, August 17, 2004 1:16 PM
To: Thomas Keller; Microscopy-at-MSA.Microscopy.Com

Hi, Thomas,

Specifically what information are you trying to obtain? If you are looking
for location of specific functional groups, you might try scanning
tunneling microscopy instead. I just sat in on a demo where Kim
Kangasniemi discussed some work like this, as part of his Master's
thesis. He can be reached at Kim-at-nt-america.com.

Hope this is helpful.

Barbara Foster
Microscopy/Microscopy Education
We've Moved!
313 S Jupiter Road, Suite 100
Allen, TX 75002
PH: 972-954-8011 FX: 972-954-8018 Web: www.MicroscopyEducation.com

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Optimizing Light Microscopy for Biological and Clinical Labs is available
in individual copies or classroom size orders. Visit
www.MicroscopyEducation.com
for details.
~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-~-at-

At 12:29 AM 8/17/04, Thomas Keller wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 17 21:27:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (NairIndira2004-at-yahoo.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, August 17, 2004 at 11:07:42
---------------------------------------------------------------------------

Email: NairIndira2004-at-yahoo.com
Name: Indira Nair

Organization: Bahauddin Zakariya University

Education: Undergraduate College

Location: Multan, Pakistan

Question: Dear Gurus,
can anybody help me to find any technical information on LEO EVO 50SXVP SEM? I've found description of EVO50XVP at LEO's site but no information on the former model.

Thanks in advance,
Indira

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 18 01:09:24 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (NairIndira2004-at-yahoo.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, August 17, 2004 at 11:07:42
---------------------------------------------------------------------------

Email: NairIndira2004-at-yahoo.com
Name: Indira Nair

Organization: Bahauddin Zakariya University

Education: Undergraduate College

Location: Multan, Pakistan

Question: Dear Gurus,
can anybody help me to find any technical information on LEO EVO 50SXVP SEM? I've found description of EVO50XVP at LEO's site but no information on the former model.

Thanks in advance,
Indira

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 18 07:18:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Trypan quenching of fluroescence has been used for years to decrease
fluorescence of particles and dextran. In our case, we are trying to
use it to quench the fluorescence of surface labeled particles to
distinguish internalized particles (phagocytosis) from external
particles. We have not gotten significant quenching, and as I read
the literature, I am unclear as to how this is supposed to work. In
the original Hed paper that most people reference, they use FITC
labeled particles and quench by putting the cells in a trypan
solution in a pH 4.5 buffer. They describe this as a FRET type
quenching to a non-radiative acceptor. Trypan does emit, but lets
leave this aside for now. Their explanation makes little sense to me
since with the known pH dependence of FITC, it seems to me they are
doing primarily pH based quenching as opposed to FRET based
quenching. If so, then are they simply looking at the difference in
FITC fluorescence between the phagosomal pH (5.5) and the external pH
(4.5)?
In other papers, rhodamine labelled particles are used, and trypan
quenching is also supposed to work, however in our case, we can only
see about 50% quenching. Given how opaque the solution is, I could
easily see that being a case of simply decreasing both excitation and
emission due to opacity of the solution. In some cases (yeast
particles) I have been told that the trypan actually binds to the
particles so that you can wash it out and the particles are still
blue, and in that case, I would imagine very different quenching
properties, since the trypan is no longer freely diffusing in
solution. I have yet to find literature that clearly investigates
the quenching phenomenon with different fluors under solution vs.
bound conditions. Can anyone help? Thanks- Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 18 11:54:06 2004

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Does anyone have an idea where I can find a NIST traceable glass scale that
measures in the range of 1 ~ 10 microns possibly with the first micron
subdivided into tenths. This will be used on a light microscope for
calibration purposes. Thank you

Robert Fowler
Quality Assurance Failure Analysis Technician
TDK Components USA, Inc.
Multilayer Ceramic Capacitor Division
1 TDK Boulevard
Peachtree City GA 30269-2051
Telephone: (770) 631-0410 Ext.249
Fax: (770) 487-1460
email: robert.fowler-at-tdktca.com
www.component.tdk.com

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 18 13:24:30 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,

I'm looking at putting a digital camera (Evolution MP, QIMAGING
MicroPublisher 5.0 RTV) on my Olympus Stereozoom SZH Microscope (with DF
PLAN objectives). In the initial trial, I had some chromatic aberration.
I'm not sure where it's coming from. Does anyone have any experience with
combining this camera and microscope? Any suggestions to reduce chromatic
aberration?

Thanks,

Diane Ciaburri

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 18 15:16:57 2004

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Robert -

Not sure of the exact traceability path, but BCR and PTB are recognized
Worldwide.

http://www.irmm.jrc.be/rm/cert-reports/BCR-676_cert.pdf

Good Luck

Marc Helvey
Strategic Accounts Manager
VLSI Standards, Inc.
3087 North First Street
San Jose, CA 95134-2006
Phone: (408) 428-1800, ext. 108
FAX: (408) 428-9555
E-mail: marc.helvey-at-vlsistd.com
Internet: http://www.vlsistandards.com

-----Original Message-----
} From: Robert.Fowler-at-tdktca.com [mailto:Robert.Fowler-at-tdktca.com]
Sent: Wednesday, August 18, 2004 10:16 AM
To: Microscopy-at-MSA.microscopy.com

Post Doctoral Position in the NCSU Analytical Instrumentation Facility SIMS
Laboratory

The Analytical Instrumentation Facility (AIF) of the NC State University
College of Engineering has an opening for a postdoctoral research associate
in its SIMS laboratory. The successful candidate will operate our magnetic
sector IMS-6f magnetic sector and our Atomika 4100 quadrupole SIMS
instruments. The successful candidate must be interested in learning and
participating in the analysis of a wide variety of samples (semiconductors,
metals, ceramics, polymers). Work in the laboratory will consist of a
combination of SIMS analytical technique research, experimental design,
instrument operation and data interpretation for university and industrial
researchers. Training in SIMS and other analytical techniques and
instrumentation (AFM, FIB, SEM, XPS, optical and stylus profilometry etc.)
will be provided as needed for supporting SIMS research and analysis. For
information on AIF, see our web site: http://www.ncsu.edu/aif/.

A Ph.D or equivalent in Analytical Chemistry, Applied Physics, Materials
Science or a materials related discipline is required. SIMS experience is
highly desirable although training will be given to a suitable applicant.
Experience in vacuum equipment and/or electronics maintenance; operational
and programming experience with Windows and Unix operating systems; and
experience with analysis of semiconductor or other non biological materials
are desirable.

Please send resume and three letters of reference to: Dr.
Dieter Griffis, Associate Director; Analytical Instrumentation Facility;
North Carolina State University; Box 7531, Room 118A EGRC; 2410 Main Campus
Drive; Raleigh, NC 27695-7531 or email dgriffis-at-ncsu.edu

NC State is an EOE/AA employer. NC State welcomes all persons without
regard to sexual orientation. ADA individuals desiring reasonable
accommodations contact Dieter Griffis at above address, or
dgriffis-at-ncsu.edu, or call 919-515-2128

______________________________
Roberto Garcia
rgarcia-at-unity.ncsu.edu
http://www.ncsu.edu/aif
http://www.ncsu.edu/aif/asm

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 19 09:22:20 2004

Contents Retrieved from Microscopy Listserver Archives
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Scott,

I was assuming it was not the chip since I have blue fringes toward the
outside of the image and red fringes toward the center. If it was the chip,
I thought the colored fringes would stay on one side. Does that make sense?

Diane

-----Original Message-----
} From: Scott Whittaker [mailto:Whittaker.scott-at-nmnh.si.edu]
Sent: Wednesday, August 18, 2004 4:52 PM
To: Ciaburri, Diane A

Hello,

I'm looking at putting a digital camera (Evolution MP, QIMAGING
MicroPublisher 5.0 RTV) on my Olympus Stereozoom SZH Microscope (with DF
PLAN objectives). In the initial trial, I had some chromatic aberration.
I'm not sure where it's coming from. Does anyone have any experience with
combining this camera and microscope? Any suggestions to reduce chromatic
aberration?

Thanks,

Diane Ciaburri

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 19 09:33:11 2004

Contents Retrieved from Microscopy Listserver Archives
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Jim,

It sounds interesting. Could you give me a few more details about running a
test with a color chart? What kind of color chart, and what would I do with
it?

Thanks!

Diane Ciaburri

-----Original Message-----
} From: Jim Quinn [mailto:jquinn-at-www.matscieng.sunysb.edu]
Sent: Wednesday, August 18, 2004 5:30 PM
To: Ciaburri, Diane A

Dear Listees,

Does anyone have a spare Chiller for our Hitachi 7000, TEM? or do you know
some one who might?

Flow of 4-5 L/Min.
Pressure: 0.5-2 kg/sq. cm
Temp: 10-25 degrees Centigrade

Thanks,

Darryl Krueger
Research Associate
Clemson University

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 19 15:35:04 2004

Contents Retrieved from Microscopy Listserver Archives
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I'm dismantling a vintage 1968 Hitachi HU125E TEM that has been our faithful
scope since 1986. Anyone need some parts? Contact me off-list.

Robert
--
Robert Fitton
Teaching Associate/Director of Laboratories
Luther College
Department of Biology
700 College Drive
Decorah, IA 52101

fittonro-at-luther.edu
Voice 563-387-1559
FAX 563-387-1080

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 19 22:07:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (rgr-at-georgetown.edu) from
http://www.msa.microscopy.org/Ask-A-Microscopist/Ask-A-Microscopist.html
on Thursday, August 19, 2004 at 08:41:36
---------------------------------------------------------------------------

Email: rgr-at-georgetown.edu
Name: Robert Russell

Organization: Georgetown University

Education: Graduate College

Location: Washington,District of Columbia, USA

Question: I am seeking information about suitable resins/plastics in which to
embed metal stents and similar devices and then
conduct imunohistochemistry staining for biomarkers
in the surrounding tissues - i.e. artery and soft tissue.
This nquiry is about suitable protocols/experience
of plastics or other embedding methods that preserve
the antigens during the polymerization process so
that IHC or immunofluorescence staining can be conducted
for biomarkers. As I understand, it the heat in the
polymerization exothermic reaction may destroy destroy
the antigens. I assume that the plastic requires
pretreatment etching to expose the antigenic epitopes.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 20 09:36:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

What are the makes of ultramicrotomes currently on the market and what is the consensus about them? I'm aware of RMC (Boeckeler) and Leica. I'm helping a colleague equip her new lab and she needs to submit three bids.

Thank you very much,

Jaclynn Lett
Senior Research Technician, EM Core Facility
Washington University School of Medicine
Department of Otolaryngology
660 South Euclid Ave., Box 8115
St. Louis, MO 63110

email: lettj-at-ent.wustl.edu

Note: NEW PHONE NUMBERS
voice: 314-747-7257
fax: 314-747-7230

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 20 13:33:59 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I would like to hear from anyone who may be able to help me find and
install a backscatter detector. Our SEM is a JEOL T-220A (built approx.
1987).

Tom Bargar
Core Electron Microscopy Research Facility
Univ. of Nebraska Medical Center
986395 Nebraska Medical Center
Omaha, NE 68198-6395
phone 402-559-7347
e-mail tbargar-at-unmc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 20 16:42:45 2004

Contents Retrieved from Microscopy Listserver Archives
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Robert,
In my lab, we have had very good luck using
butyl-methyl-methacrylate for immuno work. It is polymerized by UV at
4 C, minimizing the heat problem you mentioned, and after sectioning,
the resin can be removed with 10 min in acetone. We also include
dithiothreitol (DTT) in the resin which also seems to keep those
antigens nice and perky. You can find results and information in 1992
Planta 187: 405 - 413. and in 1997 Plant Physiology 115: 101 - 111.
If you are interested, I'll be happy to send you a detailed protocol
and discuss technical stuff. Caveat: I work on plants and have no
idea about the metal stent issue. My answer speaks only for a
generally useful resin for immnocyt.

Hope thise helps,
tobias
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (rgr-at-georgetown.edu) from
} http://www.msa.microscopy.org/Ask-A-Microscopist/Ask-A-Microscopist.html
} on Thursday, August 19, 2004 at 08:41:36
} ---------------------------------------------------------------------------
}
} Email: rgr-at-georgetown.edu
} Name: Robert Russell
}
} Organization: Georgetown University
}
} Education: Graduate College
}
} Location: Washington,District of Columbia, USA
}
} Question: I am seeking information about suitable resins/plastics in which to
} embed metal stents and similar devices and then
} conduct imunohistochemistry staining for biomarkers
} in the surrounding tissues - i.e. artery and soft tissue.
} This nquiry is about suitable protocols/experience
} of plastics or other embedding methods that preserve
} the antigens during the polymerization process so
} that IHC or immunofluorescence staining can be conducted
} for biomarkers. As I understand, it the heat in the
} polymerization exothermic reaction may destroy destroy
} the antigens. I assume that the plastic requires
pretreatment etching to expose the antigenic epitopes

From MicroscopyL-request-at-ns.microscopy.com Sat Aug 21 18:25:21 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi!

I need som advice about BEEM capsules for LR White embedding.

I am developing a work where I want to do both LM and TEM studies.

First I will include material about 8mm (or maybe a little more) diameter
(or major axis measure) in LR White, then I want to look at H&E sections
in order to select an area for appropiate preparation for TEM and
Immunocytochemical analysis.

I am not finding an appropiate BEEM capsule (or equivalent) to include
material without oxygen penetration. I need a capsule which prevent oxygen
penetration and with both flat ends (Top and bottom), not the usual
conical or pyramid end shapes we usually see in standard BEEM capsules
(excellent when the only concern is TEM).

It doesn´t matter if if square or cylindrical what matters is its flat end
for appropiate inclusion of my material.

I´d like to hear suggestion from those of you who might already developed
similar studies.
Does anyone know a supplier(s) where I can get such capsules?

As for LR White polymerization, I only can use an oven so I pretend to
work with 55-60°C. I have no access to ultraviolet.

I'd appreciate both list replies or private ones
(silvia_nit200-micro-at-yahoo.com.br)

Thanks,
Silvia E. Navas

__________________________________________________
Do You Yahoo!?
Tired of spam? Yahoo! Mail has the best spam protection around
http://mail.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Sat Aug 21 21:51:20 2004

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Hi, Tom

I suppose you've explored the 3rd-party manufacturers, like Oxford Intruments's Tetra,
and GW Electronics.

I don't know your model, but if JEOL ever made one for it, that may be your best bet, at
least for the actual detector, because you know that their one will actually fit without
compromising anything else. The signal-processing electronics is relatively easy.

I fooled around once with bits of solar cell, but it didn't get anywhere close to as good as
the JEOL one for my old JXA-5A.

good luck

rtch

}
}
} I would like to hear from anyone who may be able to help me find and
} install a backscatter detector. Our SEM is a JEOL T-220A (built
} approx. 1987).
}
} Tom Bargar
} Core Electron Microscopy Research Facility
} Univ. of Nebraska Medical Center
} 986395 Nebraska Medical Center
} Omaha, NE 68198-6395
} phone 402-559-7347
} e-mail tbargar-at-unmc.edu
}
}

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Sat Aug 21 23:54:29 2004

Contents Retrieved from Microscopy Listserver Archives
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I used to cut the tips off the BEEM capsules and place an extra cap
on the cut end. This would give me a cylinder with two end caps. The
block would be a little shorter than the standard capsule. Would
that work for you?

Joel

Date sent: Sat, 21 Aug 2004 20:47:52 -0300 (ART)
} From: {silvia_nit2000-micro-at-yahoo.com.br}
Send reply to: silvia_nit2000-micro-at-yahoo.com.br

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (popco-at-toast.net) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Sunday, August 22, 2004 at 23:36:12
---------------------------------------------------------------------------

Email: popco-at-toast.net
Name: Lloyd McClure

Education: Undergraduate College

Location: White City, OR

Question: Hi,
I just picked up a 2X Bausch microscope of unknown age numbered 312684119.
I have a set of 10X WF eyepieces and would like to know if higher
magnification eyepieces were made for this model and if so, where I
might buy them.
Thanks,
Newbie, Mac McClure

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 00:24:04 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (zerfasp-at-ors.od.nih.gov) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Sunday, August 22, 2004 at 14:06:24
---------------------------------------------------------------------------

Email: zerfasp-at-ors.od.nih.gov
Name: Patricia Zerfas

Organization: NIH

Title-Subject: [Microscopy] [Filtered] MListserver: Lactoferrin gold

Question: Does anyone know of a source for lactoferrin gold? It was
once manufactured by Sigma and was discontinued. I am willing to pay
for the lactoferrin gold and shipping.

Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 02:48:19 2004

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} Sylvia,
} You can try gelatin capsules of the bigger size,
of course both the
ends are not going to be flat, other option is to try
getting plastic
stoppers for bottles which come in various sizes and
can be used as
mould, unless polymerization has to be done in
airtight capsules.
} regards
} shashi
} CCMB Hyderabad
} INDIA

_______________________________
Do you Yahoo!?
Win 1 of 4,000 free domain names from Yahoo! Enter now.
http://promotions.yahoo.com/goldrush

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 02:47:53 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

} Sylvia,
} You can try gelatin capsules of the bigger size,
of course both the
ends are not going to be flat, other option is to try
getting plastic
stoppers for bottles which come in various sizes and
can be used as
mould, unless polymerization has to be done in
airtight capsules.
} regards
} shashi
} CCMB Hyderabad
} INDIA

_______________________________
Do you Yahoo!?
Win 1 of 4,000 free domain names from Yahoo! Enter now.
http://promotions.yahoo.com/goldrush

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 06:07:17 2004

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Re LR White embedding temperature. We can polymerise our
blocks at a tlower temperature - 50 degrees for 48hrs.

Dave

On Sat, 21 Aug 2004 20:47:52 -0300 (ART)
silvia_nit2000-micro-at-yahoo.com.br wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi!
}
} I need som advice about BEEM capsules for LR White embedding.
}
} I am developing a work where I want to do both LM and TEM studies.
}
} First I will include material about 8mm (or maybe a little more) diameter
} (or major axis measure) in LR White, then I want to look at H&E sections
} in order to select an area for appropiate preparation for TEM and
} Immunocytochemical analysis.
}
} I am not finding an appropiate BEEM capsule (or equivalent) to include
} material without oxygen penetration. I need a capsule which prevent oxygen
} penetration and with both flat ends (Top and bottom), not the usual
} conical or pyramid end shapes we usually see in standard BEEM capsules
} (excellent when the only concern is TEM).
}
} It doesn´t matter if if square or cylindrical what matters is its flat end
} for appropiate inclusion of my material.
}
} I´d like to hear suggestion from those of you who might already developed
} similar studies.
} Does anyone know a supplier(s) where I can get such capsules?
}
} As for LR White polymerization, I only can use an oven so I pretend to
} work with 55-60°C. I have no access to ultraviolet.
}
} I'd appreciate both list replies or private ones
} (silvia_nit200-micro-at-yahoo.com.br)
}
} Thanks,
} Silvia E. Navas
}
} __________________________________________________
} Do You Yahoo!?
} Tired of spam? Yahoo! Mail has the best spam protection around
} http://mail.yahoo.com
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 08:30:18 2004

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Greetings Everyone,

I would appreciate hearing from anyone who has had experience with field emission SEM both cold and thermal in regards to WDS. Also interested in some of the in lens detectors used for imaging. We are in the process of evaluating FESEM's to add to our laboratory. Please reply off line and if there is enough response I will summarize the information.

Thanks very much,

John Humenansky john.humenansky-at-guidant.com {mailto:john.humenansky-at-guidant.com}
Guidant Corporate Laboratory
4100 Hamline Ave. No.
St. Paul, MN 55117

651-582-6730

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 09:23:58 2004

Contents Retrieved from Microscopy Listserver Archives
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You can buy flat bottom polyethylene of polypropylene capsules through
Pelco (number 133 or 133-P) with an outside diameter of 7.9mm. That may
be big enough for your purpose. I have successfully used them for LR
White.

{} {} {} {} {} {} {} {} {} {}
Kim Rensing PhD
Research Associate
Wood Science, UBC
Vancouver BC, Canada
V6T 1Z4
{} {} {} {} {} {} {} {} {} {}

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 09:41:17 2004

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Hello to all on the listserv-

My boss asked me last week to start researching macrophotography
systems; I managed to turn up a few leads via Google, but it wasn't
much. For those of you who are using such a system, could you please
tell me about it? Which camera, what equipment, software,etc. And, most
importantly, what you like and don't like about it?

Thank you in advance for all your help-
Kathleen Roberts
Principal Lab Technician
Neurotoxicology Labs
Dept of Pharmacology & Toxicology
Ernest Mario School of Pharmacy
Rutgers University
41 B Gordon Rd
Piscataway, NJ 08854

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 10:19:59 2004

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Dear Sylvia,

We at TAAB Laboratories supply 8mm diameter polythene or polyethylene
capsules with a flat end (instead of the pyramid) and an air tight attached
lid as one of our standard products. Please contact us directly if you think
this may be of interest,

Best regards

Terry Cooper
TAAB Laboratories Equipment Ltd
3 Minerva House, Calleva Park
Aldermaston, Berks, RG7 8NA, England
Tel ++44 (0)118 981 7775 Fax ++44 (0)118 981 7881
e-mail sales-at-taab.co.uk
www.taab.co.uk

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 10:49:46 2004

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In a message dated 8/23/04 12:03:47 PM, kgrobert-at-rci.rutgers.edu writes:

} My boss asked me last week to start researching macrophotography
} systems; I managed to turn up a few leads via Google, but it wasn't
} much. For those of you who are using such a system, could you please
} tell me about it? Which camera, what equipment, software,etc. And, most
} importantly, what you like and don't like about it?

Whoa-- that's way to broad a question for any meaningful answers. What kind
of things are you trying to image - what sizes and particularly what heights
(relevant to the depth-of-field problem)? Are they colored and does reproducing
the color accurately matter? Are they shiny and reflective? Is the purpose to
document and build a file of images, or to make measurements, or to produce
good prints?

There are a lot of camera/software systems that can be used to do a good job
in the hands of someone who has built up some basic photography skills. I
happen to like the Nikon D70 myself, but mostly because I've used Nikons for a
long time and have a bunch of really good lenses. For someone else it might be a
poor choice. Software like Fovea is great for serious processing and
measurement but for some purposes just Photoshop is all you would need (probably it
will be basic to any digital imaging setup). And then there are printers - that
is a field unto itself. A lot of your problems will revolve around proper
lighting, rather than the camera/software choices.

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 12:55:29 2004

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In a message dated 8/23/04 1:44:08 PM, kgrobert-at-rci.rutgers.edu writes:

} Sorry for being so broad-I am a neophyte when it comes to this stuff.
}
} What we are trying to image: We are a university neurotoxicology lab that
} also serves
} as a general core facility for pathology, so we provide services in that
} area-necropsy,
} tissue fixation and processing into paraffin, microtomy, staining (anything
} from H&E to
} IHC) and likewise for TEM and LM. One of the things we would like to do
} is capture
} images of tumors or other pathology in mouse, rat, other animal species,
} etc. organs in
} situ during necropsies as necessary for research purposes. Size, heights
} and color
} will vary; they might be shiny if we wet them down with enough fixative
} to keep them
} moist. I assume that accurate reproduction of color would be necessary.
} The purpose
} here is to document pathology for both research and teaching purposes,
} so measurements
} and good prints would be necessary, and it would be great if we could build
} an archive
} of images.

If you have been doing your photography with film and are just trying to
switch to digital, there are a few things to consider:
1. depending on the camera body you select, you may be able to use your
existing macro lenses, ringlights, and other attachments. That's why I went with
the Nikon D70. It's a fine digital camera, but not the only good one. Take a
look at {http://www.dpreview.com/reviews/specs.asp} for good reviews on most of
the current models. You will certainly want a camera that accepts
interchangeable lenses, not one of the all-in-one models.
2. With that level of camera, you will be able to get the raw output rather
than being limited to a lossy-compressed jpeg image (you will NEVER want to use
jpeg). Photoshop CS will read the raw files and recover more than 8 bits -
sometimes as much as 10 - of data. That is important because with film the
dynamic range (brightness range) that can be handled is much greater than any
digital camera, and you want to capture as much as possible so that the highlights
don't blow out and the shadows plug and hide information (it's worse with
shiny specimens)
3. Check out ReindeerGraphics.com for their package deal on Fovea and
Optipix. The former is great for serious processing, color correction and
measurement. The latter has several tools for macrophotographry and comes with two books
- my "Photoshop for Digital Photographers" and George DeWolfe's guide to
workflow- that will help you to convert from film to digital.
4. If true color is important, you will almost certainly need to get a color
chart (e.g., see gretagmacbeth.com) to include in your scene, if not in every
picture then in every sequence under given lighting. Getting color right is
almost impossible without such a chart.
5. At some point, you will probably want to attend a workshop to pick up some
hands-on training and sharpen your skills. Skip the ones that are
Photoshop-centric - most of those folks are doing creative graphics. But there are still
lots of good choices (a hint - I teach several myself).
6. Before you start, sit down and think very hard about how you are going to
organize the images. There is nothing more frustrating when you have a huge
server or several dozen DVDs full of images and you know you've taken one of a
particular subject, but can't remember how to find it. Searching through the
thumbnails visually is practically worthless. If you use something like the
Photoshop catalog system, you will want to set up lists of keywords beforehand
that can be applied to images in order to make searching more efficient.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 13:02:30 2004

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Workshop Announcement
University of California at Santa Barbara

The Department of Molecular, Cellular, and Developmental Biology and the
Neuroscience Research Institute are sponsoring an advance course on light
microscopy. This 5-day workshop will be offered from September 13 through
September 17, 2004 and will consist of lectures and laboratory exercises
that will run from 9 am to approximately 5 pm each day. The seminar/workshop
will be intensive enabling participants to develop theoretical and hands-on
expertise with light microscopes. Attendees will interact closely with the
instructors while using modern research grade microscopes, cameras, and
computers. The seminars and laboratories will cover basic optical theory and
how it pertains to increasing contrast (signal to noise ratio) in biological
samples. Fundamental techniques such as fluorescence, phase contrast,
Nomarski differential interference contrast, and darkfield imaging will be
taught and attendees will use microscopes equipped with these optical
enhancement accessories. In addition, the theory and practice of electronic
image acquisition (analog and digital) will be discussed and attendees will
work with low-light cameras, digital image processing computers, and
morphometric programs. There are five research grade microscopes, five
electronic imaging cameras, two computer workstations, and one confocal
microscope. With a maximum enrollment of 10 students, there will be ample
opportunity to work with all of the microscopes and cameras. For those so
interested, intensive hands-on instruction and guidance on the confocal
microscope will be provided.

For a fuller description of the workshop, please check the web address
below. Enrollment forms can be completed online and this workshop provides
an opportunity to have a working-vacation in Santa Barbara, California.

http://www.lifesci.ucsb.edu/mcdb/events/events.html

Brian Matsumoto
Adjunct Associate Professor
Dept. MCDB, Neuroscience Research Institute
UCSB
Santa Barbara, CA 93106

voice mail 805-893-8702
FAX 805-893-2005

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 13:33:11 2004

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I'm not sure what you understand by "macrophotgraphy", particularly
what size object do you want to image full frame.

I've recently used a Nikon Coolpix 8700 (8MB chip, with "macro"
capability), and am not impressed by its performance in close range
(down to approx 2 inches, 5 cm). Depth of field is limited by the max
f-stop of f/8, the built in flash produces a shadow against the
extended lens (even when using the longest macro-allowable focal
length of the zoom), TTL flash exposure compensation does not work at
all (continuous light exposure comp works), and yellow color
overexposes regardless of exposure compensation settings, autofocus
has problems in close range, and there is too little detail on the
LCD screen to allow accurate manual focusing. Although the 8700 is
good for overall scenes (RAW, TIF files), macro capabilities are
disappointing.

I would recommend to use a camera with optical-glass viewfinder (not
a LCD screen) for accurate manual focusing, test the TTL-flash
exposure compensation regardless of manufacturer's claims. Consider
also bellows head lenses; Zeiss Luminars can be obtained on the
second hand market, and some manufacturer's still produce new ones
(Minolta, Olympus, I think). The smaller diameter thread mount makes
them interchangeable between systems, and the narrow diameter of the
lens barrel allows for more freedom in lighting. Depending on
magnification, get a lens with decent f-stop range. Note, that
cranking down the f-stop at higher mag (} 2:1) may cause image
degradation due to diffraction. See Sydney Ray's excellent tome
"Applied Photographic Optics" now in the 3rd edition for details; all
the personal feel, final magnification dependence, aperture blade
numbers.

I use a Contax RTS III with Contax bellows, that allow to place the
focal plane at an angle to the film plane (shift/tilt or PC bellows)
to approx 3.5:1 with a 100 mm Macro (i.e. approx. 8 mm full frame),
or the 50/1.4 reversed a bit higher. It is a film camera, but the
Carl Zeiss optics are wonderful. Some of the older bellows by Nikon
and Minolta also are PC capable, but I am not sure whether they
accept any of the new digital bodies.

RAW files are nice as they are 16 bit/channel, but they are
agonizingly slow to open. The 12 MB RAW/NEF files from the Nikon 8700
takes about 2 minutes to process on a 1 GHz Mac G4. Writing the RAW
files to a 1GB flash card also takes a while, say 20-30 seconds.

Best wishes Daniel

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
***************************************************************************************

Daniel L. Geiger, Ph.D.
Research Associate Santa Barbara Museum of Natural History
Adjunct Assistant Professsor, University of Southern California, Los Angeles

Mailing Address:
Molecular Systematics Lab, Natural History Museum of Los Angeles County
900 Exposition Blvd., Los Angeles, CA 90007, USA
phone: (213) 763 3431 fax: (213) 748 4432
NEW e-mail geiger-at-vetigastropoda.com
NEW www http://www.vetigastropoda.com

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 14:09:57 2004

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I need a mercury arc source for a Zeiss Axiovert 100. I have an old
Olympus power supply for a 100W mercury burner. Does anyone have any
idea whether it would be possible to buy a Zeiss 50 or 100W lamp
house and wire the Olympus supply to drive it? Thanks- Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 15:54:16 2004

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Adapting a good simple lens such a Zeiss Tessar or Kodak Extar with
as few surfaces and good color correction to a digital camera will
give the best images. Trying to use the photube of stereo microscope
is a bit handier but requires a very good stereo microscope to get
as sharp and high a contrasts images as a old coated cine lens off
ebay. While not as good as the f 6.3 reversed this 45 mm 2.8 Zeiss
Tessar http://www.surplusshed.com/detail.cfm?ID=L2158 sould do a
pretty good job on a digal back at 1 to 1 work. If it was stopped
down to F 8 or f 16. The focal length is a bit long for more
magification.

A Nikon CoolPix with Mark Simmons adapter
http://www.perspectiveimage.com/ and a reversed cine lens work very
well. As does his short tube microscope and good 1x to 4x objective
or Micro Tessars with the eyepice to make the work wiht the lens in
the coolpix. The quality of the objective really shows here. In
http://www.microscopy-uk.org.uk/mag/indexmag.html?http://www.microscopy-uk.org.uk/mag/artjan03/gcshorttube.html
the 12.5 Leitz Photar and Leitz 1x Plan did much better work than
the regualy objectives that I used. The sharpness of the Photar was
really noticable.

A better choice would be a camera with a removable lens or a digital
back for 4 x5 camera. so you would have full movements of the view
camera and a larger chip area.

The lighting is an area that requires a lot of attention as well. I
prefer fiber optics and several of them for control in small areas.
I also use a good deal of electronic flash slaved to the camera.

Gordon
Gordon Couger

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

----- Original Message -----
} From: "Kathleen Roberts" {kgrobert-at-rci.rutgers.edu}
To: {Microscopy-at-microscopy.com}
Sent: Monday, August 23, 2004 10:13 AM

I've been using a Nikon D1, D100 and D70 and must say that their
performances are quite close to eachother, nevertheless the price. Be aware
that TTL is not always available, eg. not only when working in manual
position you'll have problems, also in the aperture-stand (where you choose
the aperture), you might have overexposed images!

Major thing about the D70 is its price, highly competitive concerning
price/quality compared to others. Negative points: no TIFF available, only
RAW and three JPEG-values (high, medium, low compression) in 3 modes: low,
medium and high resolution. When obtaining for the RAW-file (non-compressed
JPEG at high resolution is enough for high quality printing in the
advertisement-world!), also take in account that the setup of a RAW-file
with the D100 is not the same as with the D70 (i.e. a program that can read
RAW-files from a D100 therefor is not capable of reading the RAW-file from a
D70).

The D1 on the other hand I find outdated, big, heavy, not very user-friendly
and still pricy, where a D70 costs about 1000 euro, a D1 still costs
something like 3000 euro.

My opinion, take in account the Nikon D100. It's a little heavier and
bigger than a D70, allthough not much, offers you the same capabilities, but
also the TIFF-format, which you will be using greatfully! JPEG's are very
nice for regular photography and morphometry, except if intensity and
color-definition is important, here a TIFF will offer you more. RAW is not
always better (in most cases, a TIFF-file has more data in it's pixels than
a RAW-file, allthough this is generally not known nor accepted, check the
digital photography-books and magazines for comprovement!).

A Nikon D100 you'll have for about 1400 euro without objective, a Nikon D70
for 1000 euro (also without objective), but the 400 euro make a difference.
When obtaining an objective (macro!), choose also a Nikon! The difference
in definition of your images is very big, and you will regret the day you
bought an objective from another, cheaper, brand and not one from a known
brand! You'll see the difference in definition, especially when zooming in
to look at the small details (not even talking about aberations and
color-shifts)!
I hope I helped you out a little more concerning Nikon, but it does not mean
that other brands as Canon cannot give you the same! I do not have anything
to do with Nikon, just that I've always been using them in the lab (also in
combination with Zeiss stereomicroscopes (great photo's!) and for personal
use: vacations, macro-photography of mushrooms etc... Good luck!

Sven Terclavers

-----Original Message-----
} From: Daniel Geiger [mailto:geiger-at-vetigastropoda.com]
Sent: Monday, August 23, 2004 20:55
To: kgrobert-at-rci.rutgers.edu; Microscopy-at-microscopy.com

I'm not sure what you understand by "macrophotgraphy", particularly
what size object do you want to image full frame.

I've recently used a Nikon Coolpix 8700 (8MB chip, with "macro"
capability), and am not impressed by its performance in close range
(down to approx 2 inches, 5 cm). Depth of field is limited by the max
f-stop of f/8, the built in flash produces a shadow against the
extended lens (even when using the longest macro-allowable focal
length of the zoom), TTL flash exposure compensation does not work at
all (continuous light exposure comp works), and yellow color
overexposes regardless of exposure compensation settings, autofocus
has problems in close range, and there is too little detail on the
LCD screen to allow accurate manual focusing. Although the 8700 is
good for overall scenes (RAW, TIF files), macro capabilities are
disappointing.

I would recommend to use a camera with optical-glass viewfinder (not
a LCD screen) for accurate manual focusing, test the TTL-flash
exposure compensation regardless of manufacturer's claims. Consider
also bellows head lenses; Zeiss Luminars can be obtained on the
second hand market, and some manufacturer's still produce new ones
(Minolta, Olympus, I think). The smaller diameter thread mount makes
them interchangeable between systems, and the narrow diameter of the
lens barrel allows for more freedom in lighting. Depending on
magnification, get a lens with decent f-stop range. Note, that
cranking down the f-stop at higher mag (} 2:1) may cause image
degradation due to diffraction. See Sydney Ray's excellent tome
"Applied Photographic Optics" now in the 3rd edition for details; all
the personal feel, final magnification dependence, aperture blade
numbers.

I use a Contax RTS III with Contax bellows, that allow to place the
focal plane at an angle to the film plane (shift/tilt or PC bellows)
to approx 3.5:1 with a 100 mm Macro (i.e. approx. 8 mm full frame),
or the 50/1.4 reversed a bit higher. It is a film camera, but the
Carl Zeiss optics are wonderful. Some of the older bellows by Nikon
and Minolta also are PC capable, but I am not sure whether they
accept any of the new digital bodies.

RAW files are nice as they are 16 bit/channel, but they are
agonizingly slow to open. The 12 MB RAW/NEF files from the Nikon 8700
takes about 2 minutes to process on a 1 GHz Mac G4. Writing the RAW
files to a 1GB flash card also takes a while, say 20-30 seconds.

Best wishes Daniel

} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
****************************************************************************
***********

Daniel L. Geiger, Ph.D.
Research Associate Santa Barbara Museum of Natural History
Adjunct Assistant Professsor, University of Southern California, Los Angeles

Mailing Address:
Molecular Systematics Lab, Natural History Museum of Los Angeles County
900 Exposition Blvd., Los Angeles, CA 90007, USA
phone: (213) 763 3431 fax: (213) 748 4432
NEW e-mail geiger-at-vetigastropoda.com
NEW www http://www.vetigastropoda.com

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 16:06:43 2004

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As far as I understand, BEEM capsules (at least original ones) are not good
for LR White. Don't ask me why, it's a mystery! 8 mm also looks like too
big to fit a standard ultratome holder. I had similar problem previously
doing EM on 0.2 mm mouse brain slices. I solved it by flat embedding of
the brain slices in LR White (between two sheets of polypropylene) and then
gluing the sample to the standard post with epoxy. Gluing appeared to be a
problem - it seems to me that LR White at high humidity adsorbs water and
do not stick well to the posts... Otherwise, it was working quite well.
Additional reason to do flat-embedding is because such large (8 mm) samples
tends to be curved, so I actually straighten them between two
polypropylene sheets with some force. You need to understand that plastic
will not polymerize at the edges, so sheets should be much bigger than your
sample.
I hope it may help. Sergey

At 08:47 PM 8/21/2004 -0300, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 16:13:12 2004

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Kathleen,

I agree with most of what John says in his posting. A couple of things I
would like to add:

1) You may want to check out if a "copystand" or some other device that lets
you set up more consistent illumination and imaging conditions is the right
thing to use. this would also allow you to apply correct calibrations to
your images. Call me if you have any questions.

2) I would also consider a microscope camera with live imaging on the
computer screen. That way it is a lot easier to adjust lighting or exposure
to avoid reflections and/or dark areas.

3) Photoshop is certainly a capable application. However, you may want to
investigate other software that is geared more towards microscopy. You may
want to use the same software for microscopes as well, and then other
software might be better suited. You can start by looking at our website,
but there are other vendors as well.

4) I could not agree more with John regarding cataloging the images. Again,
I think you can do better than Photoshop, especially when it comes to
automatically reading parameters from microscopes, etc.

5) From your address I see that your work is related to Pharma. I don't know
if FDA rules apply to your work, but if so, make sure that the software you
use is Rule 11 compliant. There is a good chance that you don't need this,
but I'd make sure. Again, you can check our web site for more information.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Monday, August 23, 2004 12:17
To: kgrobert-at-rci.rutgers.edu; microscopy-at-microscopy.com

In a message dated 8/23/04 1:44:08 PM, kgrobert-at-rci.rutgers.edu writes:

} Sorry for being so broad-I am a neophyte when it comes to this stuff.
}
} What we are trying to image: We are a university neurotoxicology lab that
} also serves
} as a general core facility for pathology, so we provide services in that
} area-necropsy,
} tissue fixation and processing into paraffin, microtomy, staining (anything
} from H&E to
} IHC) and likewise for TEM and LM. One of the things we would like to do
} is capture
} images of tumors or other pathology in mouse, rat, other animal species,
} etc. organs in
} situ during necropsies as necessary for research purposes. Size, heights
} and color
} will vary; they might be shiny if we wet them down with enough fixative
} to keep them
} moist. I assume that accurate reproduction of color would be necessary.
} The purpose
} here is to document pathology for both research and teaching purposes,
} so measurements
} and good prints would be necessary, and it would be great if we could build
} an archive
} of images.

If you have been doing your photography with film and are just trying to
switch to digital, there are a few things to consider:
1. depending on the camera body you select, you may be able to use your
existing macro lenses, ringlights, and other attachments. That's why I went
with
the Nikon D70. It's a fine digital camera, but not the only good one. Take a

look at {http://www.dpreview.com/reviews/specs.asp} for good reviews on most
of
the current models. You will certainly want a camera that accepts
interchangeable lenses, not one of the all-in-one models.
2. With that level of camera, you will be able to get the raw output rather
than being limited to a lossy-compressed jpeg image (you will NEVER want to
use
jpeg). Photoshop CS will read the raw files and recover more than 8 bits -
sometimes as much as 10 - of data. That is important because with film the
dynamic range (brightness range) that can be handled is much greater than
any
digital camera, and you want to capture as much as possible so that the
highlights
don't blow out and the shadows plug and hide information (it's worse with
shiny specimens)
3. Check out ReindeerGraphics.com for their package deal on Fovea and
Optipix. The former is great for serious processing, color correction and
measurement. The latter has several tools for macrophotographry and comes
with two books
- my "Photoshop for Digital Photographers" and George DeWolfe's guide to
workflow- that will help you to convert from film to digital.
4. If true color is important, you will almost certainly need to get a color

chart (e.g., see gretagmacbeth.com) to include in your scene, if not in
every
picture then in every sequence under given lighting. Getting color right is
almost impossible without such a chart.
5. At some point, you will probably want to attend a workshop to pick up
some
hands-on training and sharpen your skills. Skip the ones that are
Photoshop-centric - most of those folks are doing creative graphics. But
there are still
lots of good choices (a hint - I teach several myself).
6. Before you start, sit down and think very hard about how you are going to

organize the images. There is nothing more frustrating when you have a huge
server or several dozen DVDs full of images and you know you've taken one of
a
particular subject, but can't remember how to find it. Searching through the

thumbnails visually is practically worthless. If you use something like the
Photoshop catalog system, you will want to set up lists of keywords
beforehand
that can be applied to images in order to make searching more efficient.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 17:08:49 2004

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You can buy flat-bottomed capsules, most microscopy suppliers should have
them. For example, EMS
(http://www.emsdiasum.com/microscopy/products/catalog.aspx ) has them under
Specimen preparation.... Vials and sample storage. I used to use some from
TAAB a few years ago. Even if they aren't in the catalogue, many suppliers
can find them for you.

good luck,
Rosemary

No commercial affiliation, etc, etc

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

} From: shashi singh {shashis_99-at-yahoo.com}
} Date: Mon, 23 Aug 2004 01:09:51 -0700 (PDT)
} To: microscopy-at-msa.microscopy.com
} Cc: silvia_nit200-micro-at-yahoo.com.br
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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}
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-
}
}
} } Sylvia,
} } You can try gelatin capsules of the bigger size,
} of course both the
} ends are not going to be flat, other option is to try
} getting plastic
} stoppers for bottles which come in various sizes and
} can be used as
} mould, unless polymerization has to be done in
} airtight capsules.
} } regards
} } shashi
} } CCMB Hyderabad
} } INDIA
}
}
}
}
} _______________________________
} Do you Yahoo!?
} Win 1 of 4,000 free domain names from Yahoo! Enter now.
} http://promotions.yahoo.com/goldrush
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 22:35:46 2004

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Dear fellow microscopists,

I am looking for comments regarding a general protocol for DAB staining
for correlative light and TEM. I found a procedure of Essner (1973) that
uses 3% glut fixation, incubation in DAB for 2 hours, followed by 1%
hydrogen peroxide, subsequent washing steps, and incubation in buffered
KFeCN (3 mM) to eliminate non-specific adsorption of DAB. Samples are
further fixed with OsO4, dehydrated and embedded in epoxy resin.

I would like to hear tips from people who have success with this or
other DAB protocol for TEM. We are trying to visualize heme-containing
cytochromes in bacteria.

Many thanks in advance,
Alice.

Alice Dohnalkova
Research Scientist
Environmental Microbiology
Pacific Northwest National Laboratory
Richland, WA 99352
(509) 372-0692 office
(509) 376-3654 TEM lab

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 23 23:23:17 2004

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Hi, Kathleen,

I'd suggest you take a look at Microptics. They have a great system ...
fully integrated and very functional and cost-effective.

You should be able to find them on the web. If you can't, get in touch
with me offline and I'll find their info for you.

Caveat: MME has no financial interest in this company.

Good hunting

Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
At 10:13 AM 8/23/2004, Kathleen Roberts wrote:

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From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 00:15:18 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (wall1-at-llnl.gov) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Monday, August 23, 2004 at 11:08:27
---------------------------------------------------------------------------

Email: wall1-at-llnl.gov
Name: Mark A. Wall

Organization: LLNL

Title-Subject: [Microscopy] [Filtered] MListserver: CBED software

Question: I would like information on software (free or commercial)
for the simulation/comparison of HOLZ lines in CBED patterns. For
lattice parameter and strain measurements.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 03:54:32 2004

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: }
: } Hello to all on the listserv-
: }
: } My boss asked me last week to start researching macrophotography
systems;
: } I managed to turn up a few leads via Google, but it wasn't much.
For
: } those of you who are using such a system, could you please tell
me about
: } it? Which camera, what equipment, software,etc. And, most
importantly,
: } what you like and don't like about it?
: }
: } Thank you in advance for all your help-
: } Kathleen Roberts
: } Principal Lab Technician
: } Neurotoxicology Labs
: } Dept of Pharmacology & Toxicology
: } Ernest Mario School of Pharmacy
: } Rutgers University
: } 41 B Gordon Rd
: } Piscataway, NJ 08854
: }

Evaluate what you already have first. Particularly in skills.

If you set up a comprehensive faculty the camera is a small part of
the expense. A really good camera to build a versatile systems
hasn't really been made yet. The closest are the backs for 4X5
camera to use in existing set ups using lenses and lighting you
already have. A better choice would be a system that used a digital
camera that could use your existing 35 mm macro equipment. Most
reports are not very encouraging.

Jan Hinsch wrote about using a Digital SLR on a microscope for
McCrone's www.ModernMicroscopy.com
http://www.modernmicroscopy.com/main.asp?article=33 and was
satisfied. Ted Clarke discuses some of the issues of resolution of
digital image in the same online journal.
http://www.modernmicroscopy.com/main.asp?article=31

With a digital SLR the first problem all your lenses are twice the
effective size due to the smaller image area of the CCD. Other
problems include the inability to take long exposures, many cameras
can't lock the mirror up, problems with preview on some cameras and
mirror lock up. Mostly the cameras haven't evolved to the point that
the features need for macro work are available on enough cameras.
The lack of long exposure times is a problem with noise form heat
that can be solved by cooling the sensor or with software by adding
images.

Before you spend a lot of time on the project find out what they
mean by macro photography. If you are replacing a 4X5 with a full
set of Zeiss micro Tessars on a Leitz Astrophot stand with all the
nice lighting accessories that go with it and an operator that knows
how to use them a 4x5 digital insert for the camera will probably be
the way to go.

If you are starting from scratch and need to take product shots of
pills a good consumer camera may do the job with a careful selection
of lighting and backgrounds. I expect you application falls
somewhere in between. But getting the answer before you understand
the problem will most likely be time wasted.

Good luck
Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 04:39:43 2004

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Chair in Materials Science, Institute of Materials Science & Technology
(IMT), Friedrich-Schiller University (FSU) Jena, Germany

Postdoctoral research scientist or PhD student position (government
pay scale BAT-O IIa for initially 24 months, full time or part time,
depending on qualification, subject to approval of funds) to be filled
by 1. October 2004 in the research area:

Phase Boundaries of Proteins and Biomaterials

Aim of the project is an enhanced understanding of the interaction of
biological molecules or cells and different biomaterials.
The interest is in understanding the correlation between materials
structure and properties and the process of biological reactions, such
as blood coagulation or complement activation.
The ideal candidate for this position has sound experience in atomic
force microscopy (AFM) and is interested to work with TEM, CLSM, XPS
applied to biomaterials.
A background in one or more of the following areas is suitable:
physics, biophysics biomaterials, materials science, chemistry/polymer
chemistry, biology, engineering or related disciplines.

There are opportunities to co-operate with the members of the Start-up
Centre for Young Entrepreneurs at the department.
The group co-operates closely with other groups at the FSU, nationally
and internationally leading universities of the Anglo-American
countries as well as industrial partners.

Candidates for postdoctoral positions are requested to submit a
one-page research proposal.
Submit your full application, quoting ref. 34/04 including CV, photo,
research experience and qualifications and have two academic references
forwarded to

Prof. Dr. Klaus D. Jandt
(k.jandt-at-uni-jena.de)
Institute of Materials Science and Technology (IMT)
Friedrich-Schiller University Jena
Löbdergraben 32,
D-07743 Jena
Germany.

Closing date is 15. September 2004.

This is an unofficial, shortened translation of the German original
advertisement text which can be found at
http://www2.uni-jena.de/matwi/. This translation is not legally
binding.
http://www.uni-jena.de/matwi/

-----------------------------------------------------------------
Prof. Dr. Klaus D. Jandt
Chair in Materials Science
Director of Institute of Materials Science and Technology (IMT)
Friedrich-Schiller-University Jena
Löbdergraben 32
D-07743 Jena
Germany
Phone: ++ 49 3641 947730
Fax: ++ 49 3641 947732
Internet: K.Jandt-at-uni-jena.de

Visit us under http://www.uni-jena.de/matwi/

"Making Materials Science Work 4 U"

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 08:14:24 2004

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Mark,

check out our ASAC (Automatic Strain Calculation by CBED,
http://www.soft-imaging.com/rd/english/410.htm) product on our web site. It
is currently implemented for Si at various zone axes.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: wall1-at-llnl.gov [mailto:wall1-at-llnl.gov]
Sent: Monday, August 23, 2004 23:38
To: microscopy-at-ns.microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (wall1-at-llnl.gov) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Monday, August 23, 2004 at 11:08:27
---------------------------------------------------------------------------

Email: wall1-at-llnl.gov
Name: Mark A. Wall

Organization: LLNL

Title-Subject: [Microscopy] [Filtered] MListserver: CBED software

Question: I would like information on software (free or commercial)
for the simulation/comparison of HOLZ lines in CBED patterns. For
lattice parameter and strain measurements.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 13:32:24 2004

Contents Retrieved from Microscopy Listserver Archives
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We recently purchased a used Hitachi H7000 (without manuals,
schematics, etc.) and have a question related to magnification.

Does the H7000 generate a magnification marker bar on the negative?
If so, how is this activated from the menu?

Thanks very much.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 16:32:05 2004

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Dear All,

I have need to automate the Z axis on our JEOL JSM-6400 stage (same as
840). At one time JEOL made an automated Z-axis system that they
installed on the JXA-840 systems. Follow this link to see a few images
of this assembly.

http://www.mse.mtu.edu/~opmills/zaxis.htm

Do you have this part in a drawer or cabinet somewhere? I am seeking
to buy or have this part donated.

Please reply to me if you have this part or know one's whereabouts.

Thanks!

Owen

Owen P. Mills
Electron Optics Engineer
Applied Chemical & Morphological Analysis Laboratory
Materials Science & Engineering
Michigan Technological University
Rm 512 M&M Bldg.
Houghton, MI 49931
PH 906-369-1875
FAX 906-487-2934
mailto:opmills-at-mtu.edu
http://www.mm.mtu.edu/~opmills

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 24 16:53:13 2004

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Does anyone have experience with the EXFO X-cite 120 light source for
fluorescence microscopy? THanks-Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 25 02:13:51 2004

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Greetings All,

After many years of faithful service an old Sony CCD has passed on. It was
used on a Zeiss Stemi SV-11 and images were captured on a MAC G4 running OS
8.6, via Photoshop 5.5 using Import/Export plugins.

Can anyone recommend a camera that would:
1. Fit on a Zeiss Stemi SV-11
2. Interface with a MAC (preferably via Firewire)
3. Interface with Photoshop
4. Include micron markers with the captured image

I realise that I will probably have to upgrade the OS and add some RAM.

Any suggestions would be greatly appreciated.

Regards
George

George Theodossiou
Physicist / Electron Microscopist

AMCOR Research and Technology
Ph: +61 3 9490 6135
Fax: +61 3 9499 4295
Mobile: 0409 568 840
email: George.Theodossiou-at-amcor.com.au

************************************************************************
CAUTION - This message may contain privileged and confidential
information intended only for the use of the addressee named above.
If you are not the intended recipient of this message you are hereby
notified that any use, dissemination, distribution or reproduction of
this message is prohibited. If you have received this message in error
please notify AMCOR immediately.
Any views expressed in this message are those of the individual sender
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From MicroscopyL-request-at-ns.microscopy.com Wed Aug 25 03:22:59 2004

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John

I'm afraid that the basic Hitachi H7000 doesn't generate a micron mark, although the STEM and SEM system does. I just checked a couple of old brochures and the micron mark capability seems to have come in with the H 7100.

Let me know if you need any help with the manuals or basic schematics for the H7000.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: "John J. Bozzola" {bozzola-at-siu.edu}

Our data collection contractor in Virginia has been instructed to close the
MT Salary and Equipment Usage Survey on September 1st.

This survey was mailed to nearly 17,000 MT subscribers in June and
handed-out in hard copy at the M&M meeting in Savannah.

If you have already sent your completed survey form to Virginia, thank you.
If you have been putting it off, please mail it in TODAY!

If you wish to remain anonymous, just fill in your home state so we can
report salary vs. state data.

The drawing for the hand-held TV prize will take place in the first week in
September. Naturally, we cannot award the prize to anonymous submissions.

If you live in the USA and Canada and want to participate, send me an email
and I'll fax you the survey plus the fax number of the data collection
contractor.

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 25 16:20:28 2004

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Greetings David,
Toludine blue and sodium borohydride are also commonly used quenching
agents where broadly emmitting background fluorescence is concerned.
Trypan blue is an acid dye and will bind positively charged moeties, and
toluidine blue is a basic stain known to bind negatively charged
substrates such as chromatin. The quenching idea simply involves
getting some chemical moiety to absorb the frequency being emmitted, a
solution of green absorbing fluorochrome such as rhodamine may do the
same thing without absorbing your illumination source as much (I'm
assuming these are adherent cells). I'm not entirely sure what sodium
borohydride does, but it is a popular method for quenching
autofluorescence in the presence of GFP.
One approach which might prove to be a more specific (and expensive)
system for quenching would involve the use of anti-FITC antibodies (I
believe Sigma carries them), although I'm not positive that the bound
anti-body will quench the fluorochome. Anti-fluorochrome antibodies
will quench some target fluorochromes. One could also label the FITC
targets with a different color fluorochrome through the use of
antibodies to FITC. The alternate fluorochrome or a gold conjugate may
be in close enough proximity for non-radiative transfer and subsequent
quenching to occur.
Regards,
Karl

David Knecht wrote:

}
}
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}
} Trypan quenching of fluroescence has been used for years to decrease
} fluorescence of particles and dextran. In our case, we are trying to
} use it to quench the fluorescence of surface labeled particles to
} distinguish internalized particles (phagocytosis) from external
} particles. We have not gotten significant quenching, and as I read
} the literature, I am unclear as to how this is supposed to work. In
} the original Hed paper that most people reference, they use FITC
} labeled particles and quench by putting the cells in a trypan solution
} in a pH 4.5 buffer. They describe this as a FRET type quenching to a
} non-radiative acceptor. Trypan does emit, but lets leave this aside
} for now. Their explanation makes little sense to me since with the
} known pH dependence of FITC, it seems to me they are doing primarily
} pH based quenching as opposed to FRET based quenching. If so, then
} are they simply looking at the difference in FITC fluorescence between
} the phagosomal pH (5.5) and the external pH (4.5)?
} In other papers, rhodamine labelled particles are used, and trypan
} quenching is also supposed to work, however in our case, we can only
} see about 50% quenching. Given how opaque the solution is, I could
} easily see that being a case of simply decreasing both excitation and
} emission due to opacity of the solution. In some cases (yeast
} particles) I have been told that the trypan actually binds to the
} particles so that you can wash it out and the particles are still
} blue, and in that case, I would imagine very different quenching
} properties, since the trypan is no longer freely diffusing in
} solution. I have yet to find literature that clearly investigates the
} quenching phenomenon with different fluors under solution vs. bound
} conditions. Can anyone help? Thanks- Dave

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 25 17:55:46 2004

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Dear colleagues
I am looking for simple sign-in calendar software (preferably freeware), so
users could sign-in for the instruments on the WEB. I expect this software
should work on my server (windows based) and provide easy way to sign-in,
sign-out for users for the different instruments. I do remember, this
issue was discussed on the server a few years ago but I want to see what
people currently used. I was trying Google search and it was not so
productive: most links were addressed to the calendars hosted on the
Internet (like free E. mail accounts) or calendars for the business
(intranet). I would really appreciate your input. Have a great day
(night?). Sergey.

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Aug 25 19:55:54 2004

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Dear listers,
Does anyone have access to a set of schematics (11" x 17") for the Amray
1000? This is not the 1000B (and 1600 series) with the microprocessor-based
mag control, but the original 1000 with analog controls
We can copy and return originals or pay copy and shipping costs. Please
contact Earl Weltmer at: earlw-at-sbcglobal.net

Or me, below.

Thanks,

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

___________________________________________________________
$0 Web Hosting with up to 120MB web space, 1000 MB Transfer
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From MicroscopyL-request-at-ns.microscopy.com Wed Aug 25 23:08:29 2004

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Good to hear someone is still running a 1000, as we have not set ours up
yet, it and all the documentation is boxed up. I fear it may be behind a few
thousand pounds of boxes in the warehouse, but I can check on it. we ended
up with the unit from Honeywell computer plant here in phoenix.

It would be good to know who else out there is running one of these units. I
suspect we are a small group. Just have Amray in the title of the message
and it will catch my eye.

Thanks Ed Sharpe, Archivist for SMECC - - See the Museum's Web Site at
www.smecc.org

Coury House / SMECC
5802 W. Palmaire Ave. Phone 623-435-1522
Glendale Az 85301 USA
----- Original Message -----
} From: "Ken Converse" {kenconverse-at-qualityimages.biz}
To: "MSA Listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, August 25, 2004 6:18 PM

Hi,

I just would like to inform you that if you want to change
with Nikon D1, D100 or D70 from macroscopy to microscopy we
have camera adapters for SLR cameras and many other cameras
which fit for your microscope.

If you are interested let me know, I send you a camera list.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

ST} ------------------------------------------------------------------------------
ST} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
ST} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
ST} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
ST} -------------------------------------------------------------------------------

ST} I've been using a Nikon D1, D100 and D70 and must say that their
ST} performances are quite close to eachother, nevertheless the price. Be aware
ST} that TTL is not always available, eg. not only when working in manual
ST} position you'll have problems, also in the aperture-stand (where you choose
ST} the aperture), you might have overexposed images!

ST} Major thing about the D70 is its price, highly competitive concerning
ST} price/quality compared to others. Negative points: no TIFF available, only
ST} RAW and three JPEG-values (high, medium, low compression) in 3 modes: low,
ST} medium and high resolution. When obtaining for the RAW-file (non-compressed
ST} JPEG at high resolution is enough for high quality printing in the
ST} advertisement-world!), also take in account that the setup of a RAW-file
ST} with the D100 is not the same as with the D70 (i.e. a program that can read
ST} RAW-files from a D100 therefor is not capable of reading the RAW-file from a
ST} D70).

ST} The D1 on the other hand I find outdated, big, heavy, not very user-friendly
ST} and still pricy, where a D70 costs about 1000 euro, a D1 still costs
ST} something like 3000 euro.

ST} My opinion, take in account the Nikon D100. It's a little heavier and
ST} bigger than a D70, allthough not much, offers you the same capabilities, but
ST} also the TIFF-format, which you will be using greatfully! JPEG's are very
ST} nice for regular photography and morphometry, except if intensity and
ST} color-definition is important, here a TIFF will offer you more. RAW is not
ST} always better (in most cases, a TIFF-file has more data in it's pixels than
ST} a RAW-file, allthough this is generally not known nor accepted, check the
ST} digital photography-books and magazines for comprovement!).

ST} A Nikon D100 you'll have for about 1400 euro without objective, a Nikon D70
ST} for 1000 euro (also without objective), but the 400 euro make a difference.
ST} When obtaining an objective (macro!), choose also a Nikon! The difference
ST} in definition of your images is very big, and you will regret the day you
ST} bought an objective from another, cheaper, brand and not one from a known
ST} brand! You'll see the difference in definition, especially when zooming in
ST} to look at the small details (not even talking about aberations and
ST} color-shifts)!
ST} I hope I helped you out a little more concerning Nikon, but it does not mean
ST} that other brands as Canon cannot give you the same! I do not have anything
ST} to do with Nikon, just that I've always been using them in the lab (also in
ST} combination with Zeiss stereomicroscopes (great photo's!) and for personal
ST} use: vacations, macro-photography of mushrooms etc... Good luck!

ST} Sven Terclavers

ST} -----Original Message-----
} } From: Daniel Geiger [mailto:geiger-at-vetigastropoda.com]
ST} Sent: Monday, August 23, 2004 20:55
ST} To: kgrobert-at-rci.rutgers.edu; Microscopy-at-microscopy.com
ST} Subject: [Microscopy] Re: Digital Macrophotography

ST} ----------------------------------------------------------------------------
ST} --
ST} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
ST} To Subscribe/Unsubscribe --
ST} http://www.msa.microscopy.com/MicroscopyListserver
ST} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
ST} ----------------------------------------------------------------------------
ST} ---

ST} I'm not sure what you understand by "macrophotgraphy", particularly
ST} what size object do you want to image full frame.

ST} I've recently used a Nikon Coolpix 8700 (8MB chip, with "macro"
ST} capability), and am not impressed by its performance in close range
ST} (down to approx 2 inches, 5 cm). Depth of field is limited by the max
ST} f-stop of f/8, the built in flash produces a shadow against the
ST} extended lens (even when using the longest macro-allowable focal
ST} length of the zoom), TTL flash exposure compensation does not work at
ST} all (continuous light exposure comp works), and yellow color
ST} overexposes regardless of exposure compensation settings, autofocus
ST} has problems in close range, and there is too little detail on the
ST} LCD screen to allow accurate manual focusing. Although the 8700 is
ST} good for overall scenes (RAW, TIF files), macro capabilities are
ST} disappointing.

ST} I would recommend to use a camera with optical-glass viewfinder (not
ST} a LCD screen) for accurate manual focusing, test the TTL-flash
ST} exposure compensation regardless of manufacturer's claims. Consider
ST} also bellows head lenses; Zeiss Luminars can be obtained on the
ST} second hand market, and some manufacturer's still produce new ones
ST} (Minolta, Olympus, I think). The smaller diameter thread mount makes
ST} them interchangeable between systems, and the narrow diameter of the
ST} lens barrel allows for more freedom in lighting. Depending on
ST} magnification, get a lens with decent f-stop range. Note, that
ST} cranking down the f-stop at higher mag (} 2:1) may cause image
ST} degradation due to diffraction. See Sydney Ray's excellent tome
ST} "Applied Photographic Optics" now in the 3rd edition for details; all
ST} the personal feel, final magnification dependence, aperture blade
ST} numbers.

ST} I use a Contax RTS III with Contax bellows, that allow to place the
ST} focal plane at an angle to the film plane (shift/tilt or PC bellows)
ST} to approx 3.5:1 with a 100 mm Macro (i.e. approx. 8 mm full frame),
ST} or the 50/1.4 reversed a bit higher. It is a film camera, but the
ST} Carl Zeiss optics are wonderful. Some of the older bellows by Nikon
ST} and Minolta also are PC capable, but I am not sure whether they
ST} accept any of the new digital bodies.

ST} RAW files are nice as they are 16 bit/channel, but they are
ST} agonizingly slow to open. The 12 MB RAW/NEF files from the Nikon 8700
ST} takes about 2 minutes to process on a 1 GHz Mac G4. Writing the RAW
ST} files to a 1GB flash card also takes a while, say 20-30 seconds.

ST} Best wishes Daniel

} } ---------------------------------------------------------------------------
ST} ---
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

ST} --
ST} ****************************************************************************
ST} ***********

ST} Daniel L. Geiger, Ph.D.
ST} Research Associate Santa Barbara Museum of Natural History
ST} Adjunct Assistant Professsor, University of Southern California, Los Angeles

ST} Mailing Address:
ST} Molecular Systematics Lab, Natural History Museum of Los Angeles County
ST} 900 Exposition Blvd., Los Angeles, CA 90007, USA
ST} phone: (213) 763 3431 fax: (213) 748 4432
ST} NEW e-mail geiger-at-vetigastropoda.com
ST} NEW www http://www.vetigastropoda.com

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 06:55:25 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear vacationing listers,
Last night I posted a message. This morning I received 17 e-mails: 4 were
submissions to the list server, 3 were other e-mails and the following 10
were auto replies from the Listserver.

Mei Lie Wong [wong-at-msg.ucsf.edu]
moritz-andreas.meyer-at-amd.com
Oparowski, Joseph [Joseph_Oparowski-at-bose.com]
scosgrove [scosgrove-at-diaginc.com]
Rice, Trisha [TRice-at-FEICO.com]
Dunlap, Jonathan C. [Jonathan.Dunlap-at-sylvania.com]
Stewart Bean [bean-at-smt.zeiss.com]
rhumphre-at-ucalgary.ca
Postmaster-at-mxg.usuhs.mil
Mike Ingram [MIngram-at-rohmhaas.com]

Please read the rules of use. Please review Nestor’s many suggestions in
the archives. Please don’t just add to all the spam we all get.

Thank you for your consideration,

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

___________________________________________________________
$0 Web Hosting with up to 120MB web space, 1000 MB Transfer
10 Personalized POP and Web E-mail Accounts, and much more.
Signup at www.doteasy.com

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 08:50:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi Sergey,

I was looking for sign-up calendar software recently myself as we were
trying to set up on-line instrument reservation and most of what I found was
web calendar hosting service such as http://www.calendars.net/. I know that
some laboratories are using it and quite happy.

Our lab is using Calcium software from http://www.brownbearsoftware.com/
that we run from our own server. It is not free unfortunately, but except
for a few minor things we are quite happy with it. Contact me if you need
more feedback on Calcium.

Evgenia

====================================
Evgenia Pekarskaya
Keck Electron Microscopy Laboratory
University of Massachusetts, Amherst
Tel. 413 545 2261
E-fax 325 202 7338
pekarskaya-at-mail.pse.umass.edu
====================================

-----Original Message-----
} From: Sergey Ryazantsev [mailto:sryazant-at-ucla.edu]
Sent: Wednesday, August 25, 2004 7:19 PM
To: Microscopy-at-microscopy.com

Dear colleagues
I am looking for simple sign-in calendar software (preferably freeware), so
users could sign-in for the instruments on the WEB. I expect this software
should work on my server (windows based) and provide easy way to sign-in,
sign-out for users for the different instruments. I do remember, this
issue was discussed on the server a few years ago but I want to see what
people currently used. I was trying Google search and it was not so
productive: most links were addressed to the calendars hosted on the
Internet (like free E. mail accounts) or calendars for the business
(intranet). I would really appreciate your input. Have a great day
(night?). Sergey.

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 09:24:44 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

List,

As a result of a new instrument purchase, we are going to offer for sell our Scintag PadV X-ray Powder Diffraction System.

The system is configured with a vertical 2-Theta:Theta X-ray goniometer, high intensity Cu X-ray tube (replaced about 3 years ago), and a Kevex psi peltier cooled silicon detector. Automation and data collection is accomplished through a Compaq computer running Windows NT and the latest version of Scintag's DMSNT software including stress analysis.

Some spare parts will also be available with the system.

Contact me directly if you have an interest in this instrument.

Regards

Roy Beavers

Southern Methodist University
Department of Geological Sciences
P.O. Box 750395
Dallas, TX 75275
Voice: 214-768-2756
Fax: 214-768-2701
Email: rbeavers-at-mail.smu.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 11:11:32 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (ryan.davis-at-hydro.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on
Thursday, August 26, 2004 at 09:30:09
---------------------------------------------------------------------------

Email: ryan.davis-at-hydro.com
Name: Ryan Davis

Title-Subject: [Microscopy] [Filtered] MListserver: Unstable emission current

Question: Over the past couple of weeks I watched the emission
current on our Hitachi 3500N jump around like a dancing lady. I have
spoken with the service engineer, and he seemingly thinks dust might
be in the gun chamber. So, I wiped the gun chamber down using
Kimwipes and ethanol, and blew out the gun chamber out to remove any
fibers or debris left behind after cleaning. After cleaning I am
still having this problem. So, does anyone have any tricks for
removing dust?

} A list of things I have checked or replaced:

} Checked for whiskers on the filament. Saw none.
} Replaced filament. Emission current still unstable.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 13:24:30 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi All,

Do you know who is going to give up his ESEM E3?
Is there an ESEM E3 near Washington Thank you for
your help.

Tim
}
}
}
}
}
}
} __________________________________
} Do you Yahoo!?
} New and Improved Yahoo! Mail - 100MB free storage!
} http://promotions.yahoo.com/new_mail

} ATTACHMENT part 2 message/rfc822
} From: "Ken Converse" {kenconverse-at-qualityimages.biz}
} To: "MSA Listserver" {Microscopy-at-MSA.Microscopy.Com}
} Subject: [Microscopy] Amray 1000 schematics
} Date: Wed, 25 Aug 2004 21:18:03 -0400
}
}
}
}
------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------
}
} Dear listers,
} Does anyone have access to a set of schematics (11"
} x 17") for the Amray
} 1000? This is not the 1000B (and 1600 series) with
} the microprocessor-based
} mag control, but the original 1000 with analog
} controls
} We can copy and return originals or pay copy and
} shipping costs. Please
} contact Earl Weltmer at: earlw-at-sbcglobal.net
}
} Or me, below.
}
} Thanks,
}
} Ken Converse
}
} owner
} QUALITY IMAGES
} Servicing Scanning Electron Microscopes
} Since 1981
} 16 Creek Rd.
} Delta, PA 17314
} 717-456-5491
} Fax 717-456-7996
} kenconverse-at-qualityimages.biz
} qualityimages.biz
}
}
}
}
}
}
___________________________________________________________
} $0 Web Hosting with up to 120MB web space, 1000 MB
} Transfer
} 10 Personalized POP and Web E-mail Accounts, and
} much more.
} Signup at www.doteasy.com
}
}
}
}

__________________________________
Do you Yahoo!?
Yahoo! Mail - You care about security. So do we.
http://promotions.yahoo.com/new_mail

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 15:54:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Microscopists,

For a seminar about "Progress in imaging since Van Leeuwenhoeck", I'm
looking for:

Firstly: a photo (and description) of the largest microscope in the world
(it's dimensions, therefor not specifically it's magnification), and not the
particle accelerator of CERN in Swiss (since this is somehow also
'microscope').

Secondly: Websites with new achievements about imaging, here I mean new
technologies like EM, PET-scan, MicroCT, Synchrotron,... compared to normal
brightfield microscopy

Thanks a lot in advance!

Sven Terclavers

^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
Sven Terclavers
Life Science Imaging - Microscopy
Center for Transgene Technology & Gene Therapy - VIB
Campus Gasthuisberg O&N
Herestraat 49
3000 Leuven
Belgium
Tel.: +32 (0)16 34 61 73
Fax: +32 (0)16 34 59 90
Email: Sven.Terclavers-at-med.kuleuven.ac.be
Intranet: http://debian.med.kuleuven.ac.be
Internet: http://www.kuleuven.ac.be/mcm
^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^

From MicroscopyL-request-at-ns.microscopy.com Thu Aug 26 16:24:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Ryan,
Does the SE image change intensity with the emission current
fluctuations? If not, it could simply be a defective metering circuit. Or,
check the following:
1. Poor vacuum in the gun chamber - Are the walls of the gun chamber a
silver-blue color which wipes off easily with some acetone on a cloth? This
indicates a vacuum leak in the gun area, check your "O" rings for dirt, etc.
2. Remover your filament entirely, pump the SEM back down, turn on the HV
and run up the filament current knob to where your filament is normally
peaked and see if (A) you get an emission current above the normal "dark"
current and (B) does it still fluctuate. If the answer is no, I would
suspect vacuum. If Yes, then your gun may be contaminated, a bad HV cable,
or High Voltage Power Supply, or the emission (BIAS) circuit. If you HVPS
is an oil filled tank like the JEOL SEM's, the oil may be old and
contaminated and simply may need to be exchanged with fresh. Good luck!

Gary M. Easton
Scanners Corporation
Independent SEM Service, EDS and SEM Digital Imaging Sales
410-857-7633

----- Original Message -----
} From: "by way of MicroscopyListserver" {ryan.davis-at-hydro.com}
To: {microscopy-at-ns.microscopy.com}
Sent: Thursday, August 26, 2004 12:33 PM

Dear Ryan,
In addition to the suggestions you have already received, a couple of other
things you might check:
1. whiskers on the inside of the hole in the Wehnelt cap. It never hurts to
clean the Wehnelt, anode plate and check just under the anode plate for
contamination.
2. remove the Wehnelt and check the two little copper contacts in the gun
that the legs of the filament engage when you put the filament assembly into
the gun. Make sure they are firm, not bent or broken.
3. Make sure you are not putting the filament into the Wehnelt at right
angles to the proper direction. In my S-3000N, the legs of the filament must
line up with the notches in the Wehnelt, but with another, older Hitachi
SEM, they must be at right angles to the notches. Check your
filament-changing instructions in the manual.
I hope this helps.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "by way of MicroscopyListserver" {ryan.davis-at-hydro.com}
To: {microscopy-at-ns.microscopy.com}
Sent: Thursday, August 26, 2004 9:33 AM

I have received the following responses to my inquirey about care and sectioning of 17 year old paraplast blocks. I cannot begin to repay or even relate the help I have received through the Internet over the past five years or so on microscope issues. These replies are further evidence of the good will of microscopists everywhere. I don't mind expressing my gratitude to a friend, a microscopist who is a wealth of information and advice about every level of microscopy from the most primitive LM to the most advanced electronic varieties, who has offered to provide a microtome which is not being used, for which I will pay shipping. My benefactor, whom I am loathe to identify for fear of embarassing him, has made the use of a lonely phase contrast scope, several remarkable objectives, and other diverse parts available for my teaching and research.

Meanwhile, upon opening the box of wax blocks, I have found a number of slides of previously sectioned material that was not deparaffinized. I don't remember why, in the heat of the moment, when I was packing up to leave the laboratory where I'd been working, I made these particular sections.

Thanks to everyone who has offered advice, as follows:

Damian Neuberger Ph.D.:

Having made more Paraplast embeddings than I care to remember.....
The only thing I can think of is to keep them in a cool dry place;
otherwise, they should last a very long time. The other question
about how to section is an interesting one. You already have a hand
microtome and it might be worth a try although I don't know how it is
to be set up. You have a microtome blade but do you have a handle for
it? If not, it should be a low cost item to acquire and I have the
name of a local place that may have some.

I made a hand microtome using a screw type micrometer gauge, cutting
off the arch portion and mounting the screw portion to a steel
cylinder with a hole in it through which the screw part would push the
tissue sample out by a known amount. The top of the cylinder of
course was ground to a reasonably fine polish. The exposed sample was
then cut using a microtome blade on a handle. I used it primarily for
fresh plant samples that I would sandwich between some soft material
like balsa, or Sambucus pith, cork, etc before inserting it into the
hole.

} From: "Ray Hicks" {rayh-at-fcspress.com}

some plans are given here
http://www.microscopy-uk.org.uk/mag/art97b/microt.html
along the lines of damian's suggestion - if you don't want to destroy
a micrometer, you can buy the moving part (minus the frame) as a
separate component - this gives you a neat cylindrical stub that you
can insert into your tube, and hold it with a grub screw. This thing
is sold as a "micrometer head", slightly more expensive (Ł7.95) than a
micrometer (Ł6.95)
http://www.proopsbrothers.com/acatalog/
Online_Catalogue_Micrometers_54.html,
(this is the cheapest I can find them on the web btw, they range up to
250 pounds) but easier to handle I'm sure, also more reproducible than
the heated rod method (these are graduated in 10 micron steps, but you
can estimate smaller steps - although I imagine that the effect of
cutting will cause wedge-shaped sections unless the core you're
cutting is pretty much jammed in the barrel, I made something similar
to make plastic discs from teflon rod, and had to fit a friction screw
to stop the rod being dragged out of the tube by the force of cutting)

as an alternative, the shop at microscopy org has two microtomes (a
hand one -at- 32 pounds, and a rocking one -at- 120 pounds) that might just
be worth exploring... http://www.microscopy-uk.org.uk/full_shop.html

} From: {jb_sanderson-at-yahoo.com}

You are very unlikely to cut good sections on a hand
microtome, and the wax blocks will probably need
softening and then cutting very cold on a modern
microtome with sharp new Feather disposable blades. I
suggest that you try to contact your local
histopathology department for more help at your
hospital.

} From: "Michael Pendleton" {mpendleton-at-mic.tamu.edu}

While I worked at the USDA, I used paraplast blocks for thin
sectioning of insects which were about 10 years old and they still had
active peptides capable of immunocytochemical labelling. The sections
looked very good also. Perhaps it is more important that the
fixatives used worked well because it is probably unlikely that the
paraplast has deteriorated. My guess is the samples will work well if
they were well fixed.

Gordon Couger gcc-at-couger.com:

As a high school teacher in the Pacific you can probably get some
one to donate a microtome if you pay the freight. A wanted message
in the equipment exchange section of the MSA web page would be one
place and wanted messages are free on www.labx.com if you highschool
will give a letter to the person donating the micotome a letter for
a tax deduction it is probably worth more than a used microtome will
sell for.

Of course the freight is going to be a good deal of money on a
microtome.

Frederick Monson:

As far as preserving the blocks, there is only one thing that you will
have to insure. You must try to keep the blocks from temperatures
over 40 degrees C. In a black box, such outside temperatures can
become elevated and cause damage. On the other hand, as long as the
tissues/specimens remain enveloped in the paraffin, you can always
'trim' them out and re-block them before you are ready to section.

On Sat, 14 Aug 2004 17:35:22 +1000
"Alan E. Davis" {aedavis-at-eccomm.com} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I have just received a box full of wax blocks I made about 18 years ago for a study of reproductive biology and zooxanthellae of Millepora platyphylla, fire coral. I don't have a microtome, but thanks to the generosity of a microscopist cleaning out a lab, I have a steel microtome knife. I surely cannot afford a microtome, or especially the shipping, but I remember some plans from some discarded library material some years ago, for microtomes. One used a candle to heat a long metal rod, effectuating a gradual lengthening, for example.
}
} Can anyone suggest whether hand sections are worth while to try of wax blocks. The blocks were made with paraplast. Being several years old, even though I have to assume they are still ok, should I take any special steps with storage or rejuvenation?
}
} I'm afraid to ruin them. The study broke some ground, has not been published, and deserves to be followed through. Even though my notes have been lost through years of sore neglect, typhoons, and ex-spousal neglect, there are some hopeful clues in these specimens that would still be worthwhile, and dates of collection and other information are still recoverable for the most part, through existence of a parallel labelled collection of hard parts, with dates written on them. So... any suggestions on long term care of wax blocks, as well as suggestions for hand-sectioning, would be welcome.
}
} I have a hand microtome, with German inscriptions, that may be useful.
}
} Thank you,
}
} Alan Davis
} Kagman High School
} Saipan, N. Mariana Islands
} aedavis-at-eccomm.com
}

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 08:49:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We have an Amray 1000A currently in use. 1977 or 1978 vintage.
I assume that it is the model that you are referring to as
the "1000". As far as I know all the manuals, charts, etc. are still
in the cabinet
but we have not needed to refer to them in some time so I will check for you.
If you have already received the schematics please let me know.

Pat Connelly
Univ. of Pennsylvania, Dept. of Biology
Philadelphia, PA 19104-6018
215-898-7145

} ----- Original Message -----
} } From: "Ken Converse" {kenconverse-at-qualityimages.biz}
} To: "MSA Listserver" {Microscopy-at-MSA.Microscopy.Com}
} Sent: Wednesday, August 25, 2004 6:18 PM
} Subject: [Microscopy] Amray 1000 schematics
}
} } Does anyone have access to a set of schematics (11" x 17") for the Amray
} } 1000? This is not the 1000B (and 1600 series) with the
} } microprocessor-based
} } mag control, but the original 1000 with analog controls
} } We can copy and return originals or pay copy and shipping costs. Please
} } contact Earl Weltmer at: earlw-at-sbcglobal.net
} } Or me, below.
} }
} } Thanks,
} } Ken Converse
} }
} } owner
} } QUALITY IMAGES
} } Servicing Scanning Electron Microscopes
} } Since 1981
} } 16 Creek Rd.
} } Delta, PA 17314
} } 717-456-5491
} } Fax 717-456-7996
} } kenconverse-at-qualityimages.biz
} } qualityimages.biz
} } ___________________________________________________________
} Good to hear someone is still running a 1000, as we have not set ours up
} yet, it and all the documentation is boxed up. I fear it may be behind a few
} thousand pounds of boxes in the warehouse, but I can check on it. we ended
} up with the unit from Honeywell computer plant here in Phoenix.
}
} It would be good to know who else out there is running one of these units. I
} suspect we are a small group. Just have Amray in the title of the message
and it will catch my eye.

} Thanks Ed Sharpe, Archivist for SMECC - - See the Museum's Web Site at
} www.smecc.org
}
} Coury House / SMECC
} 5802 W. Palmaire Ave. Phone 623-435-1522
Glendale Az 85301 USA

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 13:33:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (watson-at-wi.mit.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday, August 27, 2004 at 10:20:20
---------------------------------------------------------------------------

Email: watson-at-wi.mit.edu
Name: Nicki Watson

Organization: Whitehead Institute

Title-Subject: [Microscopy] [Filtered] MEM training schools

Question: Hi all,
I am trying to find the name and web site of the two schools that
offer an associate degree in electron microscopy.
I believe there is one on the west coast, and one in the mid west.
I met a few of the students from those schools at the recent meeting
in Savannah, and I would like to get some more information about
their program, and possibly submit a want ad to their placement
department.
If anyone knows of these schools please let me know.
Thanks
Nicki Watson

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 15:14:08 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Aug 27, 2004, at 11:56 AM, by way of MicroscopyListserver wrote:

} I am trying to find the name and web site of the two schools that
} offer an associate degree in electron microscopy.
} I believe there is one on the west coast, and one in the mid west.
} I met a few of the students from those schools at the recent meeting
} in Savannah, and I would like to get some more information about their
} program, and possibly submit a want ad to their placement department.
} If anyone knows of these schools please let me know.
}
Dear Nicki,
Delta College is probably the West Coast school you have in mind. It
was run by Judy Murphy for a long time. I do not know the present
situation with that program, since Judy is no longer affiliated with
it; however, up until Judy left, it was an excellent program, and I
would be certain that any graduate of that program would be exceedingly
well trained.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 16:53:52 2004

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Nicki:

The training schools are as follows:

Madison Area Technical College
http://matcmadison.edu/electronmicros/

San Joaquin Delta College
http://www.deltacollege.edu/dept/electmicro/index.html

We have hired people from both places and have been very pleased with
the quality of students they turn out.

I hope this helps.

Best regards-

David

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for
Metallogaphy, Crystallography and Electron Microscopy.
Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is
privileged and confidential. This message is intended for the
individual or entity addressed. If you are not the intended recipient,
please do not read, copy or disclose this communication. Notify the
sender of the mistake by calling +1-949-492-2600 and delete this message
from your system.

by way of MicroscopyListserver wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (watson-at-wi.mit.edu) from
} http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Friday, August 27, 2004 at 10:20:20
} ---------------------------------------------------------------------------
}
}
} Email: watson-at-wi.mit.edu
} Name: Nicki Watson
}
} Organization: Whitehead Institute
}
} Title-Subject: [Microscopy] [Filtered] MEM training schools
}
} Question: Hi all,
} I am trying to find the name and web site of the two schools that
} offer an associate degree in electron microscopy.
} I believe there is one on the west coast, and one in the mid west.
} I met a few of the students from those schools at the recent meeting
} in Savannah, and I would like to get some more information about their
} program, and possibly submit a want ad to their placement department.
} If anyone knows of these schools please let me know.
} Thanks
} Nicki Watson
}
}
} ---------------------------------------------------------------------------
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 17:02:33 2004

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Check out:

http://www.deltacollege.edu/dept/electmicro/

It is Delta College in Stockton, CA.

gary g.

At 11:56 AM 8/27/2004, you wrote:

} Email: watson-at-wi.mit.edu
} Name: Nicki Watson
}
} Organization: Whitehead Institute
}
} Title-Subject: [Microscopy] [Filtered] MEM training schools
}
} Question: Hi all,
} I am trying to find the name and web site of the two schools that offer
} an associate degree in electron microscopy.
} I believe there is one on the west coast, and one in the mid west.
} I met a few of the students from those schools at the recent meeting in
} Savannah, and I would like to get some more information about their
} program, and possibly submit a want ad to their placement department.
} If anyone knows of these schools please let me know.
} Thanks
} Nicki Watson
}
}
} ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 17:14:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Just using Delta will get you to the wrong spot I think its full name is:
San Joaquin Delta College
http://www.deltacollege.org/dept/electmicro/
it is in Stockton Ca.

Jim

James L. Roberts
Firearm & Toolmark Examiner
Ventura Co. Sheriff's Lab
800 S. Victoria Ave.
Ventura, CA. 93009

(805) 654-2308

James.Roberts-at-mail.co.ventura.ca.us

} } } "Bill Tivol" {tivol-at-caltech.edu} 08/27/04 01:44PM } } }

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On Aug 27, 2004, at 11:56 AM, by way of MicroscopyListserver wrote:

} I am trying to find the name and web site of the two schools that
} offer an associate degree in electron microscopy.
} I believe there is one on the west coast, and one in the mid west.
} I met a few of the students from those schools at the recent meeting
} in Savannah, and I would like to get some more information about their
} program, and possibly submit a want ad to their placement department.
} If anyone knows of these schools please let me know.
}
Dear Nicki,
Delta College is probably the West Coast school you have in mind. It
was run by Judy Murphy for a long time. I do not know the present
situation with that program, since Judy is no longer affiliated with
it; however, up until Judy left, it was an excellent program, and I
would be certain that any graduate of that program would be exceedingly
well trained.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Aug 27 20:26:42 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Glad to know of other users out there!

we also have a strange specimen holder that holds many specimens and you
can rotate them in and out of the beam and switch to another one while still
maintaining the vacuum on the column!

Thanks Ed Sharpe archivist for SMECC

Please check our web site at
http://www.smecc.org
to see other engineering fields, communications and computation stuff we
buy, and by all means when in Arizona drop in and see us.

address:

coury house / smecc
5802 w palmaire ave
glendale az 85301

----- Original Message -----
} From: "Pat Connelly" {psconnel-at-sas.upenn.edu}
To: "ed sharpe" {esharpe-at-uswest.net}
Cc: "Ken Converse" {kenconverse-at-qualityimages.biz} ; "MSA Listserver"
{Microscopy-at-MSA.Microscopy.Com}
Sent: Friday, August 27, 2004 7:09 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (patrick.stallings-at-amd.com) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Friday, August 27, 2004 at 16:28:15
---------------------------------------------------------------------------

Email: patrick.stallings-at-amd.com
Name: Patrick Stallings

Organization: AMD

Title-Subject: [Microscopy] [Filtered] TEM junction stain for FIB prepared
semiconductor samples

Question: All,
I am trying to prepare samples for TEM analysis using focused ion
beam and then using a chemical stain to visually enhance the
semiconductor junction. Does anyone have a recipe that does this
well on FIB samples. I have tried several HNO3:HF solutions with no
real luck.
Thanks,

Patrick Stallings

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Aug 28 08:36:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Greetings,

Listers,

Here is the September 2004 Microscopy Today table of contents. I will close
the subscription list for this issue on Tuesday 7 September 2004.
Microscopists in North America and MSA members anywhere can subscribe for
free. Anyone else may subscribe for US$35 per year (to PARTIALLY cover
postage). All subscriptions at http://www.microscopy-today.com Thank you.

Carmichael: Cells Connected by Tiny Tunnels

Gillies: Microscopy & Microanalytical Support for NASA's Microgravity
Materials Science Programs

Magonov: High-Resolution Imaging with Atomic Force Microscopy

Brown, Nicholls, Royston, & D'Keidek: A Suspended Floor for
High-Performance Electron Microscopy and Nanoscience

Favret and Fuentes: RIMAPS and Variogram Analysis of Barley Leaf Surfaces

Hugo and Cady: Preparation of Geological and Biological TEM Specimens by
Embedding in Sulfur

Armitage: Artifacts from Rapid Microwave Processing of Trematode
Tissues (Ascocotyle pachycystis and leighi)

Neal and Russ: Principal Components Analysis of Multispectral Image Data

Camp, Byun, and Jacob: Electron Microscopy Analysis of Multilamellar
Vesicles Prepared from Synthetic Lipids: A Model System for Studying
Membrane Structure in the Molecular Cell Biology Classroom and Laboratory

Greenhut and Greenhut: Flicker Stereo: Digital 3D Viewing for PC &
Presentation

New and Interesting at Microscopy & Microanalysis 2004
Industry News
NetNotes

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 30 07:11:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

The midwest school offering an Associate Degree in Electron Microscopy is
Madison Area Technical College. The students that we have worked with
from MATC have been very good. Information is available at:

http://matcmadison.edu/electronmicros/

Joe Neilly, Research Investigator
Abbott Laboratories
R4R9, AP31
200 Abbott Park Rd.
Abbott Park, IL 60064-6202

Voice: 847-938-5024
Fax: 847-938-5027
E-mail: joe.neilly-at-abbott.com

} Email: watson-at-wi.mit.edu
} Name: Nicki Watson
}
} Organization: Whitehead Institute
}
} Title-Subject: [Microscopy] [Filtered] MEM training schools
}
} Question: Hi all,
} I am trying to find the name and web site of the two schools that offer
} an associate degree in electron microscopy.
} I believe there is one on the west coast, and one in the mid west.
} I met a few of the students from those schools at the recent meeting in
} Savannah, and I would like to get some more information about their
} program, and possibly submit a want ad to their placement department.
} If anyone knows of these schools please let me know.
} Thanks
} Nicki Watson
}

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 30 07:50:08 2004

Contents Retrieved from Microscopy Listserver Archives
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Greetings all,

I'm posting this on behalf of my McCrone colleague, David Wiley. He's
the managing editor of the online journal, ModernMicroscopy.com, and he
asked me to provide this update to the listserver.

Regards,

Elaine Schumacher
McCrone Associates, Inc.
eschumacher-at-mccrone.com

I would like to take this opportunity to thank everyone who visited or
tried to visit our new online journal www.ModernMicroscopy.com. Many of
you responded because of difficulties accessing the site, and I
appreciate your feedback. I tried to work with our ISP at the time, to
fix the problems with the site. In the end, the decision was made to
move the site to another ISP.

The move has been completed, and I would like to extend another
invitation to everyone. I hope that you will give the site a second
chance, if you haven't already. ModernMicroscopy.com is a peer reviewed
journal featuring articles, reviews and tutorials about microscopy by
some of the most experienced microscopists in the field. We are
actively looking for new topics and ideas from the entire microscopy
community. Submission information can be found on the site.

Regards,

David Wiley
Managing Editor
ModernMicroscopy.com
editor-at-modernmicroscopy.com

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 30 09:53:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Does anyone have a cut-away drawing of a scroll pump?

I give a lecture on vacuum including pumping systems in my SEM class and
have demo pumps that have been disassembled or cut open. However, I do not
have a demo scroll pump, their being relatively new as standard on new
instruments. A good drawing or comparison of features and maintenance
compared to oil rotary pump would be appreciated.

Thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Aug 30 12:30:39 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

There are diagrams that may be helpful in "High-Vacuum Technology - A
Practical Guide", 2E, M. H. Hablanian, 1997, Marcel Dekker, Inc. pp 190-196.

Michael Zemyan
Schafer Corporation

-----Original Message-----
} From: Debby Sherman [mailto:dsherman-at-purdue.edu]
Sent: Monday, August 30, 2004 8:16 AM
To: message to: MSA list

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mfein-at-bu.edu) from http://www.msa.microscopy.org/Ask-A-Microscopist/Ask-A-Microscopist.html on Monday, August 30, 2004 at 09:56:16
---------------------------------------------------------------------------

Email: mfein-at-bu.edu
Name: Marcia D. Feinberg

Organization: Boston University

Education: Graduate College

Location: Boston, MA , U.S.A.

Question: My Pioloform coated slot grids continue to break under the 6okV TEM beam. I cut and look at serial thin sections and we note that the Pioloform usually starts to break between two adjacent sections. We use a lot of liquid Nitrogen in the scope and it helps somewhat, but we still get breakage. I understand at 60kV the electrons are slower and are heating up the grid, compared to working at higher kV's but because of our low contrast brain tissue, we are forced to work at 60kV. I could try re-coating the grids with a thinner layer of Pioloform but that has some risks and lowers resolution somewhat. We also don't have a carbon coater and choose not to carbon coat because of the risks of messing up our series. Knowing all this, could someone suggest another way we can solve our problem? I thank you very much for your consideration. Marcia Feinberg

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 07:12:30 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

With a number of on-going building modifications here as well as the
potential for relocating my EM Facility. we find ourselves in need of a vibration
testing/monitoring system. What I am hoping to find is a simply system to
plug into a Laptop. Having had various vibration testing done in the past, and
where as I fully acknowledge the quality experience of testing service
providers we just can't afford that kind of expense on a continuing basis. We
are looking to do this in-house, monitor "baseline" building vibrations every
couple of weeks or so.

I have picked up the recommendations for a Wilcoxon 731A/P31
Accelerometer but now I need a compatible PCMCIA spectrum analyzer
interface board and software.

Any recommendations? And yes, vendors may respond directly back to
me.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 10:05:22 2004

Contents Retrieved from Microscopy Listserver Archives
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We have hired Vibration Engineering Consultants to do site surveys and I
believe they also sell survey equipment that runs from a laptop. You can
find more inforation at:
www.vibeng.com
We have been very happy with their work.

Regards,
Joe Neilly, Research Investigator
Abbott Laboratories
R4R9, AP31
200 Abbott Park Rd.
Abbott Park, IL 60064-6202

Voice: 847-938-5024
Fax: 847-938-5027
E-mail: joe.neilly-at-abbott.com

"Richard Edelmann" {edelmare-at-MUOhio.edu}
08/31/2004 07:34 AM
Please respond to edelmare

To: microscopy-at-MSA.Microscopy.com
cc:
Subject: [Microscopy] Vibration testing system

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

With a number of on-going building modifications here as
well as the
potential for relocating my EM Facility. we find ourselves in need of a
vibration
testing/monitoring system. What I am hoping to find is a simply system to

plug into a Laptop. Having had various vibration testing done in the
past, and
where as I fully acknowledge the quality experience of testing service
providers we just can't afford that kind of expense on a continuing basis.
We
are looking to do this in-house, monitor "baseline" building vibrations
every
couple of weeks or so.

I have picked up the recommendations for a Wilcoxon
731A/P31
Accelerometer but now I need a compatible PCMCIA spectrum analyzer
interface board and software.

Any recommendations? And yes, vendors may respond
directly back to
me.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 11:27:16 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Aug 31, 2004, at 5:22 AM, by way of Ask-A-Microscopist wrote:

} Question: My Pioloform coated slot grids continue to break under the
} 6okV TEM beam. I cut and look at serial thin sections and we note that
} the Pioloform usually starts to break between two adjacent sections.
} We use a lot of liquid Nitrogen in the scope and it helps somewhat,
} but we still get breakage. I understand at 60kV the electrons are
} slower and are heating up the grid, compared to working at higher kV's
} but because of our low contrast brain tissue, we are forced to work at
} 60kV. I could try re-coating the grids with a thinner layer of
} Pioloform but that has some risks and lowers resolution somewhat. We
} also don't have a carbon coater and choose not to carbon coat because
} of the risks of messing up our series. Knowing all this, could someone
} suggest another way we can solve our problem? I thank you very much
} for your consideration. Marcia Feinberg
}
Dear Marcia,
You need to conduct heat and charge away from the spot where the
electron beam interacts with the specimen, and, since you do not want
to coat the specimen and the Pioloform is not a good conductor, a
remaining possibility is to lower the dose rate to the point that the
heat and charge will dissipate. Possibly, pre-irradiation of the
entire slot with a low dose could produce enough conductivity in the
Pioloform to overcome the problem. I'd experiment with grids that do
not have valuable material on them to determine what pre-irradiation
and/or dose rate are optimal. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 13:58:03 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Marcia
Try Formvar instead Pioloform. Carbon coating of the grids (before
attaching sections) also highly recommended (you could bought them from any
major EM suppliers) problems with contrast even using Spurr resin (images
in Spurr for some reason looks less contrasty than from Epon) at 80 kV. I
don't believe lowering accelerating voltage could benefit on very (yes)
thick Pioloform film. Pioloform itself will scatter a lot of electrons, so
your signal (image) would be very noisy and less informative. You could
easily adjust contrast using higher voltage and smaller obj aperture. Low
voltage also damaged your sample, so we are not talking here about better
"resolution" at lower voltage... Sergey

At 07:22 AM 8/31/2004 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 14:09:56 2004

Contents Retrieved from Microscopy Listserver Archives
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We just bought the Spicer Consulting Analysis System SC11. It is a Laptop
based system to measure vibrations using a Wilcoxon 731A Accelerometer,
AC/DC-fields and Sounds.

You can find more information at http://www.spicerconsulting.com/

Robert

At 08:34 AM 8/31/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

----------
Robert F. Klie, PhD
Goldhaber Distinguished Fellow
Center for Functional Nanomaterials (Bldg.480)
Brookhaven National Laboratory
Upton, NY 11973
Tel. (631) 344-7709
Fax. (631)344-4071

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 15:45:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

An inexpensive possibility...

The accelerometer may need a signal conditioner/buffer/amplifier - I have
not checked it's specifications. If a PC sound card meets your frequency
range and resolution requirements, the rest is simple and cheap.

A number of free/shareware programs that will turn your PC into an audio
range spectrum analyzer are available. Adjust the accelerometer/amplifier
output level to be compatible with the sound card "line in" requirement
(typically 1 volt peak, max)and you are there...

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOhio.edu]
Sent: Tuesday, August 31, 2004 8:34 AM
To: microscopy-at-MSA.Microscopy.com

With a number of on-going building modifications here as well as the

potential for relocating my EM Facility. we find ourselves in need of a
vibration
testing/monitoring system. What I am hoping to find is a simply system to
plug into a Laptop. Having had various vibration testing done in the past,
and
where as I fully acknowledge the quality experience of testing service
providers we just can't afford that kind of expense on a continuing basis.
We
are looking to do this in-house, monitor "baseline" building vibrations
every
couple of weeks or so.

I have picked up the recommendations for a Wilcoxon 731A/P31
Accelerometer but now I need a compatible PCMCIA spectrum analyzer
interface board and software.

Any recommendations? And yes, vendors may respond directly back
to
me.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 18:11:33 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kn77-at-uwyo.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, August 31, 2004 at 14:43:11
---------------------------------------------------------------------------

Email: kn77-at-uwyo.edu
Name: Kusum Naithani

Organization: University of Wyoming

Education: Graduate College

Location: Laramie, Wyoming, USA

Question: Hi!
I'm working on plant leaf material (sagebrush). Leaf is covered by minute white hairs and due to this reason I'm not able to find the distribution of stomatal cells. Could you please suggest a way to remove these hairs so that I can see stomatal cells.
2nd question..
I want to measure the size and depth of stomatal cells. Could you please tell me the way to fix leaf in its living conditions.
I would greatly appreciate your help.
Thanks!
Kusum

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 18:13:35 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donaldawbrey-at-texashealth.org) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, August 31, 2004 at 13:00:40
---------------------------------------------------------------------------

Email: donaldawbrey-at-texashealth.org
Name: Donald G. Awbrey

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] MSA Certification

Question: Dear MSAnetters,

Is there a MSA certification for TEM? If so, where does one go about looking for information. If any one knows, please contact me.

Thank you in advance,

Donald G. Awbrey, HT(ASCP) QIHC
donaldawbrey-at-texashealth.org

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Aug 31 19:04:58 2004

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Greetings all

What embedding protocol have you used for skin (epidermis and dermis)
into Spurr?

Thanks

Bob Becker

Robert Becker, PhD
Department of Anatomy and Cell Biology (mc512)
Univ IL -at- Chicago
Room 578
808 S Wood St
Chicago, IL 60612-7308
312 996 7215 ph
312 413 0354 fx

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 06:16:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello All

I'm a student now considering studies in basics of microscopy to consider a
possible career change.

I'm seeking information on flourescence microscopy, why would someone use
this over other methods, the difference between single photon and two photon
fluorescence . Anyone's experience on laser scanning confocal microscopes (
1photon and 2 photon), is it worth the expense? Although I don't know what
they cost, I am told that they are expensive, does anyone know?

Thank You
Paul Bitetto

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 06:42:33 2004

Contents Retrieved from Microscopy Listserver Archives
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Silvia,
There are indeed flat, enclosable embedding cylindrical molds, standard size
#00, with a flat end....on both sides! Just like BEEM capsules. I
get ours from Electron Microscopy Sciences (#70021):

http://www.emsdiasum.com/microscopy/products/preparation/capsule.aspx#70021

These should work great with LR White, though I typically use the #00
gelatin capsules with LR White.

Walter F. Bobrowski
Investigative Pathology
Safety Sciences
Pfizer Global Research & Development
Ann Arbor, MI 48105

TEL: 734-622-7814
FAX: 734-622-3478
Mobile: 734-646-0502

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From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 08:33:47 2004

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Kusum,

I don't know a good way to remove the hairs, but for counting and
measuring stomata, it would be easier if any waxy cuticle was removed
during processing. I have done this by using acetone as a dehydrant,
rather than ethanol. In my experience, it cleans up the surface of the
leaf quite well and makes the stomata and other surface features stand
out nicely.

Good luck.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:kn77-at-uwyo.edu]
Sent: Tuesday, August 31, 2004 6:34 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (kn77-at-uwyo.edu) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Tuesday, August 31, 2004 at 14:43:11
------------------------------------------------------------------------
---

Email: kn77-at-uwyo.edu
Name: Kusum Naithani

Organization: University of Wyoming

Education: Graduate College

Location: Laramie, Wyoming, USA

Question: Hi!
I'm working on plant leaf material (sagebrush). Leaf is covered by
minute white hairs and due to this reason I'm not able to find the
distribution of stomatal cells. Could you please suggest a way to remove
these hairs so that I can see stomatal cells.
2nd question..
I want to measure the size and depth of stomatal cells. Could you please
tell me the way to fix leaf in its living conditions. I would greatly
appreciate your help. Thanks! Kusum

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 08:58:41 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mingram-at-rohmhaas.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 1, 2004 at 05:24:13
---------------------------------------------------------------------------

Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Organization: Rohm and Haas

Title-Subject: [Microscopy] [Filtered] MListserver: Registration of SEM's due to X-rays

Question: In Delaware it appears we are required to register our SEM as a X-ray source. Does any know this to be true?

Thanks

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 11:05:14 2004

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Kusum,

You can try removing the trichomes by very gently shaving the leaf.
Hold a razor blade almost vertical, just not touching the leaf
surface, and pull in the direction of the tilt. This requires a
steady hand, and doesn't work on robust trichomes, but might on
sagebrush -- I don't know that plant. The other approach would be to
go at the leaf with the blade near horizontal and again just not
touching the leaf, like shaving your face. But I haven't done that in
so long, I've forgotten how.
You don't need to remove the entire trichome, just most of it, so the
surface is revealed.
The best way to measure the size of the stomatal cells would be with
a light microscope on freshly picked leafs in a room (or chamber) of
the appropriate humidity. Or, same conditions, but make a replica
with dental silicone or one of the replica materials the EM companies
sell. The replica could then be examined in the SEM, or with a light
microscope.

Phil

} Email: kn77-at-uwyo.edu
} Name: Kusum Naithani
}
} Organization: University of Wyoming
}
} Education: Graduate College
}
} Location: Laramie, Wyoming, USA
}
} Question: Hi!
} I'm working on plant leaf material (sagebrush). Leaf is covered by
} minute white hairs and due to this reason I'm not able to find the
} distribution of stomatal cells. Could you please suggest a way to
} remove these hairs so that I can see stomatal cells.
} 2nd question..
} I want to measure the size and depth of stomatal cells. Could you
} please tell me the way to fix leaf in its living conditions.
} I would greatly appreciate your help.
} Thanks!
} Kusum
}
} ---------------------------------------------------------------------------

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 11:16:27 2004

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Hi Paul,
Fluorescence microscopy when you have access to confocal microscope is awesome.
For career, every experimentals fields, particulary with bio tag on the name is
not an easy career from money perspective, but from scientific point of view it
is great.

All the best,

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------
}
}
} Hello All
}
} I'm a student now considering studies in basics of microscopy to consider a
} possible career change.
}
} I'm seeking information on flourescence microscopy, why would someone use
} this over other methods, the difference between single photon and two photon
} fluorescence . Anyone's experience on laser scanning confocal microscopes (
} 1photon and 2 photon), is it worth the expense? Although I don't know what
} they cost, I am told that they are expensive, does anyone know?
}
} Thank You
} Paul Bitetto
}
}
}
}
}
}
}
}

--
Antoine Blanc, Research Associate
Ecole Polytechnique de Montreal
Chemical Engineering, Mike Buschmann Laboratory
CP 6079, succ. Centre-ville
Montréal Qc, Canada H3C 3A7
Tel.:514-340-4711 ext.:3212,3336,3337
FAX:514-340-4159
secrétariat: 514-340-4711 ext.:4984

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 11:44:29 2004

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I'm not sure about Delaware, but this is true for the
State of Michigan. You may want to check your State's
website in the registration or health section for
information.

In the last conversation I had with the state
inspector, the State is considering dropping
registration for scanning electron microscopes because
of the negligible danger from SEMs leaking X-rays.
Since the SEM by all practical purposes cannot operate
unless everything is buttoned up for the vacuum, the
chance for X-ray leakage is just about nil.

Stu Smalinskas, P.E.
SKF USA
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Mike wrote:

Question: In Delaware it appears we are required to
register our SEM as a X-ray source. Does any know
this to be true?

Thanks

Email: mingram-at-rohmhaas.com
Name: Mike Ingram
Organization: Rohm and Haas

__________________________________
Do you Yahoo!?
Yahoo! Mail is new and improved - Check it out!
http://promotions.yahoo.com/new_mail

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 12:27:45 2004

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O.k., here is my suggestion for removing the root hairs: Follow any standard
fixation protocol (I know you asked about them as well) but you'll find that
sagebrush does not "wet" very well, so you'll need to add a surfactant like
Kodak Photo-flo or Tween (1 drop / 10ml fixative is generally enough) - if you
are looking to follow up with light microscopy then FAA might work very nicely
for you [FAA = Formalin-Acedic acid-Alcohol Formulation: 50% (or 70%)
ethyl alcohol - 90ml, Glacial Acetic Acid - 5ml, Formalin - 5ml]. In which the
alcohol works well to "wet" the material.

In any case, dehydrate the samples to 50%-100% solvent (EtOH), plunge
freeze in liquid nitrogen, rub the surface of the leaves with a wood stick, pre-
cooled razor blade, plastic bar, etc. This should break all the tricomes off the
leaf surface revealing the stomata. Transfer samples back from liquid
nitrogen and continue with sample prep.

To accurately measure somata depth you will have to section the samples and
look at the cells in cross-section.

Standard fixatation

1) Primary Fixation: 1-2% paraformaldehyde, 2-4% glutaraldehyde, in a
suitable pH buffer (i.e. 6.8-7.2 pH 0.2 M Sodium Phosphate, 0.05 M Sodium
Cacodylate, HEPES, PIPES, etc. ). Fixation for 5-120 min. at room temp. (20-
22 C), normal growth temp (37 C?) or on ice (0-4 C). [50 min. -at- room
temp]. Specimens should be cut as small as possible.

2) Rinse: 4 times -at- 10-15 min. each with the above buffer without
aldehyde fixatives. (Residual aldehydes will bind with OsO4 in secondary
fixation if used.)

*3) Secondary Fixation: 1-2% Osmium tetroxide (OsO4) in full to half
strength buffer used above. Fixation for 2-6 hours at room temperature.
(OsO4 fixation generally not used if immunological staining procedures will be
used.)

*4) Rinse: 4 times -at- 15-20 min. each with distilled water.

5) Dehydration: Generally either absolute ethanol (200 proof) or glass
distilled acetone is used.

% Solvent in water Time

25% 20-30 min
50% 20-30 min
75% 20-30 min
95% 30-60 min
100% 60+ min
100% 60+ min

SEM: CPD samples

TEM: resin embbedd samples

}
} Email: kn77-at-uwyo.edu
} Name: Kusum Naithani
}
} Organization: University of Wyoming
}
} Education: Graduate College
}
} Location: Laramie, Wyoming, USA
}
} Question: Hi!
} I'm working on plant leaf material (sagebrush). Leaf is covered by minute white
} hairs and due to this reason I'm not able to find the distribution of stomatal
} cells. Could you please suggest a way to remove these hairs so that I can see
} stomatal cells. 2nd question.. I want to measure the size and depth of stomatal
} cells. Could you please tell me the way to fix leaf in its living conditions. I
} would greatly appreciate your help. Thanks! Kusum
}
} ---------------------------------------------------------------------------
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 12:57:24 2004

Contents Retrieved from Microscopy Listserver Archives
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This is also true for Illinois. We used to have routine inspections by the
IL Dept of Nuclear Safety, but they felt it was no longer justified for SEMs.

Alan Stone
ASTON

At 12:06 PM 9/1/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 14:02:18 2004

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Mike,
As of July 2000 it was still required. Try contacting

Delaware Health and Social Services
Division of Public Health
Office of Radiation Control
P.O. Box 637
Dover, DE 19903
302-739-3787

Perhaps 4 years later you might be able to find a website for them. From
Stu's reply it sounds like some sanity might be returning concerning SEMs
and x-rays, but I'm not going to go there today.

Good luck,
Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:mingram-at-rohmhaas.com]
Sent: Wednesday, September 01, 2004 10:21 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mingram-at-rohmhaas.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday,
September 1, 2004 at 05:24:13
---------------------------------------------------------------------------

Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Organization: Rohm and Haas

Title-Subject: [Microscopy] [Filtered] MListserver: Registration of SEM's
due to X-rays

Question: In Delaware it appears we are required to register our SEM as a
X-ray source. Does any know this to be true?

Thanks

---------------------------------------------------------------------------

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From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 14:55:47 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Marcia,

Just some thoughts on your breaking grids:
1. Make sure the Pioloform is absolutely fresh.
2. Can you use a regular mesh grid for additional support?
3. You could obtain carbon coated slot grids from Ladd or some other EM
supplier.

John Arnott

Disclaimer: Ladd Research sells grids, custom coated grids, and the supplies
needed to make them yourself.

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: ladres-at-att.net

----- Original Message -----
} From: "Bill Tivol" {tivol-at-caltech.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Tuesday, August 31, 2004 12:57 PM

The fall meeting of the Texas Society for Microscopy will be Oct. 21-23
at the Hilton Garden Inn in Allen, TX. We have an exciting schedule
planned including the Thursday workshop "EBSD and FESEM - A Formidable
Combination for Characterization of Semiconductor Materials" to be
presented by Dr. Keith Dicks from Oxford Instruments. The workshop will
take place at Microtech Analytical Labs, Inc., 538 Haggard Street, Suite
402 Plano, TX 75074.
In addition to the Thursday workshop, Oxford Instruments, JEOL and
Microtech Analytical Labs are making the Inca Energy EDX and Inca
Crystal EBSD system on a JEOL 6500F available for demo Tues, Wed and Fri
(Oct. 19-20, 22). This is an opportunity to bring your own samples and
evaluate this technique with one on one contact with the industry
experts. To schedule demo time, contact Mike Crowley with Oxford
Instruments at 512-246-7551 or by email at crowley-at-ma.oxinst.com. Space
is limited so sign up early.

All registration forms and hotel information are available on our web
site: http://www.texasmicroscopy.org/. We look forward to seeing you
in the fall.

Regards,
Jodi Roepsch
Program Chair
972-952-3228, j-roepsch1-at-raytheon.com

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 17:00:06 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (nbauer-at-paulstra.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Wednesday, September 1, 2004 at 10:11:08
---------------------------------------------------------------------------

Email: nbauer-at-paulstra.com
Name: Nathan Bauer

Organization: Paulstra

Education: Graduate College

Location: Grand Rapids, Mi, USA

Question: Can carbon nano tubes :
1) Carry an electrical current (and if so, how much)?

2) Can they be polorized?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 18:19:04 2004

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This is not strictly true, Michigan are thinking of stopping the
registration if the instrument is "unmodified" from the manufacturer.
If you have added anything that was not supplied by the manufacturer,
i.e an XEDS system, CL system, viewport or similar then they still want
it registered and tested. We just had our health and safety people
check all our stuff because the Michigan inspector came round and
checked all of our machines (TEMs, SEMs FIBs and XPS).

--
John Mansfield PhD MInstP
North Campus Electron Microbeam Analysis Laboratory
417 SRB, University of Michigan
2455 Hayward, Ann Arbor MI 48109-2143 USA
Phone: (734) 936-3352 FAX (734) 763-2282
Cell. Phone: (734) 834-3913
(Leaving a phone message at 936-3352 is preferable to 834-3913)
Email: jfmjfm-at-engin.umich.edu
URL: http://emalwww.engin.umich.edu/people/jfmjfm/jfmjfm.html
Location: Lat. 42° 16' 48" Long. 83° 43' 48"
AIM: thejfmjfm

Home address:
4304 Spring Lake Boulevard
Ann Arbor MI 48108-9657
Phone (734) 994-3096

On Sep 1, 2004, at 1:06 PM, Kestutis Smalinskas wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} I'm not sure about Delaware, but this is true for the
} State of Michigan. You may want to check your State's
} website in the registration or health section for
} information.
}
} In the last conversation I had with the state
} inspector, the State is considering dropping
} registration for scanning electron microscopes because
} of the negligible danger from SEMs leaking X-rays.
} Since the SEM by all practical purposes cannot operate
} unless everything is buttoned up for the vacuum, the
} chance for X-ray leakage is just about nil.
}
} Stu Smalinskas, P.E.
} SKF USA
} Plymouth, Michigan
}
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
}
} Mike wrote:
}
} Question: In Delaware it appears we are required to
} register our SEM as a X-ray source. Does any know
} this to be true?
}
} Thanks
}
} Email: mingram-at-rohmhaas.com
} Name: Mike Ingram
} Organization: Rohm and Haas
}
}
}
}
}
} __________________________________
} Do you Yahoo!?
} Yahoo! Mail is new and improved - Check it out!
} http://promotions.yahoo.com/new_mail
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 20:52:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (lotocka-at-acn.waw.pl) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 1, 2004 at 14:49:49
---------------------------------------------------------------------------

Email: lotocka-at-acn.waw.pl
Name: Barbara Lotocka

Organization: Department of Botany, Warsaw Agricultural University

Title-Subject: [Microscopy] MListserver: fixative for lichen

Question: Hello Everyone,

I would be most grateful for any suggestions on a fixation protocol (for transmission electron microscope) optimized for lichens.

I fixed some samples of Cladonia in a fixative that is routinely used for plant samples in my department (paraformaldehyde + glutaraldehyde in sodium cacodylate buffer), but after embedding in epoxy resin the thallus looked shrunken and the section were "scratched" as if the thallus was extremely hard. Perhaps the problem was in dehydration? I used the usual graded series of ethanol and acetone.

With best regards - and hope ;-)
Barbara

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 20:53:09 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (pzou-at-feico.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 1, 2004 at 20:19:52
---------------------------------------------------------------------------

Email: pzou-at-feico.com
Name: Pei Zou

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Can anybody comment on the image darkening effect as one progressively scans the surface of a sample with a SEM? What are the possible physical causes, and how to reduce the effect?

Any articles that can provide an overview of this phenomenon?

Thanks,

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 1 21:14:28 2004

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Kusum

One possible way to remove hairs that should work is to make a surface replica of the surface using nail varnish or a mounting medium such as Shur Mount and stripping off when dry. On most of the leaf tissues I've worked with it removes hairs, fungi, surface debris but does not damage the surface itself.

Ian

Ian Hallett
HortResearch
Mt Albert Research Centre, Private Bag 92 169
Auckland, New Zealand
Fax +64 9 815 4201
Telephone +64 9 815 4200
EMail ihallett-at-hortresearch.co.nz

} } } by way of Ask-A-Microscopist {kn77-at-uwyo.edu} 1/09/2004 11:34:02 a.m. } } }

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kn77-at-uwyo.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, August 31, 2004 at 14:43:11
---------------------------------------------------------------------------

Email: kn77-at-uwyo.edu
Name: Kusum Naithani

Organization: University of Wyoming

Education: Graduate College

Location: Laramie, Wyoming, USA

Question: Hi!
I'm working on plant leaf material (sagebrush). Leaf is covered by minute white hairs and due to this reason I'm not able to find the distribution of stomatal cells. Could you please suggest a way to remove these hairs so that I can see stomatal cells.
2nd question..
I want to measure the size and depth of stomatal cells. Could you please tell me the way to fix leaf in its living conditions.
I would greatly appreciate your help.
Thanks!
Kusum

---------------------------------------------------------------------------

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 01:26:55 2004

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Hi

Anyone out there know of any courses in microscopic morphometry/digital
image analysis - preferably in Europe.

Websites of special interest groups of professional bodies with special
interest sections would also be appreciated.

All the best

Med vänliga hälsningar/With best regards

Gareth

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 01:54:31 2004

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Dear Pei Zou,

See section 9.10.6 in Goldstein et al.: Scanning electron microscopy and X-ray analysis" Plenum Press 1992. It begins: "A sample subjected to electron bombardment in a diffusion-pumped vacuum gradually becomes ccovered with a contamination layer due to polymerization, under the action of the beam, of organic matter adsorbed on the surface".

Ways to reduce the effect are: clean vacuum, clean sample, cold finger.

Best regards,
Jorgen.

{:::} --- {:::} --- {:::} --- {:::} --- {:::} --- {:::}

Joergen B. Bilde-Soerensen
Senior Research Scientist, Ph. D.
Materials Research Department
Risoe National Laboratory
DK-4000 Roskilde
Denmark

e-mail: j.bilde-at-risoe.dk
phone: +45 4677 5802 (direct)
phone: +45 4677 4677 (switchboard)
fax: +45 4677 5758
website: http://www.risoe.dk/afm/Personal/jqbi/jqbi.htm

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:pzou-at-feico.com]
Sent: 2. september 2004 04:16
To: microscopy-at-microscopy.com

---------------------------
Dr Wally H. Müller
Senior University Research
University of Utrecht, Faculty of Biology
Molecular Cell Biology - Electron Microscopy
Kruyt building, Room West 510
Padualaan 8, 3584 CH Utrecht, The Netherlands
Phone +31 30 2533588 Fax +31 30 2513655
E-mail W.H.Muller-at-bio.uu.nl

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 05:16:35 2004

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http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

In a message dated 9/2/04 3:45:16 AM, Gareth.Morgan-at-labmed.ki.se writes:

} Anyone out there know of any courses in microscopic morphometry/digital
} image analysis - preferably in Europe.

Upcoming courses on quantitative image analysis that I will be teaching are:

Sunday October 3 - A one-day tutorial on strategies for quantitative image
analysis will be presented as part of the AOCS Conference on Food Structure and
Quality in Cork, Ireland. Registration for the workshop is available at
{http://www.aocs.org/meetings/fsq/courses.asp}

Tuesday, November 9 - Thursday, November 11 - A three-day hands-on course on
Quantitative Image Analysis will be presented at the University of Missouri,
Columbia, MO. Contact {rosslm-at-missouri.edu} Dr. Lou Ross, Electron Microscopy
Core Facility, W136 Veterinary Medicine, University of Missouri, Columbia, MO
65211-5120, (573) 882-4777, fax 884-5414.

Wednesday, March 16 - Friday, March 18, 2005 - A three-day hands-on course on
Photomicrography and Advanced Image Analysis will be presented at the McCrone
Institute in Chicago. Contact {rweaver-at-mcri.org} Dr. Rob Weaver at the
McCrone Institute, 2820 South Michigan Avenue, Chicago IL 60616, 312-842-7100. A
brief description of the course contents is available at
{http://www.mcri.org/Course_description.html#advdig} their website

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 08:17:25 2004

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Colleagues

The August Archives are now on-line at

http://www.microscopy.com/MicroscopyListserver

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 10:50:32 2004

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Kusum & Ian,

For a simple and effective method for making plant surface replicas for
observation by LM or SEM, see my article in the Nov/Dec 2003 issue of
Microscopy Today: Cellulose Acetate Replication of Plant Surfaces for SEM
(plug plug!!). You'll see images of stomata there.

http://www.microscopy-today.com

However, if a plant surface is very thickly populated by a tangled mess of
hairs, or trichomes, then replication may not be possible, as it will be
full of holes left by the trichomes and may tear apart upon attempted
removal from the surface. If the hair density is not too high, even though
holes from trichomes may be present, you may still be able to see enough
surface to get a good sample of the stomata.

--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra

} Kusum
}
} One possible way to remove hairs that should work is to make a surface replica
} of the surface using nail varnish or a mounting medium such as Shur Mount and
} stripping off when dry. On most of the leaf tissues I've worked with it
} removes hairs, fungi, surface debris but does not damage the surface itself.
}
} Ian
}
}
} Ian Hallett
} HortResearch
} Mt Albert Research Centre, Private Bag 92 169
} Auckland, New Zealand
} Fax +64 9 815 4201
} Telephone +64 9 815 4200
} EMail ihallett-at-hortresearch.co.nz
}
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted
} by (kn77-at-uwyo.edu) from
} http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on
} Tuesday, August 31, 2004 at 14:43:11
} ---------------------------------------------------------------------------
}
} Email: kn77-at-uwyo.edu
} Name: Kusum Naithani
}
} Organization: University of Wyoming
}
} Education: Graduate College
}
} Location: Laramie, Wyoming, USA
}
} Question: Hi!
} I'm working on plant leaf material (sagebrush). Leaf is covered by minute
} white hairs and due to this reason I'm not able to find the distribution of
} stomatal cells. Could you please suggest a way to remove these hairs so that I
} can see stomatal cells.
} 2nd question..
} I want to measure the size and depth of stomatal cells. Could you please tell
} me the way to fix leaf in its living conditions.
} I would greatly appreciate your help.
} Thanks!
} Kusum
}

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 12:45:37 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jtd1-at-psu.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, September 2, 2004 at 10:55:11
---------------------------------------------------------------------------

Email: jtd1-at-psu.edu
Name: Tom Doman

Organization: Penn State University

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Our lab is considering various photo printers (} $1K) for production of electron micrographs. Currently the Epson 2200 is the stromg favorite. Are there any recomendations for other printers which we should consider? What are your reasons for the recomended printer?

Thanks in advance!

Tom

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 12:46:17 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (walter.bobrowski-at-pfizer.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, September 2, 2004 at 11:12:16
---------------------------------------------------------------------------

Email: walter.bobrowski-at-pfizer.com
Name: Walt Bobrowski

Organization: Pfizer Global R&D

Title-Subject: [Microscopy] [Filtered] DMP-30 vs. BDMA

Question: Can one substitute BDMA for DMP-30 in a Luft-based epoxy resin? If so, what would the proportion be? Currently, I add 2ml DMP-30 to 100 ml resin (PolyBed 812, NMA, DDSA). I believe I read you can substitute to produce a less viscous mixture, but can't find it. Any references appreciated!

Walt

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 14:48:39 2004

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} Email: walter.bobrowski-at-pfizer.com
} Name: Walt Bobrowski
}
} Organization: Pfizer Global R&D
}
} Title-Subject: [Microscopy] [Filtered] DMP-30 vs. BDMA
}
} Question: Can one substitute BDMA for DMP-30 in a Luft-based epoxy
} resin? If so, what would the proportion be? Currently, I add 2ml
} DMP-30 to 100 ml resin (PolyBed 812, NMA, DDSA). I believe I read
} you can substitute to produce a less viscous mixture, but can't find
} it. Any references appreciated!
}
} Walt -

The only reason that DMP-30 is still around is tradition; by all
means substitute the same amount of BDMA. Viscosities: BDMA, 0.85
cP, DMP-30, 20.5 cP. The quantity that you use is small, so there
won't be a big change in the viscosity of the mix, but DMP-30 is so
viscous that it can actually partition out of the mix during
infiltration! AND DMP-30 is hygroscopic, which leads to more
problems. The original reference is A. Glauert, Proc. RMS 22:264
(1987) and you'll find the data in chapter 6 of Glauert & Lewis,
Biological Specimen Preparation for Transmission Electron Microscopy,
Princeton,1998.

Why not use a less viscous epoxy, such as Spurr (with the new, safer
ERL 4221) or Embed-It? They're both 65 cP, mixed.

--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 2 14:50:47 2004

Contents Retrieved from Microscopy Listserver Archives
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So after years of hearing and reading about why BDMA is better than DMP-30,
I switched to BDMA I used it at about 60-80% of the weight of DMP-30 and
got equivalent results using freshly made resin mixes. But I routinely
store my extra resin at -20 C and saw a difference. The BDMA mixtures got
much more viscous (presumably partially polymerized) after 1-2 weeks at -20
compared to the DMP-30 mixtures. So I went back to DMP-30. Whichever one
you use, I strongly advised you begin to dispense it and the other
components by weight. I have a scale in my fume hood and make 50 ml
batches of epoxy resins this way and they are much more consistent and the
mess is significantly less. good luck. tom phillips

01:08 PM 09/02/04 -0500, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 00:24:30 2004

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Dear Tom

I had a look at the archive and this had been discussed a few times in the last few years. Technology is changing fast especially in the digital world. We two would like to know the best printer (quality) out there if there is no money limitation and the best value for money meaning quality prints all editors of journals will be happy with. We got a comment like "the digital images are brilliant but the prints do not do them justice" from a editor.
Please pass all communication to us as well.
Thanks for all the help.

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:jtd1-at-psu.edu]
Sent: Thursday, September 02, 2004 8:08 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jtd1-at-psu.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, September 2, 2004 at 10:55:11
---------------------------------------------------------------------------

Email: jtd1-at-psu.edu
Name: Tom Doman

Organization: Penn State University

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Our lab is considering various photo printers (} $1K) for production of electron micrographs. Currently the Epson 2200 is the stromg favorite. Are there any recomendations for other printers which we should consider? What are your reasons for the recomended printer?

Thanks in advance!

Tom

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 02:43:09 2004

Contents Retrieved from Microscopy Listserver Archives
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In the same week there is news of significant change in two of the
companies that were
major players in silver image photography in the 20th century.
Ilford has shed almost half its staff preparative to sale of the
traditional photographic
business while it is still a going concern, allowing the company to
focus on its Swiss digital business.
http://www.channel4.com/news/news_story.jsp?storyId=156722
Agfa has shed its traditional photographic film and consumer imaging
business in a management buyout so that it can "focus on its core
growth markets of Graphic Systems and HealthCare, which are rapidly
going digital"
http://news.agfa.com/corporate/news.nsf/news/F07C0210ECC86EA9C1256EF3004D27CE?opendocument

Events like these, and Kodak's announcement earlier this year that it
would cease the production of its poneering APS cameras (though not of
films) underline the fragility of the conventional photographic
market in the face of the growth of digital imaging.

Which begs the question "can we rely on the continued availability of
EM film", and if not, how long have we got
to plan for the conversion to digital?

Dr. Chris Jeffree
University of Edinburgh
Schoolof Biological Sciences

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 05:34:31 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

If money were no object? We have been using the Fujifilm 3000 Pictrography
digital printer (it is truly a mini wet-lab). The latest model is the 4500:

http://www.fujifilm.com/JSP/fuji/epartners/PRNewsDetail.jsp?DBID=NEWS_547164
&CAT_ID=233840

These units are designed to print only photo-quality and they do it well. As
we have progressed towards keeping documents (including images) electronic
and have thrown out the darkroom, and due to cost per print ($4.00/8x10),
we only use the Pictrography to print images for manuscripts. If colleagues
want review-quality, they either must review on their computer monitor or
send image files to a B&W/Color LaserJet (yeah, lousy quality, but it's only
for review).

Best regards,

Walter F. Bobrowski
Investigative Pathology
Safety Sciences
Pfizer Global Research & Development
Ann Arbor, MI 48105

TEL: 734-622-7814
FAX: 734-622-3478
Mobile: 734-646-0502

-----Original Message-----
} From: Coetzee, Mr S. H Physics Science [mailto:COETZEES-at-mopipi.ub.bw]
Sent: Friday, September 03, 2004 1:51 AM
To: by way of MicroscopyListserver
Cc: microscopy-at-microscopy.com

Dear Tom

I had a look at the archive and this had been discussed a few times in the
last few years. Technology is changing fast especially in the digital
world. We two would like to know the best printer (quality) out there if
there is no money limitation and the best value for money meaning quality
prints all editors of journals will be happy with. We got a comment like
"the digital images are brilliant but the prints do not do them justice"
from a editor.
Please pass all communication to us as well.
Thanks for all the help.

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:jtd1-at-psu.edu]
Sent: Thursday, September 02, 2004 8:08 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (jtd1-at-psu.edu) from
http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday,
September 2, 2004 at 10:55:11
---------------------------------------------------------------------------

Email: jtd1-at-psu.edu
Name: Tom Doman

Organization: Penn State University

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Our lab is considering various photo printers (} $1K) for
production of electron micrographs. Currently the Epson 2200 is the stromg
favorite. Are there any recomendations for other printers which we should
consider? What are your reasons for the recomended printer?

Thanks in advance!

Tom

---------------------------------------------------------------------------

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Unless expressly stated otherwise, this message is confidential and may be privileged. It is intended for the addressee(s) only. Access to this E-mail by anyone else is unauthorized. If you are not an addressee, any disclosure or copying of the contents of this E-mail or any action taken (or not taken) in reliance on it is unauthorized and may be unlawful. If you are not an addressee, please inform the sender immediately.

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 05:45:11 2004

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On the Vibration testing, the kit is available from various companies but is
expensive.
We bought a complete unit from spicer consulting
http://www.spicerconsulting.com/
Their SC11 kit costs around $10,000 but that does everything.

However there are other products available. (
http://www.predictech.com/CM/PT908.htm ) not sure though that they will be
sensitive enough.

Luc Harmsen
ANASPEC South Africa

Tel: +27 11 794 8340
Fax: +27 11 794 8349
Mobile: +27 82 4459 003
Email: luc-at-anaspec.co.za
www.anaspec.co.za

P.O. Box 2561
Honeydew 2040
Gauteng, South Africa
-----Original Message-----
} From: White, Woody N. [mailto:nwwhite-at-bwxt.com]
Sent: 31 August 2004 11:02
To: 'edelmare-at-MUOhio.edu'; MicroscopyListServer

An inexpensive possibility...

The accelerometer may need a signal conditioner/buffer/amplifier - I have
not checked it's specifications. If a PC sound card meets your frequency
range and resolution requirements, the rest is simple and cheap.

A number of free/shareware programs that will turn your PC into an audio
range spectrum analyzer are available. Adjust the accelerometer/amplifier
output level to be compatible with the sound card "line in" requirement
(typically 1 volt peak, max)and you are there...

Regards,
Woody

Woody White
BWXT Services:
http://www.bwxt.com/bwxt.html
My Site:
http://woody.white.home.att.net

-----Original Message-----
} From: Richard Edelmann [mailto:edelmare-at-MUOhio.edu]
Sent: Tuesday, August 31, 2004 8:34 AM
To: microscopy-at-MSA.Microscopy.com

With a number of on-going building modifications here as well as the

potential for relocating my EM Facility. we find ourselves in need of a
vibration
testing/monitoring system. What I am hoping to find is a simply system to
plug into a Laptop. Having had various vibration testing done in the past,
and
where as I fully acknowledge the quality experience of testing service
providers we just can't afford that kind of expense on a continuing basis.
We
are looking to do this in-house, monitor "baseline" building vibrations
every
couple of weeks or so.

I have picked up the recommendations for a Wilcoxon 731A/P31
Accelerometer but now I need a compatible PCMCIA spectrum analyzer
interface board and software.

Any recommendations? And yes, vendors may respond directly back
to
me.

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 07:36:56 2004

Contents Retrieved from Microscopy Listserver Archives
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Group,
In my view, simple inkjet printers do an extraordinary job.
You can get one for 200 us dollars (or more or less depending on
features). What is important is that the quality of the output is
determined by the paper you put in (and some software toggles in the
printer driver). So, there is a range of paper from high quality
photo paper to zerox paper, with the cost per print scaling
appropriately (and the time per print likewise). This makes it easy
to get low, intermediate, high quality output on the same printer,
with little fuss. And I have to say that for monochrome prints, the
highest quality settings/paper produce prints equal to anything I
have seen from the wetlab type of printers mentioned below. And even
for color the differences are pretty small.
Another issue is networking. The inexpensive inkjet that I
have is not network-able (that's an intersting word) and I don't know
if the more expensive ones give you that option.

My two pixels,
Tobias

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 08:13:25 2004

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I have already starting campaigning for a digital camera
for our TEM!

I saw an advert in Microscopy and Analysis for a company
which is (presumably) starting making TEM film as others
leave the market.

Kodak did say recently on this listserver that they have no
plans to drop EM film.

Dave

On Fri, 03 Sep 2004 09:05:45 +0100 Chris Jeffree
{c.jeffree-at-ed.ac.uk} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} In the same week there is news of significant change in two of the
} companies that were
} major players in silver image photography in the 20th century.
} Ilford has shed almost half its staff preparative to sale of the
} traditional photographic
} business while it is still a going concern, allowing the company to
} focus on its Swiss digital business.
} http://www.channel4.com/news/news_story.jsp?storyId=156722
} Agfa has shed its traditional photographic film and consumer imaging
} business in a management buyout so that it can "focus on its core
} growth markets of Graphic Systems and HealthCare, which are rapidly
} going digital"
} http://news.agfa.com/corporate/news.nsf/news/F07C0210ECC86EA9C1256EF3004D27CE?opendocument
}
} Events like these, and Kodak's announcement earlier this year that it
} would cease the production of its poneering APS cameras (though not of
} films) underline the fragility of the conventional photographic
} market in the face of the growth of digital imaging.
}
} Which begs the question "can we rely on the continued availability of
} EM film", and if not, how long have we got
} to plan for the conversion to digital?
}
}
} Dr. Chris Jeffree
} University of Edinburgh
} Schoolof Biological Sciences
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 09:21:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Kodak has included a positive statement on its continued commitment to film
products in its contribution to the "New and Interesting at M&M 2004"
section of the September issue of Microscopy Today, at the printer now and
in your mail boxes starting in a week or so.

Ron Anderson, MT Editor

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Friday, September 03, 2004 4:06 AM
To: microscopy-at-msa.microscopy.com

In the same week there is news of significant change in two of the
companies that were
major players in silver image photography in the 20th century.
Ilford has shed almost half its staff preparative to sale of the
traditional photographic
business while it is still a going concern, allowing the company to
focus on its Swiss digital business.
http://www.channel4.com/news/news_story.jsp?storyId=156722
Agfa has shed its traditional photographic film and consumer imaging
business in a management buyout so that it can "focus on its core
growth markets of Graphic Systems and HealthCare, which are rapidly
going digital"
http://news.agfa.com/corporate/news.nsf/news/F07C0210ECC86EA9C1256EF3004D27C
E?opendocument

Events like these, and Kodak's announcement earlier this year that it
would cease the production of its poneering APS cameras (though not of
films) underline the fragility of the conventional photographic
market in the face of the growth of digital imaging.

Which begs the question "can we rely on the continued availability of
EM film", and if not, how long have we got
to plan for the conversion to digital?

Dr. Chris Jeffree
University of Edinburgh
Schoolof Biological Sciences

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 10:40:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,

I recently learned that Serco-Ilford is no more and I need service for my
2150RC. Does anyone know of anyone serving the New England area? Thanks in
advance.

Mary

Mary McKee
Program in Membrane Biology
MGH-Charlestown
(617)726-3696
--

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 11:18:33 2004

Contents Retrieved from Microscopy Listserver Archives
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I freeze with DMP-30 in the tube. Generally I aliquot them so they are
only thawed once. They are certainly good for a couple of weeks this way
and longer in many cases. I make all my resin by weight (typically 20 g
Embed 812, 10 g DDSA, 10 g NMA, and 0.6 g DMP-30) in a 50 ml plastic
disposable tube and shake vigorously until well mixed. We used 0.8 g BDMA
in place of DMP-30 in this formulation and saw no difference in cutting
quality but did have the storage problem. The viscosity of the DDSA and
NMA and Embed 812 is high and requires vigorous shaking regardless of the
catylst so I don't see lower viscosity of BDMA as significant if you are
measuring by weight. If you measure by volume, a viscous solution will be
tougher to accurately measure and deliver and the percent error will be
much higher for the small volume BDMA or DMP-30 component. I have never
ever seen the DMP-30 come out of solution such as Caroline Schooley
suggests in her e-mail; if this happens I would suspect improper
mixing. My use of DMP-30 is based on careful consideration and comparison
with BDMA and not on tradition. I used BDMA exclusively for over 1 year
and then switched back so I think I gave it a fair shot.

At 10:22 AM 09/03/04 -0600, you wrote:
} I have a question about freezing the resin mixtures - you freeze them with
} the accelerator already added? How many freeze/thaw cycles can they stand?
} Or, do you aliquot them to store and thaw only once?? I was taught to
} store mine without DMP-30....if they'll last OK with it in, I'm all for it!
}
} Thanks,
}
} Tamara
}
} On Thu, 2 Sep 2004, Tom Phillips wrote:
}
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 11:35:01 2004

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For a less viscous mixture, you could try one percent DMP-30 instead of
two percent. The final cure might not be quite so hard, though, so
depending on your tissue this may or may not help.

Lesley Weston.

----- Original Message -----
} From: walter.bobrowski-at-pfizer.com (by way of MicroscopyListserver)
Sent: 9/2/2004 11:08:46 AM
To: microscopy-at-microscopy.com

} -
}
} I freeze with DMP-30 in the tube. Generally I aliquot them so they
} are only thawed once. They are certainly good for a couple of weeks
} this way and longer in many cases. I make all my resin by weight
} (typically 20 g Embed 812, 10 g DDSA, 10 g NMA, and 0.6 g DMP-30) in
} a 50 ml plastic disposable tube and shake vigorously until well
} mixed. We used 0.8 g BDMA in place of DMP-30 in this formulation
} and saw no difference in cutting quality but did have the storage
} problem. The viscosity of the DDSA and NMA and Embed 812 is high
} and requires vigorous shaking regardless of the catylst so I don't
} see lower viscosity of BDMA as significant if you are measuring by
} weight. If you measure by volume, a viscous solution will be tougher
} to accurately measure and deliver and the percent error will be much
} higher for the small volume BDMA or DMP-30 component. I have never
} ever seen the DMP-30 come out of solution such as Caroline Schooley
} suggests in her e-mail; if this happens I would suspect improper
} mixing. My use of DMP-30 is based on careful consideration and
} comparison with BDMA and not on tradition. I used BDMA exclusively
} for over 1 year and then switched back so I think I gave it a fair
} shot.

You missed my point, Tom; when I said that the DMP-30 can partition
during infiltration, I meant that it doesn't enter the tissue as
rapidly as the other resin components. The symptom is soft tissue in
a normal, hard block. I agree with you that the high DMP-30
viscosity is going to have little effect on the viscosity of the
mixed epoxy.

Caroline
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 15:21:20 2004

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Do you have evidence that the DMP-30 doesn't get in or is that your
hypothesis to explain the problem? How do you know it is a sign that the
DMP-30 didn't get in and not the complete mixture or one of the equally
viscous components? I find it hard to believe the DMP-30 differentially
inflitrates. In addition, the DMP-30 (and BDMA) has probably already begun
to react with the other components and would be "carried" in covalently
bound to the one of them. Poor infiltration of the entire mix would (and
does) result in the symptom you describe. Take a resin mix made with BDMA
and do a short infiltration on a tough to infiltrate tissue like maize
endosperm and the center will be softer than the perimeter and free resin
regions. BDMA is frequently touted as superior due to its lower viscosity
and less hydrophilic. It is lower viscosity but I don't see that as a
problem or benefit. I have no data on the relative hydroscopic properties
but I have never had a bottle of DMP-30 go bad on me in the 25 years I have
been doing TEM. Maybe I use my bottles up before they goes bad. We do
close it up promptly after using but I assume most labs do. I have nothing
against BDMA if one is making the resin up fresh each time (which is the
best practice regardless of whether you use BDMA or DMP-30). But for our
routine samples, we commonly make 40-50 gm batches and store the resin at
-20 C for 1-3 weeks. This works when we use DMP-30 but not with BDMA. I
agree that lots of what microscopists do is because of "tradition" but the
selection of DMP-30 can be the result of a careful, reasoned and
experimentally tested decision process. Tom Phillips

At 01:21 PM 09/03/04 -0700, you wrote:
} } -
} }
} } I freeze with DMP-30 in the tube. Generally I aliquot them so they are
} } only thawed once. They are certainly good for a couple of weeks this way
} } and longer in many cases. I make all my resin by weight (typically 20 g
} } Embed 812, 10 g DDSA, 10 g NMA, and 0.6 g DMP-30) in a 50 ml plastic
} } disposable tube and shake vigorously until well mixed. We used 0.8 g
} } BDMA in place of DMP-30 in this formulation and saw no difference in
} } cutting quality but did have the storage problem. The viscosity of the
} } DDSA and NMA and Embed 812 is high and requires vigorous shaking
} } regardless of the catylst so I don't see lower viscosity of BDMA as
} } significant if you are measuring by weight. If you measure by volume, a
} } viscous solution will be tougher to accurately measure and deliver and
} } the percent error will be much higher for the small volume BDMA or DMP-30
} } component. I have never ever seen the DMP-30 come out of solution such
} } as Caroline Schooley suggests in her e-mail; if this happens I would
} } suspect improper mixing. My use of DMP-30 is based on careful
} } consideration and comparison with BDMA and not on tradition. I used BDMA
} } exclusively for over 1 year and then switched back so I think I gave it a
} } fair shot.
}
} You missed my point, Tom; when I said that the DMP-30 can partition during
} infiltration, I meant that it doesn't enter the tissue as rapidly as the
} other resin components. The symptom is soft tissue in a normal, hard
} block. I agree with you that the high DMP-30 viscosity is going to have
} little effect on the viscosity of the mixed epoxy.
}
} Caroline
} --
} Caroline Schooley
} Project MICRO Coordinator
} Microscopy Society of America
} Box 117, 45301 Caspar Point Road
} Caspar, CA 95420
} Phone/FAX (707)964-9460
} Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
} Intertidal invertebrates: http://www.fortbragg.k12.ca.us/AG/marinelab.html

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 20:08:29 2004

Contents Retrieved from Microscopy Listserver Archives
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I'm looking for sources of acoustic/anachoic
blocks of foam to reduce SEM room interference.

These are like standard anechoic chamber panels.
I'm having trouble getting above 400KX without
mechanical noise from the scroll pump that is
located in a separate room. The acoustical
isolation from one room to the other is not
all that great, I suppose.

Does anyone have experience with suppliers of
these panels? I'd like to glue them to drywall.

Supplier responses are welcomed as off-line
messages.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 3 21:05:34 2004

Contents Retrieved from Microscopy Listserver Archives
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Gary,

You can try http://www.illbruck-sonex.com/ for what you need. I'm familiar
with this product when we used it at the High Voltage EM lab at UW Madison.
Worked well.

Damian Neuberger

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Friday, September 03, 2004 8:31 PM
To: MSA listserver

I'm looking for sources of acoustic/anachoic
blocks of foam to reduce SEM room interference.

These are like standard anechoic chamber panels.
I'm having trouble getting above 400KX without
mechanical noise from the scroll pump that is
located in a separate room. The acoustical
isolation from one room to the other is not
all that great, I suppose.

Does anyone have experience with suppliers of
these panels? I'd like to glue them to drywall.

Supplier responses are welcomed as off-line
messages.

gary g.

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 4 07:05:23 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Researchers:

           We use a Polaroid SprintScan 45 multi-format film scanner to
scan our EM negatives. It has been a work horse for us for 7 years, and
the hardware is still in a good shape. However, We lost the original
disk with driver (for Mac) on it and we could not get support from the
company anymore because Polaroid has discontinued scanner
business. Does anyone out there have the same scanner and would be
willing to lend us the driver software? Our machine is currently down
because the computer could not locate it even though the scanner was on
and all cables were connected. We need to re-install the driver as the
first trouble shooting step.

           If we can not find a driver, we might have to purchase a new
film scanner. Does anyone has a recommendation on makes and models?

           Thank you very much in advance.


Hong
Emory EM
hyi-at-emory.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 4 11:39:26 2004

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Bill Robertson in his reply posting pointed out
a very good point about wall mass. My initial
thoughts were to put the acoustic tiles in the SEM room.
But the noise is more likely coming from the adjacent
room where the scroll pump and specimen interchange
pump are located. The specimen interchange pump
is not at issue. The scroll pump is an Edwards XDS 10.
Based on limited experience, it does not sound like
it is running as it should. Vacuum is fine but the
sound is odd. It makes a mechanical knocking noise.
I'm told that either these pumps work almost forever
when new or die quickly. Sounds like I have the latter.

In either case, wall mass has a high probability
of attention. The intervening wall is standard
drywall with 2x4 studs. There is no insulation
in the wall. I'm thinking of having liquid foam
insulation put in the wall cells and seeing if that
helps. In the mean time, the plinth anti-vibration
system is not exactly right and will get adjusted
shortly. then, based on how that turns out, acoustic
tiles in the pump room may be a good solution. If that
does not help much, then foam insulation.

The chiller is in the same room as the SEM but turning
it off makes no change in image noise. So the noise
is external.

Thanks for the replies. Will work on this in the
next couple of weeks.

gary g.

At 08:38 AM 9/4/2004, you wrote:
} Gary,
}
} They can be pricey. One reason is that most jurisdictions require that
} insulation
} applied to an open wall surface be flame proof. Not only that, the
} adhesive used
} to apply it must also be flame proof, per the fire department and building
} codes.
} (Recall the disasterous fire in the Rhode Island night club a couple years
} back).
} Some years ago I found that the material required behind an XRD system in
} a small
} room ran several hundred dollars for a half dozen panels. However, I
} found that I
} could get a big improvement by placing a small number of them so as to
} block the
} noise at the source, rather than covering the more distant wall
} surfaces. Buy a
} small number to try out, or experiment with packing foam. Have an
} assistant hold
} them in different locations so as to block acoustic reflections. You may
} find that
} suspending one from the ceiling in the plane of the instrument helps alot with
} noise at the position where the operator sits.
}
} John Twilley
}
} Gary Gaugler wrote:
}
} }
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} -------------------------------------------------------------------------------
} }
} } I'm looking for sources of acoustic/anachoic
} } blocks of foam to reduce SEM room interference.
} }
} } These are like standard anechoic chamber panels.
} } I'm having trouble getting above 400KX without
} } mechanical noise from the scroll pump that is
} } located in a separate room. The acoustical
} } isolation from one room to the other is not
} } all that great, I suppose.
} }
} } Does anyone have experience with suppliers of
} } these panels? I'd like to glue them to drywall.
} }
} } Supplier responses are welcomed as off-line
} } messages.
} }
} } gary g.

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 4 11:44:55 2004

Contents Retrieved from Microscopy Listserver Archives
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I was a fan of Epson photo printers for quite
some time. Notable was the 890 & 980. It is a
small format printer compared to the 2200.
I recently (a year or so ago) bought a Epson Stylus
Photo 2000. It lasted about six months and
then jammed constantly. In-warranty customer
service and any idea of repair was on a wish list.
It never happened. The printer was scrapped.

The 2200 may have solved teething problems
with large format printers. However, the 2000
was VERY slooooow using photo paper. When it
worked, the results were stunning. Many times
(too many) it would stop printing 1/4 or 1/2
way through the print and just die. The job
hung (Win2K Pro) and had to be restarted with
a new sheet of paper.

The Epson and Canon small format printers seem
to do a better, more reliable job. As a result
of being burned by Epson, I now take print jobs
to a local service bureau. they do a very nice
job for not much cost. These are mostly for
24" x 48" glossy mounted prints. Small ones
are done on my HP 4550 color laser printer.
If the color gamut is matched well between
the monitor and Photoshop, the HP does a nice job
for reports. For transparencies (not much used
any longer), the Kodak dye sub is excellent.

Let us know what you find. There are a lot
of options. Also, check out the Ethernet print
servers that will connect a non-network printer
to a LAN and allow all to use it. HP and others
make these. they usually cost about $100 or so.

gary g.

At 11:08 AM 9/2/2004, you wrote:

} Email: jtd1-at-psu.edu
} Name: Tom Doman
}
} Organization: Penn State University
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: Our lab is considering various photo printers (} $1K) for
} production of electron micrographs. Currently the Epson 2200 is the stromg
} favorite. Are there any recomendations for other printers which we should
} consider? What are your reasons for the recomended printer?
}
} Thanks in advance!
}
} Tom
}
} ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 4 13:33:46 2004

Contents Retrieved from Microscopy Listserver Archives
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From your description of the sound coming from your pump, it sounds
like your issue might be low frequency. For low frequencies, acoustic
tiles and the like are not very effective. The strategy for reducing
high frequencies is to absorb the energy, and usually involves foam or
fibruous materials that will vibrate and dissipate the energy. For low
frequencies, the strategy is to block/reflect the energy, and this
requires rigidity and mass. The best is a very solid wall, but there
are also a number of lead-backed sheet materials, either separately or
in combination with absorbers. If you have access to a McMaster Carr
catalog, I suggest you check out "Sound Absorbers" (or visit their web
site at www.mcmaster.com and do a keyboard search for "sound". There
is also a helpful summary on page 3266 of their online catalog which
explains the various types and ratings systems. (No financial interest
in McMaster Carr, but use them all the time.)
Fred Schamber
ASPEX, LLC

Gary Gaugler wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
}
} Bill Robertson in his reply posting pointed out
} a very good point about wall mass. My initial
} thoughts were to put the acoustic tiles in the SEM room.
} But the noise is more likely coming from the adjacent
} room where the scroll pump and specimen interchange
} pump are located. The specimen interchange pump
} is not at issue. The scroll pump is an Edwards XDS 10.
} Based on limited experience, it does not sound like
} it is running as it should. Vacuum is fine but the
} sound is odd. It makes a mechanical knocking noise.
} I'm told that either these pumps work almost forever
} when new or die quickly. Sounds like I have the latter.
}
} In either case, wall mass has a high probability
} of attention. The intervening wall is standard
} drywall with 2x4 studs. There is no insulation
} in the wall. I'm thinking of having liquid foam
} insulation put in the wall cells and seeing if that
} helps. In the mean time, the plinth anti-vibration
} system is not exactly right and will get adjusted
} shortly. then, based on how that turns out, acoustic
} tiles in the pump room may be a good solution. If that
} does not help much, then foam insulation.
}
} The chiller is in the same room as the SEM but turning
} it off makes no change in image noise. So the noise
} is external.
}
} Thanks for the replies. Will work on this in the
} next couple of weeks.
}
} gary g.
}
}
} At 08:38 AM 9/4/2004, you wrote:
}
} } Gary,
} }
} } They can be pricey. One reason is that most jurisdictions require
} } that insulation
} } applied to an open wall surface be flame proof. Not only that, the
} } adhesive used
} } to apply it must also be flame proof, per the fire department and
} } building codes.
} } (Recall the disasterous fire in the Rhode Island night club a couple
} } years back).
} } Some years ago I found that the material required behind an XRD
} } system in a small
} } room ran several hundred dollars for a half dozen panels. However, I
} } found that I
} } could get a big improvement by placing a small number of them so as
} } to block the
} } noise at the source, rather than covering the more distant wall
} } surfaces. Buy a
} } small number to try out, or experiment with packing foam. Have an
} } assistant hold
} } them in different locations so as to block acoustic reflections. You
} } may find that
} } suspending one from the ceiling in the plane of the instrument helps
} } alot with
} } noise at the position where the operator sits.
} }
} } John Twilley
} }
} } Gary Gaugler wrote:
} }
} } }
} } ------------------------------------------------------------------------------
} }
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America
} } } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } -------------------------------------------------------------------------------
} }
} } }
} } } I'm looking for sources of acoustic/anachoic
} } } blocks of foam to reduce SEM room interference.
} } }
} } } These are like standard anechoic chamber panels.
} } } I'm having trouble getting above 400KX without
} } } mechanical noise from the scroll pump that is
} } } located in a separate room. The acoustical
} } } isolation from one room to the other is not
} } } all that great, I suppose.
} } }
} } } Does anyone have experience with suppliers of
} } } these panels? I'd like to glue them to drywall.
} } }
} } } Supplier responses are welcomed as off-line
} } } messages.
} } }
} } } gary g.
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sun Sep 5 11:32:17 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jbarclay-at-southpointresources.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, September 5, 2004 at 08:40:08
---------------------------------------------------------------------------

Email: jbarclay-at-southpointresources.com
Name: Jim Barclay

Organization: Calgary, Alberta

Title-Subject: [Microscopy] [Filtered] Wild Heerbrug M5A microscope & camera attachment

Question: I am trying to see if I can find some type of adaptor that will fit my older Wild Heerbrug M5A binocular microscope (15-20 years old?) and allow me to fit a digital camera to the scope. I would need some type of beam splitter that would continue to allow simultaneosu viewing of samples while also allowing occasional photo taking.

I have already contacted and am waiting for reply from a Leica Microsystems representative which owns the Wild Leitz brand.

Thank you for listening to a newbie to this board. Any suggestions welcome.

JB.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Sep 5 17:01:07 2004

Contents Retrieved from Microscopy Listserver Archives
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On Sep 3, 2004, at 6:30 PM, Gary Gaugler wrote:

} I'm looking for sources of acoustic/anachoic
} blocks of foam to reduce SEM room interference.
}
} These are like standard anechoic chamber panels.
} I'm having trouble getting above 400KX without
} mechanical noise from the scroll pump that is
} located in a separate room. The acoustical
} isolation from one room to the other is not
} all that great, I suppose.
}
} Does anyone have experience with suppliers of
} these panels? I'd like to glue them to drywall.
}
} Supplier responses are welcomed as off-line
} messages.
}
Dear Gary,
Fred has it right about the difference between low and high
frequencies. The depth of the invaginations in anechoic panels has to
be 1/4 of the wavelength of the sound in order to be effective, so for
low frequencies, the panels could take up the entire room, leaving no
space for the equipment.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Sun Sep 5 18:43:56 2004

Contents Retrieved from Microscopy Listserver Archives
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I don't have any direct way of knowing whether the
noise is high or low frequency. It only shows up
above 60KX as sinusoids on the edges of specimen
details.

I can probably use FFT to compute the frequency.
It is consistent.

gary g.

At 03:34 PM 9/5/2004, you wrote:

} On Sep 3, 2004, at 6:30 PM, Gary Gaugler wrote:
}
} } I'm looking for sources of acoustic/anachoic
} } blocks of foam to reduce SEM room interference.
} }
} } These are like standard anechoic chamber panels.
} } I'm having trouble getting above 400KX without
} } mechanical noise from the scroll pump that is
} } located in a separate room. The acoustical
} } isolation from one room to the other is not
} } all that great, I suppose.
} }
} } Does anyone have experience with suppliers of
} } these panels? I'd like to glue them to drywall.
} }
} } Supplier responses are welcomed as off-line
} } messages.
} Dear Gary,
} Fred has it right about the difference between low and high
} frequencies. The depth of the invaginations in anechoic panels has to be
} 1/4 of the wavelength of the sound in order to be effective, so for low
} frequencies, the panels could take up the entire room, leaving no space
} for the equipment.
} Yours,
} Bill Tivol, PhD
} EM Scientist and Manager
} Cryo-Electron Microscopy Facility
} Broad Center, Mail Code 114-96
} California Institute of Technology
} Pasadena CA 91125
} (626) 395-8833
} tivol-at-caltech.edu
}
}

From MicroscopyL-request-at-ns.microscopy.com Sun Sep 5 23:13:35 2004

Contents Retrieved from Microscopy Listserver Archives
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If you are building a wall that may transmuted vibration making the
wall a 6 inch wall with double 4 inch studs that are every 8 inches
with every other stud supporting opposite faces of the wall. If you
use a sound deadening blanket widen the wall to leave room to weave
the padding between the studs with out compressing it.

Two layers of 5/8 inch gypsum wall board are generaly considered
fire proof enough for university buildings at Oklahoma State. The
last I knew there were no paints that could be used on anything but
aluminum to increase their fire rating. But that has been a while.
In actual practice there are paints that improve the fire resistance
of anything but last I knew it changed so much with age that for
anything but metal it was too unpredictable to approve.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Gary Gaugler" {gary-at-gaugler.com}
:
: Bill Robertson in his reply posting pointed out
: a very good point about wall mass. My initial
: thoughts were to put the acoustic tiles in the SEM room.
: But the noise is more likely coming from the adjacent
: room where the scroll pump and specimen interchange
: pump are located. The specimen interchange pump
: is not at issue. The scroll pump is an Edwards XDS 10.
: Based on limited experience, it does not sound like
: it is running as it should. Vacuum is fine but the
: sound is odd. It makes a mechanical knocking noise.
: I'm told that either these pumps work almost forever
: when new or die quickly. Sounds like I have the latter.
:
: In either case, wall mass has a high probability
: of attention. The intervening wall is standard
: drywall with 2x4 studs. There is no insulation
: in the wall. I'm thinking of having liquid foam
: insulation put in the wall cells and seeing if that
: helps. In the mean time, the plinth anti-vibration
: system is not exactly right and will get adjusted
: shortly. then, based on how that turns out, acoustic
: tiles in the pump room may be a good solution. If that
: does not help much, then foam insulation.
:
: The chiller is in the same room as the SEM but turning
: it off makes no change in image noise. So the noise
: is external.
:
: Thanks for the replies. Will work on this in the
: next couple of weeks.
:
: gary g.
:
:
: At 08:38 AM 9/4/2004, you wrote:
: } Gary,
: }
: } They can be pricey. One reason is that most jurisdictions
require that
: } insulation
: } applied to an open wall surface be flame proof. Not only that,
the
: } adhesive used
: } to apply it must also be flame proof, per the fire department and
building
: } codes.
: } (Recall the disasterous fire in the Rhode Island night club a
couple years
: } back).
: } Some years ago I found that the material required behind an XRD
system in
: } a small
: } room ran several hundred dollars for a half dozen panels.
However, I
: } found that I
: } could get a big improvement by placing a small number of them so
as to
: } block the
: } noise at the source, rather than covering the more distant wall
: } surfaces. Buy a
: } small number to try out, or experiment with packing foam. Have
an
: } assistant hold
: } them in different locations so as to block acoustic reflections.
You may
: } find that
: } suspending one from the ceiling in the plane of the instrument
helps alot with
: } noise at the position where the operator sits.
: }
: } John Twilley
: }
: } Gary Gaugler wrote:
: }
: } }
:
} ------------------------------------------------------------------
------------
: } } The Microscopy ListServer -- Sponsor: The Microscopy Society
of America
: } } To Subscribe/Unsubscribe --
: } http://www.msa.microscopy.com/MicroscopyListserver
: } } On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
: } }
:
} ------------------------------------------------------------------
-------------
: } }
: } } I'm looking for sources of acoustic/anachoic
: } } blocks of foam to reduce SEM room interference.
: } }
: } } These are like standard anechoic chamber panels.
: } } I'm having trouble getting above 400KX without
: } } mechanical noise from the scroll pump that is
: } } located in a separate room. The acoustical
: } } isolation from one room to the other is not
: } } all that great, I suppose.
: } }
: } } Does anyone have experience with suppliers of
: } } these panels? I'd like to glue them to drywall.
: } }
: } } Supplier responses are welcomed as off-line
: } } messages.
: } }
: } } gary g.
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 01:14:19 2004

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chris, ron, and everyone else...

not wanting to sound paranoid, i think we have to consider chris's words
carefully.

while digital systems are good, after 35 years i cannot get the same
results from a digital image than i can from film, no matter how hard i
try. double exposures with polychromatic paper using different filters,
dodging, burning, combined, can contribute to excellent prints. perhaps
others can get the same results from digitized images, after 5 years, i
cannot.

we currently maintain two older Philips 201 and one cm10 microscopes.
they have 35mm cameras. Kodak has discontinued manufacture of Direct
Positive 5302, which we use for these instruments. the only sources of
which i now know for this film is the different suppliers. but how long
will their stocks last? what other 35mm format films are there that
have the same high resolution that is found with 5302?

all in all, the promise from Kodak is fine and dandy, but will that hold
when Kodak decides that the digital market has made it no longer viable
to support wet chemistry with specialized, high resolution films such as
we require.

of course, as far as i am concerned, i have 25 roles of 5302 in the
freezer, so i'm set until our microscopes die. but it is an ongoing
concern for the rest of you who were not ordering at the time that Kodak
made their decision and were not able to stock up.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 01:57:23 2004

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Dear Mr. Barclay,

we produce c-mount adapters which can be connected to the
eyepiece of a microscope. The eyepiece remains in place, you
put our eyepiece adapter on top of it. Our eyepiece adapter
has a lens built-in. This has the advantage of capturing most
of what you see through the eyepiece. You can easily remove
the adapter and look through the eyepiece again. We offer
different sizes of eyepiece adapters. We also manufacture on
demand.

If you would like to get more information please contact me.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

bwoM} ------------------------------------------------------------------------------
bwoM} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
bwoM} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
bwoM} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
bwoM} -------------------------------------------------------------------------------

bwoM} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jbarclay-at-southpointresources.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
bwoM} Sunday, September 5, 2004 at 08:40:08
bwoM} ---------------------------------------------------------------------------

bwoM} Email: jbarclay-at-southpointresources.com
bwoM} Name: Jim Barclay

bwoM} Organization: Calgary, Alberta

bwoM} Title-Subject: [Microscopy] [Filtered] Wild Heerbrug M5A microscope & camera attachment

bwoM} Question: I am trying to see if I can find some type of adaptor that will fit my older Wild Heerbrug M5A binocular microscope (15-20 years old?) and allow me to fit a digital camera to the
bwoM} scope. I would need some type of beam splitter that would continue to allow simultaneosu viewing of samples while also allowing occasional photo taking.

bwoM} I have already contacted and am waiting for reply from a Leica Microsystems representative which owns the Wild Leitz brand.

bwoM} Thank you for listening to a newbie to this board. Any suggestions welcome.

bwoM} JB.

bwoM} ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 02:20:34 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Chris Jeffree wrote the following:
======================================================================
In the same week there is news of significant change in two of the
companies that were
major players in silver image photography in the 20th century.
Ilford has shed almost half its staff preparative to sale of the
traditional photographic
business while it is still a going concern, allowing the company to
focus on its Swiss digital business.
http://www.channel4.com/news/news_story.jsp?storyId=156722
Agfa has shed its traditional photographic film and consumer imaging
business in a management buyout so that it can "focus on its core
growth markets of Graphic Systems and HealthCare, which are rapidly
going digital"
http://news.agfa.com/corporate/news.
nsf/news/F07C0210ECC86EA9C1256EF3004D27CE?opendocument

Events like these, and Kodak's announcement earlier this year that it would
cease the production of its poneering APS cameras (though not of films)
underline the fragility of the conventional photographic market in the face
of the growth of digital imaging.

Which begs the question "can we rely on the continued availability of
EM film", and if not, how long have we got
to plan for the conversion to digital?
============================================================================
Chris is correct in that there has been a real decline worldwide of emulsion
based photographic products.

But for the TEM film, the main people who are spreading the "fear" of a
"filmless day" soon to arrive are the ones who would benefit the most if one
did convert to all digital recording. There could be legitimate reasons to
do that, of course, but the inability to purchase high quality TEM film is
not going to be one of them at least not in the near and intermediate term
future. And besides, someone with a ten or more year old TEM probably is
not going to be too keen on making the large capital investment needed to
convert to digital anyhow, since the digital add-on would be worth far more
than the TEM onto which it is going.

When a large manufacturer decides to get out of a particular business, it is
not at all uncommon or unusual for them to find a smaller firm to continue
the manufacturing, marketing and distribution of the soon-to-be discontinued
product. This makes sense ethically as well since that way they don't leave
their existing customers "cut off at their knees". And what would seem like
"peanuts" to a large global manufacturer if not also a nuisance could be
seen as gigantic volume to a much smaller firm. This kind of licensing of
"mature" products being discontinued goes on all the time, including even
the marketplace for TEM film. For example, when Agfa " discontinued" the
Agfa Scientia brand of TEM film, they licensed a highly reputable German
photographic film manufacturing firm, MACO, to continue to manufacturer the
TEM films that users around the world had used for their work. And the MACO
TEM film is available from PLANO in Germany and from SPI Supplies everywhere
else. Everyone can rest well assured that MACO will continue to manufacture
TEM film well into the future, farther in fact than most would even want to
look.

More information and prices about the MACO film could be found at URL
http://www.2spi.com/catalog/photo/maco-TEM-film.html

Disclaimer: SPI Supplies is the worldwide distributor for the MACO TEM film
so we have an obviously vested interest in publicizing that fact.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 05:32:46 2004

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Chuck
Thanks for this clear statement of the position, which will surely
reassure many
TEM users like myself with a middle-aged instrument and little
prospect
of going digital at the moment. I will try to relax, but our
audio-visual services have
just refreshed my paranoia by announcing that they are no longer able
to source 35mm
slide projectors and lenses suitable for use in lecture theatres. (Is
that really true??)
We are therefore being encouraged to reduce our dependence on slides.

Best wishes
Chris

Dr. Chris Jeffree

----- Original Message -----
} From: "Garber, Charles A." {cgarber-at-2spi.com}
To: "MICROSCOPY BB" {Microscopy-at-MSA.Microscopy.com}
Sent: Monday, September 06, 2004 9:45 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (stokes-at-saturn.med.nyu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, September 5, 2004 at 19:04:28
---------------------------------------------------------------------------

Email: stokes-at-saturn.med.nyu.edu
Name: David Stokes

Organization: NYU Skirball Inst

Title-Subject: [Microscopy] [Filtered] EM Core Director

Question: The Skirball Institute of New York University School of Medicine seeks an individual to set up and direct an imaging core facility with an initial emphasis on electron microscopy. The Skirball Insitute, located in midtown Manhattan, consists of 35 laboratories with a diverse array of biomedical research projects, which are described in detail at http://saturn.med.nyu.edu. Individual laboratories currently operate two electron microscopes and several confocal microscopes together with various ancillary equipment for specimen preparation and image analysis. To organize these into a shared facility, we seek an individual with extensive experience in conventional thin sectioning and immunolabeling of biological organisms. The ideal individual will also have management skills and an ambition to develop a comprehensive facility with additional staff offering a wide range of imaging services. Applicants should send their curriculum vitae along with the names and addresses of three references to: Dr. David Stokes at stokes-at-saturn.med.nyu.edu.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 08:13:55 2004

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Can anyone recommend a good commercial photolab that is
also reasonably priced, for scanning hundreds of 35 mm
slides and saving on CDs?

Sandra K. Masur, PhD
Prof. Ophthalmology
MSSM
NYC

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 14:57:27 2004

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Hi People

We here at the end of the world have already suffered from this "problem" for the last 4 or 5 years where Kodak could not supply us with "EM" grade film.
We still use film for all the reasons already quoted; particularly that it still produces the best results compared to digital.

Four years ago we switched suppliers to Agfa and use a product called Copex Positive Pet 10.
Code number 2OYAT CNP3 NP EI
This is in the 35mm format

Good Luck
Raymond Bennett

Keith Williamson EM Unit
HortResearch
Private Bag 11030
Palmerston North
NEW ZEALAND

} } } Paul Hazelton {paul_hazelton-at-umanitoba.ca} 09/06/04 4:06:52 a.m. } } }

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The Microscopy ListServer -- Sponsor: The Microscopy Society of America

chris, ron, and everyone else...

not wanting to sound paranoid, i think we have to consider chris's words
carefully.

while digital systems are good, after 35 years i cannot get the same
results from a digital image than i can from film, no matter how hard i
try. double exposures with polychromatic paper using different filters,
dodging, burning, combined, can contribute to excellent prints. perhaps
others can get the same results from digitized images, after 5 years, i
cannot.

we currently maintain two older Philips 201 and one cm10 microscopes.
they have 35mm cameras. Kodak has discontinued manufacture of Direct
Positive 5302, which we use for these instruments. the only sources of
which i now know for this film is the different suppliers. but how long
will their stocks last? what other 35mm format films are there that
have the same high resolution that is found with 5302?

all in all, the promise from Kodak is fine and dandy, but will that hold
when Kodak decides that the digital market has made it no longer viable
to support wet chemistry with specialized, high resolution films such as
we require.

of course, as far as i am concerned, i have 25 roles of 5302 in the
freezer, so i'm set until our microscopes die. but it is an ongoing
concern for the rest of you who were not ordering at the time that Kodak
made their decision and were not able to stock up.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

______________________________________________________

The contents of this e-mail are privileged and/or confidential to the
named recipient and are not to be used by any other person and/or
organisation. If you have received this e-mail in error, please notify
the sender and delete all material pertaining to this e-mail.
______________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 15:59:54 2004

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TEM Research Scientist

Industrial Research Limited is New Zealand's leading industrial scientific research organisation. Our role is to develop leading-edge technologies into practical business opportunities (http://www.irl.cri.nz).

IRL is strengthening its research efforts in the area of superconducting materials and is now seeking expressions of interest from suitably qualified scientists for a two year Post-doctoral position, at our Gracefield site (near Lower Hutt, Wellington). This is an opportunity to join an internationally renowned team working on both Government and industry funded projects in the area of superconducting technologies.

Key responsibilities, knowledge and qualifications:
* To undertake applied research and development projects in superconducting materials, including the preparation and analysis of samples of so-called "2nd generation" Yttrium Barium Copper OxideYBCO tapes
* PhD or equivalent in materials science or a related field with a focus on TEM work.
* Experience in preparing TEM samples of composite materials is highly desirable
* To develop and contribute to the development of new research areas
* To take an active role in the technology transfer process
* Experience with superconducting materials is desirable but not essential
*
*
* The successful applicant will possess:
* Strong aptitude for experimental research and development
* Demonstrated TEM experience
* Good planning, organisational and problem solving skills
* An ability to work independently and as part of a team
* Superior oral and written communication skills

An attractive remuneration package commensurate with qualifications and experience will be offered to the successful candidate as well as a wonderful opportunity to live in a vibrant capital city in a country renowned for its quality of life and outdoor activities.

'Expressions or Interest' are invited and should be forwarded by 17 September 2004 to: Jennie Scott, Industrial Research Limited, P O Box 31-310, Lower Hutt, Wellington,
Phone: (04) 931 3094, Fax: (04) 569 0019, E-mail: j.scott-at-irl.cri.nz {mailto:j.scott-at-irl.cri.nz} .

Industrial Research Limited is an Equal Opportunities Employer

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 16:26:07 2004

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chuck

i had been thinking of looking up agfa, then they went out of the
field. does MACO produce a 35mm film, and is it of similar grain?

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 20:12:30 2004

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-----Original Message-----
} From: Paul Hazelton [mailto:paul_hazelton-at-umanitoba.ca]
Sent: Sunday, September 05, 2004 11:07 AM

double exposures with polychromatic paper using different filters,
dodging, burning, combined, can contribute to excellent prints.

---------------------------------------

I don't mean to sound sarcastic, and I know it's going to, so please
understand that's not how I mean it.

How is the above different from manipulating a digital image?

I guess there are two parts to the question. First, is this any less of
a manipulation (and hence potential for inaccurate or inappropriate
artifacts) than using digital techniques to improve the appearance of an
image? I mention this in the context of other discussions on digital
image integrity.

Second, is the specific problem you're describing a limit of digital
technology, or a limit of the skills and resources available? It is
certainly a different set of skills to work in a "wet" darkroom than
that used in the "digital" darkroom. (Having worked some in both, I too
found the digital harder. None the less, I can see where given the
right set of tools and skills, the "useable quality" of digital and film
could be equal.)

John R.

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 21:41:28 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Raymond Bennett wrote:
===============================================
We here at the end of the world have already suffered from this "problem"
for the last 4 or 5 years where Kodak could not supply us with "EM" grade
film.
We still use film for all the reasons already quoted; particularly that it
still produces the best results compared to digital.
===============================================
I am sympathetic to your problem but it is a different kind of problem, not
to be confused with the issue already being discussed on the listserver.
Your problem is a distribution problem and is the result of the way Kodak
(and other manufacturers) distribute(s) their films and other photographic
products. Now I am not the last word on this but I am sure someone from
Kodak would correct me quite quickly should I be wrong.

My perception is that Kodak establishes an exclusive distributorship,
sometimes their own subsidiary, to distribute film in a specific market,
such as NZ. But it is up to that particular distributor to decide what they
will either a) keep in stock or b) "handle" even on special order.
Unfortunately, too many such distributors decide that because the volume is
so low, and perhaps they don't want to end up with stale-dated film, they
just don't want to be bothered with the handling of such a specialty item
like the EM films so they tell their customers it is "not available" but of
course, they are really saying it is not available from them, even thought
it certainly could be avalable generally, such as in the USA or other
countries.

That is why so many end users in New Zealand purchase their Kodak EM film
from those firms already providing EM consumables, such as SPI Supplies, Ted
Pella, or Ladd (to name a few) in the USA. By ordering this way, you can
combine all your other needs for TEM supplies and consumables and the end
result is that the incremental shipping costs associated with the film can
become almost negligible if not zero. This problem is far from being
limited to NZ and in fact gets repeated in many other countries and markets
around the world.

With regard to getting superior results with film vs.digital, I hear this
all the time, but some would say it would depend on the quality of the
digital system you are using to make the comparison. Could you comment on
what digital system you used to make your comparison? Those of us who have
not converted yet could find your answer very interesting.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 22:09:56 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Paul R. Hazelton wrote:
============================================================================
==
i had been thinking of looking up agfa, then they went out of the field.
does MACO produce a 35mm film, and is it of similar grain?
============================================================================
===
Was this a 35 mm film that actually went into the vacuum of the TEM or are
you talking about using it with a camera that photographed the screen
through a viewing glass from outside the vacuum? Do you have a former Agfa
product number?

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 6 23:01:14 2004

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john

certainly your comments are taken well. probably because i agree, and
that the whole intent of what i said is that i can manipulate the images
much better with wet chemistry after 35 years than i can after 4-5 years
digital. i know someone in the advertising business who tells me
digital is great, he just hires someone to do the digital work. i
cannot do that.

paul

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 02:28:03 2004

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Kodak is not the only maker of film on earth and even if 5302 is the
best film for the job it is not the only film that will work. Any
film can be a direct positive film with the right chemistry. Unless
there is some reason it needs to insensitive to red light there are
any number of films that with the right developers will work. If you
limit it to ortho film the field is a bit limited but there are
still a few others.

Gordon

} From: "Paul Hazelton" {paul_hazelton-at-umanitoba.ca}

:
: chris, ron, and everyone else...
:
: not wanting to sound paranoid, i think we have to consider chris's
words
: carefully.
:
: while digital systems are good, after 35 years i cannot get the
same
: results from a digital image than i can from film, no matter how
hard i
: try. double exposures with polychromatic paper using different
filters,
: dodging, burning, combined, can contribute to excellent prints.
perhaps
: others can get the same results from digitized images, after 5
years, i
: cannot.
:
: we currently maintain two older Philips 201 and one cm10
microscopes.
: they have 35mm cameras. Kodak has discontinued manufacture of
Direct
: Positive 5302, which we use for these instruments. the only
sources of
: which i now know for this film is the different suppliers. but
how long
: will their stocks last? what other 35mm format films are there
that
: have the same high resolution that is found with 5302?
:
: all in all, the promise from Kodak is fine and dandy, but will
that hold
: when Kodak decides that the digital market has made it no longer
viable
: to support wet chemistry with specialized, high resolution films
such as
: we require.
:
: of course, as far as i am concerned, i have 25 roles of 5302 in
the
: freezer, so i'm set until our microscopes die. but it is an
ongoing
: concern for the rest of you who were not ordering at the time that
Kodak
: made their decision and were not able to stock up.
:
: paul
:
: Paul R. Hazelton, PhD
: Electron Microscope Unit
: University of Manitoba
: Department of Medical Microbiology
: 531 Basic Medical Sciences Building
: 730 William Avenue
: Winnipeg, Manitoba, Canada, R3E 0W3
: e-mail: paul_hazelton-at-umanitoba.ca
: Phone:204-789-3313
: Pager:204-931-954
: Cell:204-781-1502
: Fax:204-789-3926
:
:
:
:
:
:

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 07:16:40 2004

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Unless the eye alone is used to view a scene (and almost every human eye is
different) some form of manipulation has occurred. The minute that an image
detector other than the eye is used, its response characteristics define what can
be seen or not seen. By definition, every mode of imaging other than that of
visible light has been through the selective filtration of some device. As soon as
the interpretive and adaptive mechanisms of the brain are divorced from the
immediate act of seeing a scene in context, in visible light, a greatly diminished
amount of information is available.

For conventional film photography every image has been manipulated from the moment
that the decision was made to record it. The choice of one film over another is a
choice to use a certain set of contrast and density limits over some other. This
is what professionals do - they make informed decisions about work that they are
uniquely trained to do. Anyone who is not prepared to take that responsibility for
the product of their work probably should stick to an arbitrary formula since they
apparently are no more qualified to make those judgments than those to whom any
exercise of professional judgment somehow looks suspicious.

John Twilley

Chiphead wrote:

} How is the above different from manipulating a digital image?
} is this any less of
} a manipulation (and hence potential for inaccurate or inappropriate
} artifacts) than using digital techniques to improve the appearance of an
} image?

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 08:05:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tnicklee-at-uhnresearch.ca) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 6, 2004 at 13:33:11
---------------------------------------------------------------------------

Email: tnicklee-at-uhnresearch.ca
Name: Trudey

Organization: Ontario Cancer Institute

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Has any one performed a dual immunohistochemistry staining, then removed, destained or stripped the antibodies and performed either a second series of immunofluoresecnce or immunohistochemistry? I have heard this discussed at conferences, but can not find a recent reference.
We initially are staining for HIF, CA9 and EF5 in fluorescence, which are working. We are then interested in restaining for CD34 (Nova Red in immunohistochemistry) which is a very robust antibody. CD34 should be in regions where HIF CA9 and EF5 are not, but for some reason it is not staining.
Thanks for any suggestions.

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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 08:05:11 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sarbu-at-mf.mpg.de) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 6, 2004 at 11:52:53
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Email: sarbu-at-mf.mpg.de
Name: Corneliu Sarbu

Organization: National Institute for Materials Research, Bucharest

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear colleagues,
does anybody know of a software able to assist in the geometrical drawing of the relationship between the Buergers vector, dislocation line direction, diffraction vector and perhaps electron beam direction (all expressed in a crystallographical way) in in a given material (of cubic symmetry) whose crystallographical constants are known ? The task can be fulfilled by hand drawing, in an approximate way, but I would be pleased to do it in authomatically, as I have to cope with a large variety of such configurations.
A software able to display dinamically the variation of all the above mentioned parameters would be great.

Thank you for your attention.

Dr. Corneliu Sarbu

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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 08:06:36 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Stacey.Andringa-at-uc.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, September 7, 2004 at 06:04:51
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Email: Stacey.Andringa-at-uc.edu
Name: Stacey Andringa

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I processed quite a few blocks of tissue in Spurr last week.
Some of the tissue was actually cell pellets embedded in conical
capsules. These blocks and some others in regular capsules did not
polymerize in the 2 days as I expected. I left them in the oven
over the Holiday, but they are still soft. I may have made the
Spurr wrong. Does anyone know if these will eventually cure
or can I dig out the tissue, put it into a Spurr/Propylene oxide
mixture and try to re-embed it? Of course these were the most
important blocks in all that I embedded!
Thanks.
Stacey Andringa

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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 08:07:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (walter.bobrowski-at-pfizer.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, September 7, 2004 at 07:16:18
---------------------------------------------------------------------------

Email: walter.bobrowski-at-pfizer.com
Name: Walt Bobrowski

Organization: Pfizer Global R&D

Title-Subject: [Microscopy] [Filtered] RE: DMP-30 vs. BDMA

Question: Thanks all for the wonderful advice. Yes, old habits die hard! Caroline, I've "always" used the Mollenhauer recipe as I liked it's cutting properties (it felt 'just right'). However, I'm attempting to optimize our 13-year old Lynx el automated processor and moving toward a less-viscous epoxy formulation (Luft with BDMA) for our routine embedding. Yes, I know that Spurr's is even less viscous, but didn't know they had re-formulated the components to be less toxic. I'll have to look into that.

Best regards,

Walter F. Bobrowski
Investigative Pathology
Safety Sciences
Pfizer Global Research & Development
Ann Arbor, MI 48105

TEL: 734-622-7814
FAX: 734-622-3478
Mobile: 734-646-0502

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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 08:36:41 2004

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There are sound-deadening metal channels that are attached to the wall
studs, then drywall attached to them. A drywall supply firm could supply
them. These, and a second layer of 'rock' over the old one could obviate
tearing out the wall. With the enduring popularity of 'bass you can feel',
in popular 'music', this should be an ongoing concern. :0)

Paul Grover

-----Original Message-----
} From: Gary Gaugler [mailto:gary-at-gaugler.com]
Sent: Saturday, September 04, 2004 12:01 PM
To: John Twilley
Cc: MSA listserver

Bill Robertson in his reply posting pointed out
a very good point about wall mass. My initial
thoughts were to put the acoustic tiles in the SEM room.
But the noise is more likely coming from the adjacent
room where the scroll pump and specimen interchange
pump are located. The specimen interchange pump
is not at issue. The scroll pump is an Edwards XDS 10.
Based on limited experience, it does not sound like
it is running as it should. Vacuum is fine but the
sound is odd. It makes a mechanical knocking noise.
I'm told that either these pumps work almost forever
when new or die quickly. Sounds like I have the latter.

In either case, wall mass has a high probability
of attention. The intervening wall is standard
drywall with 2x4 studs. There is no insulation
in the wall. I'm thinking of having liquid foam
insulation put in the wall cells and seeing if that
helps. In the mean time, the plinth anti-vibration
system is not exactly right and will get adjusted
shortly. then, based on how that turns out, acoustic
tiles in the pump room may be a good solution. If that
does not help much, then foam insulation.

The chiller is in the same room as the SEM but turning
it off makes no change in image noise. So the noise
is external.

Thanks for the replies. Will work on this in the
next couple of weeks.

gary g.

At 08:38 AM 9/4/2004, you wrote:
} Gary,
}
} They can be pricey. One reason is that most jurisdictions require that
} insulation
} applied to an open wall surface be flame proof. Not only that, the
} adhesive used
} to apply it must also be flame proof, per the fire department and building
} codes.
} (Recall the disasterous fire in the Rhode Island night club a couple years
} back).
} Some years ago I found that the material required behind an XRD system in
} a small
} room ran several hundred dollars for a half dozen panels. However, I
} found that I
} could get a big improvement by placing a small number of them so as to
} block the
} noise at the source, rather than covering the more distant wall
} surfaces. Buy a
} small number to try out, or experiment with packing foam. Have an
} assistant hold
} them in different locations so as to block acoustic reflections. You may
} find that
} suspending one from the ceiling in the plane of the instrument helps alot
with
} noise at the position where the operator sits.
}
} John Twilley
}
} Gary Gaugler wrote:
}
} }
}
----------------------------------------------------------------------------
--
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
}
----------------------------------------------------------------------------
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} }
} } I'm looking for sources of acoustic/anachoic
} } blocks of foam to reduce SEM room interference.
} }
} } These are like standard anechoic chamber panels.
} } I'm having trouble getting above 400KX without
} } mechanical noise from the scroll pump that is
} } located in a separate room. The acoustical
} } isolation from one room to the other is not
} } all that great, I suppose.
} }
} } Does anyone have experience with suppliers of
} } these panels? I'd like to glue them to drywall.
} }
} } Supplier responses are welcomed as off-line
} } messages.
} }
} } gary g.

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 09:23:18 2004

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If you can see the noise as discrete horizontal sinusoids, it is
probably low frequency. If you increase your scan speed and the
spacing widens proportionately, then you are looking at the true
frequency (not an 'aliasing' effect). Also, when aliasing is
occurring, the disturbance will often appear to be propagating at an
angle, rather than purely horizontal.

A simple way to estimate low frequencies is to employ something that
generates a strong 60Hz magnetic field as a reference (I have often used
a hand-held magnetic tape eraser). Set up with a relatively high scan
speed so that your noise appears as nice sinusoidal disturbances. Count
how many cusps you get in a convenient vertical distance. Then turn on
the magnetic field generator and do the same for its disturbance.
Calculate the ratio vs 60 Hz and you have a crude frequency estimate.

However, if you are seeing discrete sinusoidal disturbances and
especially since this is coming from a piece of equipment in a
neighboring room that is described as making a "knocking" sound,
relatively low frequencies sound like a good bet.

Fred Schamber
ASPEX, LLC

Gary Gaugler wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} I don't have any direct way of knowing whether the
} noise is high or low frequency. It only shows up
} above 60KX as sinusoids on the edges of specimen
} details.
}
} I can probably use FFT to compute the frequency.
} It is consistent.
}
} gary g.
}
}
} At 03:34 PM 9/5/2004, you wrote:
}
}
}
} } On Sep 3, 2004, at 6:30 PM, Gary Gaugler wrote:
} }
} } } I'm looking for sources of acoustic/anachoic
} } } blocks of foam to reduce SEM room interference.
} } }
} } } These are like standard anechoic chamber panels.
} } } I'm having trouble getting above 400KX without
} } } mechanical noise from the scroll pump that is
} } } located in a separate room. The acoustical
} } } isolation from one room to the other is not
} } } all that great, I suppose.
} } }
} } } Does anyone have experience with suppliers of
} } } these panels? I'd like to glue them to drywall.
} } }
} } } Supplier responses are welcomed as off-line
} } } messages.
} }
} } Dear Gary,
} } Fred has it right about the difference between low and high
} } frequencies. The depth of the invaginations in anechoic panels has
} } to be 1/4 of the wavelength of the sound in order to be effective, so
} } for low frequencies, the panels could take up the entire room,
} } leaving no space for the equipment.
} } Yours,
} } Bill Tivol, PhD
} } EM Scientist and Manager
} } Cryo-Electron Microscopy Facility
} } Broad Center, Mail Code 114-96
} } California Institute of Technology
} } Pasadena CA 91125
} } (626) 395-8833
} } tivol-at-caltech.edu
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 09:38:34 2004

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Any professional photo lab could do this for you. Since you are in
New York City finding a pro lab should be easy. However, high quality
film scanners (from Nikon, Minolta, etc). that do 35 mm slides are
relatively cheap these days, you might look into buying one and scanning
the slides yourself.

Geoff

Sandra Masur wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 10:44:17 2004

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On Sep 6, 2004, at 6:35 AM, Sandra Masur wrote:

} Can anyone recommend a good commercial photolab that is
} also reasonably priced, for scanning hundreds of 35 mm
} slides and saving on CDs?
}
Dear Sandra,
I have used Dale Labs in Florida for many years for my personal
photography, and one of the services they offer is to scan 35 mm slides
onto CDs. Their phone number is (800) 327-1776. I have no affiliation
with them except as a long-time satisfied customer.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 10:50:14 2004

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Hi,

Suggest that you contact the Royal Microscopical Society in Oxford, UK. They have a wide range of courses.

Here in the US, John Russ' course at North Carolina State is one of the best respected courses.

Hope this was helpful,
Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
F: 972-954-8018

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Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.

At 01:53 AM 9/2/2004, Gareth Morgan wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 11:05:12 2004

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Dear Gary,
I have had some success here isolating the noise from the pump by putting
the pump up on a sound-deadening material such as two-inch-thick packing
foam, with a piece of plywood on top. I now have all my rotary pumps up on
pads. There can be considerable noise transmission through the floor to your
SEM column.
Regards and good luck,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Gary Gaugler" {gary-at-gaugler.com}
To: "John Twilley" {jtwilley-at-sprynet.com}
Cc: "MSA listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Saturday, September 04, 2004 10:00 AM

MACO have contacted me to draw my attention to their company, which
produces EM film, X-ray film and other specialist B&W films, printing
paper and chemicals. The company partners Oriental in Japan and Lucky
in China, both large producers of silver photographic emulsions and
coated papers for digital printers.

I had not been aware of the existence of this company until I started
this thread on continued availability of EM film, and I suspect that
is true of many other EM users on this list.

MACO's web site is at http://www.mahn.net

Prompted by Nestor, I have suggested to MACO that they should list
themselves as a company on the MSA Commercial Organisations site
http://www.amc.anl.gov/docs/nonanl/wwwform.html

This is not an attempt to promote MACO in particular, and I have no
financial interest whatever in this particular company, although I
will be trying out their EM film if I can obtain a sample of it here.
I merely wish to draw attention to the fact that, as Chuck has pointed
out, this is a new company already poised to take over film production
if the big companies pull out. It would be a service to us all if
other emerging companies producing EM films and related photographic
materials and equipment could also be encouraged to register with the
Commercial Organisations site.

Best wishes
Chris

Dr. Chris Jeffree
University of Edinburgh

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 12:36:21 2004

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I have inherited some aged vials of crystalline osmium. They are a tad
older than normal which is to say 1940! But they look quite normal and are
sealed in glass ampules just like a more modern vintage. I have offered 30
x 1 gm vials so it was hard to not accept the gift; this would be a
lifetime supply. I intend to try them out in an experiment tomorrow. If
anyone knows why this is doomed to failure, please let me know
asap. Otherwise I will let the list know how it works out. Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 13:39:18 2004

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I need to do some embedding in Lowicryl HM20 and will be ordering new resin kit. I noticed EMS is now offering "MonoStep" - a pre-mixed variation of the normal kit that supposedly gets rid of all the manipulations. Does anybody have some experience with this resin? I am a bit cautious about possible partial polymerization of the pre-made mixture.

Thanks,

Michael

--
Michael Jarnik, Ph.D.
Electron Microscope Facility
Fox Chase Cancer Center
7701 Burholme Ave.
Philadelphia, PA 19111
Tel. 215-728-5675
Fax 215-728-2412

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 15:54:56 2004

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I think you have a winner!
Chris

} I have inherited some aged vials of crystalline osmium. They are a
tad
} older than normal which is to say 1940! But they look quite normal
and are
} sealed in glass ampules just like a more modern vintage. I have
offered 30
} x 1 gm vials so it was hard to not accept the gift; this would be a
} lifetime supply. I intend to try them out in an experiment
tomorrow. If
} anyone knows why this is doomed to failure, please let me know
} asap. Otherwise I will let the list know how it works out. Tom
}
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 16:38:43 2004

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I know nothing about "dual" immunostaining" but would think that any
"destaining", stripping etc will equally affect antibodies and antigens, so
I don't expect anything good from it. From another hand, formally speaking
you do not limited to only "double" staining in immunofluorescence. With
luck, you may use for instance mouse, rat, rabbit, chicken primary
antibodies and correspondent secondary with different
fluorochromes. Modern confocal microscopes permits to analyze the whole
spectrum of emission, so you could separate signals quite easily. I don't
know is my approach realistic or not. It would be nice to hear expert's
opinion. From biochemical point of view, you could "strip" antibodies by
low pH (=2) or a few moles of urea, but it would affect your antigen as
well (for bad or good). Sergey

At 08:30 AM 9/7/2004 -0500, you wrote:

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I haven't found any difference. Tom

At 03:04 PM 09/07/04 -0400, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 7 17:42:14 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jcai-at-nanostellar.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, September 7, 2004 at 12:57:14
---------------------------------------------------------------------------

Email: jcai-at-nanostellar.com
Name: Juan

Organization: Nanostellar

Title-Subject: [Microscopy] [Filtered] selective etching method for alumina

Question: Hi all,

I am looking for a way to chemically etch gama-alumina powders, without etching Ag and Cu nano-pariticles mixed in them.

The weight percentage of Ag or Cu in Alumina is around 0.5-1%. We have tried HF, but it turned out Ag and Cu are also etched out.

Thanks in advance for your advice,

Juan

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 02:45:39 2004

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Hello,
Please, could anybody of Philips CM100 users send me a list of coil currents
(C1, C2, OBJ etc.)in LM and M Mode at 80kV for magnifications of 1.4kx, 10.5kx
and 34kx, respectively. We have some troubles with our EM and unfortunately we
do not have a record of these values.
Thanking you in advance.
Best regards from Prague
Oldrich

+-----------------------------------+
Oldrich Benada
Acad. Sci. CR
Institute of Microbiology
Laboratory of electron microscopy
Videnska 1083
CZ - 142 20 Prague 4 - Krc
Czech Republic
+------------------------------------+

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 03:17:40 2004

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Stacey

it's unlikely that the samples will polymerise much more after a couple of days. You don't say whether you use Spurr's regularly and this is a first batch to go wrong.

You can certainly try re-embedding but be prepared for a slightly poorer block but be aware of the points below in case it happens again.

Spurr's can poorly embed for a variety of reasons:
1. incomplete dehydration, incomplete removal of alcohol - although if you're using propylene oxide as well I wouldn't have thought so.
2. incomplete impregnation with resin because too little time, not enough stages (eg 50%, 75%, 2x100%), not enough agitation/rotation.
3. bad mix either due to wrong amounts or incomplete mix.
4. One of the components has deteriorated (S1 curing agent may have a shelf life of 6-12 months; I believe that the NSA anhydride hardener can go off especially if exposed to moisture over time)

Spurr's can be affected by moisture so if you chill or freeze it, allow plenty of time for it to reach room temperature and don't leave the lids of the components or mixture for too long.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Stacey.Andringa-at-uc.edu (by way of MicroscopyListserver)

Announcement and Call for Papers
Michigan Microscopy &Microanalysis Society Fall Meeting, 2004

Kellogg Center
East Lansing, MI
November 5, 2004

Abstract Deadline: October 1, 2004

The Fall Meeting of the Michigan Microscopy and Microanalysis Society will
be held on November 5th, 2004 at the Kellogg Center in East Lansing, MI. In
this one-day conference, there will be two sessions. One is a platform
session. This session will have approximately 8-10 speakers representing
industry, academia, and research laboratories. The other is a poster
session. Please encourage your colleagues who prefer to avoid a platform
presentation to submit abstracts for the poster presentations. Some
selected abstracts for the oral presentation can be transferred to the
poster session if too many abstracts come for the platform session. In
addition to the speakers, vendors will exhibit a wide range of products and
services of interest to the microscopy community. Presentations are being
solicited from researchers in the Physical and Biological Sciences,
including one vendor presentation and an invited speaker. Student
participation is particularly encouraged. Also, vendors are encouraged to
contact the below address to reserve space for product display.

Abstract Submission
Please submit a 300 to 350 word abstract by October 1st indicating which
session you prefer (poster or presentation)

Geoff Williams
MMM President
217 Brooks Hall
Biology Department
Central Michigan University
Mt. Pleasant, MI 48859
Ph 989 774 3576
Fax 989 774 3462
Email: ge.willi-at-cmich.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 14:13:31 2004

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I need a non standard band pass filter and grating for a B &L
monochromatic grating. for 500 nm to 1,000 nm. I know these are not
standard. The band pass filter can be wider and a water cell would
be actable. I would also like to find a hot or cold mirror that had
a 1,100 to 1,400 cut off. All the filters need to have pretty high
transmittance in the pass band.

Thanks
Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org
-----

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 16:13:41 2004

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That's interesting - what was it used for in 1940?

Lesley Weston.

on 07/09/2004 11:03 AM, Tom Phillips at phillipst-at-missouri.edu wrote:

}
}
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} I have inherited some aged vials of crystalline osmium. They are a tad
} older than normal which is to say 1940! But they look quite normal and are
} sealed in glass ampules just like a more modern vintage. I have offered 30
} x 1 gm vials so it was hard to not accept the gift; this would be a
} lifetime supply. I intend to try them out in an experiment tomorrow. If
} anyone knows why this is doomed to failure, please let me know
} asap. Otherwise I will let the list know how it works out. Tom
}
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 17:16:25 2004

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Oh, what a good question! I do think osmium was used pre-EM days for some
speciality stains (neuro?) but I was given at least 30 ampules so that
seems like a lot for someone doing a speciality stain. I don't know which
department this chemical stock came from. This came to me via the
Environmental Health and Safety people on campus who try to recycle
"unwanted" but unused chemicals (a great program you should all get your
schools to copy since it says lots of disposal costs and reduces the
researcher expenses). It may have been used in some chemical lab but once
again seems like a lot. These vials were packaged by Merck (stamped made
in Germany), sold by Arthur Thomas and each encased in a nice little wood
case. They have 8/13/40 or 1940 written on them. I will let the list know
how the expt comes out. Tom

At 02:39 PM 09/08/04 -0700, you wrote:
} That's interesting - what was it used for in 1940?
}
} Lesley Weston.
}
}
} on 07/09/2004 11:03 AM, Tom Phillips at phillipst-at-missouri.edu wrote:
}
} }
} }
} }
} ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ----------------------------------------------------------------------------
} --} -
} }
} } I have inherited some aged vials of crystalline osmium. They are a tad
} } older than normal which is to say 1940! But they look quite normal and are
} } sealed in glass ampules just like a more modern vintage. I have offered 30
} } x 1 gm vials so it was hard to not accept the gift; this would be a
} } lifetime supply. I intend to try them out in an experiment tomorrow. If
} } anyone knows why this is doomed to failure, please let me know
} } asap. Otherwise I will let the list know how it works out. Tom
} }
} }
} }
} } Thomas E. Phillips, PhD
} } Professor of Biological Sciences
} } Director, Molecular Cytology Core
} } 3 Tucker Hall
} } University of Missouri
} } Columbia, MO 65211-7400
} }
} } 573-882-4712 (office)
} } 573-882-0123 (fax)
} } PhillipsT-at-missouri.edu
} }
} }
} }

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 18:13:38 2004

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Hi,

OsO4 is used as a histological stain for light microscopy, this use may
have preceded its use in Electron Microscopy.

Aaron Hicks
Electron Microscopy Preparation Technician

Comparative Physiology and Anatomy
Institute of Veterinary, Animal, and Biomedical Sciences
Massey University

PN-412
Private Bag 11 222
Palmerston North
New Zealand

Phone +64 06 350 4470

-----Original Message-----
} From: Lesley Weston [mailto:lesley-at-vancouverbc.net]
Sent: Thursday, 9 September 2004 9:39 a.m.
To: Tom Phillips; Microscopy-at-msa.microscopy.com

That's interesting - what was it used for in 1940?

Lesley Weston.

on 07/09/2004 11:03 AM, Tom Phillips at phillipst-at-missouri.edu wrote:

}
}
} ----------------------------------------------------------------------
} --------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
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----
--} -
}
} I have inherited some aged vials of crystalline osmium. They are a
} tad older than normal which is to say 1940! But they look quite
} normal and are sealed in glass ampules just like a more modern
} vintage. I have offered 30 x 1 gm vials so it was hard to not accept
} the gift; this would be a lifetime supply. I intend to try them out
} in an experiment tomorrow. If anyone knows why this is doomed to
} failure, please let me know asap. Otherwise I will let the list know
} how it works out. Tom
}
}
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 8 18:50:27 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (wwiggins-at-carolinas.org) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 8, 2004 at 12:41:52
---------------------------------------------------------------------------

Email: wwiggins-at-carolinas.org
Name: Winston Wiggins

Organization: Carolinas HealthCare System

Title-Subject: [Microscopy] [Filtered] Ilford

Question: Does anyone have any details about Ilford going under? There was a blurb in the Guardian about it last month but I've heard nothing here in the States. Worried because I just got an Ilford 2150XL processor 2 years ago and hoped I could stave off digital equipment for a longer while.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 02:32:47 2004

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Winston
I posted a comment about this to the list a few days ago. See below
Some further links:
http://www.guardian.co.uk/arts/news/story/0,11711,1289459,00.html
http://www.manchesteronline.co.uk/business/general/s/128/128120_fears_for_700_jobs_as_ilford_faces_closure.html
By contrast, Ilford's web site suggests situation normal!
Hope this helps
Chris

Dr. Chris Jeffree
Inveresk Cottage
26, Carberry Road
Inveresk
Musselburgh
Midlothian
EH21 8PR
Tel: +44 131 665 6062
FAX +44 131 653 6248
Mobile 07710 585 401
----- Original Message -----
} From: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
To: {microscopy-at-msa.microscopy.com}
Sent: Friday, September 03, 2004 9:05 AM

Dear listserver readers,
I am in the lucky position of getting a second hand Micrion 2500
focused ion beam microscope. All the bits are in the room, installation
(via FEI) should start soon. However I have no manual, and no information
on how it was configured in its previous life. Are there any users of this
machine out there who can give me some advice on the 'standard'
configuration (particularly things like the gas supplies) - and what it is
like to use/maintain? It looks quite frightening to an old TEM/SEM user
like me, UHV stainless steel and a million wires and tubes, more like some
experimental surface science kit than a routine spec prep tool..

Many thanks indeed

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

=======================================================================
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not make any use of this information, or copy or show it to any
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received this e-mail, and return the original to us. Any use,
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No part of this message can be considered a request for goods or
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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 07:42:15 2004

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OsO4 is a classic stain for the basal bodies of ciliates. It's
important in ciliate systematics and morphology, as it reveals the
ciliary patterns at the light microscope level.
But.
It was usually applied to a dish of critters while watching through a
microscope.
Think Van Gogh's "Starry Night" ...

Phil

} That's interesting - what was it used for in 1940?
}
} Lesley Weston.
}
}
} on 07/09/2004 11:03 AM, Tom Phillips at phillipst-at-missouri.edu wrote:
}
} }
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} ----------------------------------------------------------------------------
} --} -
} }
} } I have inherited some aged vials of crystalline osmium. They are a tad
} } older than normal which is to say 1940! But they look quite normal and are
} } sealed in glass ampules just like a more modern vintage. I have offered 30
} } x 1 gm vials so it was hard to not accept the gift; this would be a
} } lifetime supply. I intend to try them out in an experiment tomorrow. If
} } anyone knows why this is doomed to failure, please let me know
} } asap. Otherwise I will let the list know how it works out. Tom
} }
} }
} }
} } Thomas E. Phillips, PhD
} } Professor of Biological Sciences
} } Director, Molecular Cytology Core
} } 3 Tucker Hall
} } University of Missouri
} } Columbia, MO 65211-7400
} }
} } 573-882-4712 (office)
} } 573-882-0123 (fax)
} } PhillipsT-at-missouri.edu
} }
} }
} }

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 08:00:08 2004

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Perhaps for Mann's osmium-sublimate fixative, Flemming's fixative or for
lipid staining.

Lesley Weston wrote:

} ------------------------------------------------------------------------------
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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 09:55:13 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Richard,

Congratulations on your new 2500! It is a great tool,
but you are right, it is not really designed to be
easy service-able.

The "standard" configuration of gas supply boxes would
depend on what are you planning to do with the tool.
If you could please describe your intended
applications in some detail (materials you plan to
deal with and a type of work you intend to do), I
would be more then glad to help you with selection of
he gas configuration. There are also a lot of routine
service and periodic maintenance that you can do on
your own with some skill and perhaps a bit of
training.

If it is a standard, single-column 2500, then there is
no UHV involved, so you would not have to deal with
bake-outs.

Please contact me with your application details and if
(or rather when) you will have more questions
regarding the tool.

Best Regards,
Valery Ray
Particle Beam Systems
& Technology
www.partbeamsystech.com

--- Richard Beanland {richard.beanland-at-bookham.com}
wrote:

}
}
}
------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------
}
} Dear listserver readers,
} I am in the lucky position of getting a second hand
} Micrion 2500
} focused ion beam microscope. All the bits are in
} the room, installation
} (via FEI) should start soon. However I have no
} manual, and no information
} on how it was configured in its previous life. Are
} there any users of this
} machine out there who can give me some advice on the
} 'standard'
} configuration (particularly things like the gas
} supplies) - and what it is
} like to use/maintain? It looks quite frightening to
} an old TEM/SEM user
} like me, UHV stainless steel and a million wires and
} tubes, more like some
} experimental surface science kit than a routine spec
} prep tool..
}
} Many thanks indeed
}
} Richard
}
} _______________________________
} Richard Beanland
} Analytical Services
} Bookham Technology plc
} Caswell,
} Towcester,
} Northamptonshire NN12 8EQ
} UK
} Tel: +44 (0) 1327 356362
} Fax: +44 (0) 1327 356775
} http://www.bookham.com
}
}
}
=======================================================================
} This e-mail is intended for the person it is
} addressed to only. The
} information contained in it may be confidential
} and/or protected by
} law. If you are not the intended recipient of this
} message, you must
} not make any use of this information, or copy or
} show it to any
} person. Please contact us immediately to tell us
} that you have
} received this e-mail, and return the original to us.
} Any use,
} forwarding, printing or copying of this message is
} strictly prohibited.
} No part of this message can be considered a request
} for goods or
} services.
}
=======================================================================
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 11:10:22 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Listers:
We have an SIS Megaview II mounted on the 35mm port of our Hitachi
H-7000. This interferes with the proper operation of the left specimen
traverse control. If there is anyone out there who has managed to
customize the system so that it operates properly, I would appreciate
hearing from them.
Thanks much
Greg

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 16:30:00 2004

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Hello Greg,

We have at least one other installation on an H-7000, where a pulley system
was used to "redirect" the control rod. I will send you a document directly
that shows the modifications. If you'd like I can get more information for
you (parts, prices, etc.)

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Greg Erdos [mailto:gwe-at-biotech.ufl.edu]
Sent: Thursday, September 09, 2004 10:35
To: Microscopy-at-sparc5.microscopy.com

Dear Listers:
We have an SIS Megaview II mounted on the 35mm port of our Hitachi
H-7000. This interferes with the proper operation of the left specimen
traverse control. If there is anyone out there who has managed to
customize the system so that it operates properly, I would appreciate
hearing from them.
Thanks much
Greg

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 9 21:54:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Greg,

The easy way (perhaps the easiest way) is to use flexible shaft. We use flexible shafts from Small Parts Inc. (Miami Lakes, FL),
www.smallparts.com or 800-220-4242 . Choose panel type, with 1/4" diameter bore at one end and 1/4" diameter shaft at the other end.
Then you can simply remove existing left specimen translation knob, attach bore end of the flexible shaft to the left control of the
specimen translation control axis, and attach removed knob to the rod end of the flexible shaft. You need also a small (rectangular)
piece of aluminum or whatever suitable material to hold the outer end of the shaft at the new location. External end of the flexible
shaft attaches to a panel (aluminum piece) in the same way as regular potentiometer or a toggle switch. Flexible shafts 6" and 12"
long are standard. Several can be joined for greater length. Part numbers Y-FDCP-4/6 and Y-FDCP-4/12 respectively, cost $19 and $23.

Please see one such camera installation on Hitachi HF-2000 TEM on our web site at http://www.sia-cam.com/2/photo2.html ;
http://www.sia-cam.com/2/photo3.html ; http://www.sia-cam.com/2/photo4.html . Both knobs were moved there. It took us 1 hour to
complete this modification from scratch.

Do not use flex. shaft much longer than needed, in order to avoid excessive free-play.

Rigid U-joint shafts can be used too, but modification becomes much more complex, since bearing support will be required on each
side of a U-joint.

You are welcome to contact me for further details.

Vitaly Feingold
Scientific Instruments and Applications
2773 Heath Lane, Duluth GA 30096
(770)232-7785 ph.
(770)232-1791 fax
(678)467-0012 mobile
www.sia-cam.com

This message is made of 100% recycled electrons.

This address can not receive messages larger than 15 kb without prior
notification.

----- Original Message -----
} From: "Greg Erdos" {gwe-at-biotech.ufl.edu}
To: "Microscopy-at-sparc5.microscopy.com" {Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, September 09, 2004 12:35 PM

Anyone know of a company that specializes in blue filters for microscopy.
We are looking for various sizes and need quite a few for student scopes,
some that are not standard sizes. Obviously the dealers have some sizes,
but I am really looking for a company that carries a large range of sizes
and types.

Thanks for the help!
David Burton
Optical Specialist
University of Washington

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 05:10:01 2004

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Dear all,
Would anyone be kind enough to comment on the relative merits of
lens-coupled and fibre-optic-coupled CCD cameras for use at the wide
angle (35 mm) port? I am currently investigating the best choice for
the recording of diffraction patterns on a FEI Tecnai.

Thanks

--
Ian MacLaren
Department of Physics and Astronomy
University of Glasgow
Glasgow G12 8QQ
Scotland
http://www.ssp.gla.ac.uk/

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 09:05:26 2004

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Dear All:

We have a Hitachi H-7500 TEM, and want to have objective aperture
strips with four 20 micron apertures made for our scope. Can anyone
recommend a company? Thank you.

Hong
Emory EM

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 12:23:58 2004

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Dear Hong:

Yes, Ladd Research can provide a customized aperture for your scope. I
believe we are the only supplier of customized apertures in the U.S., but we
can make them available through other EM suppliers if you choose.

Deb Sicard

*Disclaimer: Ladd Research is a dealer of microscopy supplies and
accessories

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: ladres-at-att.net

----- Original Message -----
} From: "Hong Yi" {hyi-at-emory.edu}
To: {microscopy-at-ns.microscopy.com}
Sent: Friday, September 10, 2004 10:30 AM

Dear All:

We have a Hitachi H-7500 TEM, and want to have objective aperture
strips with four 20 micron apertures made for our scope. Can anyone
recommend a company? Thank you.

Hong
Emory EM

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 13:52:14 2004

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In a message dated 9/9/2004 10:07:31 PM US Mountain Standard Time,
dburton-at-nwlink.com writes:
Anyone know of a company that specializes in blue filters for microscopy.
We are looking for various sizes and need quite a few for student scopes,
some that are not standard sizes. Obviously the dealers have some sizes,
but I am really looking for a company that carries a large range of sizes
and types.
David,

The "default" size for such filters seems to be 24 mm or 1 inch, which is
probably what you'll find from most of the suppliers unless you want to get
plastic filter material in sheet form and make your own.

Try the following:

Edmund Optical at [www.edmundoptical.com]. Click on their Online Catalog,
then =} Optics =} Filters and Diffusers =} Color. You'll get several options,
such as plastic, glass, wratten filters, etc.

Chroma Technology at [www.chroma.com], Toll Free: 1-800-824-7662. They're a
specialty filter manufacturer, but I've used them before for simple blue scope
filters. They can cut and mount the filters in any size you want. Paul
Millman is the person to talk to.

Good luck, hope this helps.

Cheers,

Bob Chiovetti
RMC Products / Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 14:58:15 2004

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Hi Fellow Microscopists,

I am immunolabeling cryothin sections of tissue that has been lightly fixed in 2 or 4%
paraformaldehyde with 0.1% glut, then cryoprotected, frozen and thin sectioned.
Does anyone have antigen unmasking techniques that you are very pleased with for cryothins? If
so I would be so happy to hear about them.
I have tried 0.005% trypsin, hot citrate buffer, hot tris 9.0 and 0.3% SDS and have had no effect
on the antigens that I am trying to unmask. Morphology, however, has suffered!
Thank you for any info advance.

Robert Underwood
Research Scientist
University of Washington

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 18:20:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (konishi-at-geofourpeaks.com) from http://microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Friday, September 10, 2004 at 14:57:52
---------------------------------------------------------------------------

Email: konishi-at-geofourpeaks.com
Name: Hiromi Konishi

Organization: Indiana University

Education: Graduate College

Location: Bloomington, Indiana

Question: } I am asking about how to estimate the number of atoms at the surface of nano particles.
}
} You can roughly estimate the number using volumes of sphere and unit cell. If you assume that ěsurfaceî is the region between two spheres that have a slightly different diameter, you can calculate the volume of ěsurfaceî and estimate the number of atoms in the ěsurfaceî. However, it is a very rough estimation, and it is not clear how to chose the depth to define the surface.
}
} I would like to know general method in calculation of the number of atoms on surface. Also, if there is a program for such calculation, please advise.
}
} Thank you,
} Hiromi Konishi
} Indiana University

PS. I am a member of the list, but currently I cannot post my message for unknow reason, so I used this form.

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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 10 20:11:56 2004

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Dear Colleagues:

I would like to transfer the license of MacTempas (HRTEM Image
Simulation Software package for Apple) with USB hardware key (fair
price!).
Interested please contact : benyam-at-recite.ca

Regards,
Benyam

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 11 16:10:56 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tauria-at-hotmail.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Saturday, September 11, 2004 at 12:06:51
---------------------------------------------------------------------------

Email: tauria-at-hotmail.com
Name: FRANCIS J. PRONESTI

Organization: WORLD ENERGY SERVICES

Education: Graduate College

Location: CASTELLANA GROTTE (BARI), ITALY

Question: I HAVE AN OLD UNITRON SERIES "N" METALURGICAL MICROSCOPE, PURCHASED RECENTLY ON EBAY. I DO OWE MANY OTHER MICROSCOPES, BUT I HAVE FALLEN IN LOVE WITH THIS BEAUTIFUL, OPTICALLY COMPLEX INSTRUMENT. THERE IS NOTHING INTUITIVE ABOUT ITS SET-UP AND USE, SO I WONDER IF ANYONE WOULD KNOW WHERE I CAN BUY A COPY OF THE OPERATING MANUAL FOR THIS SCOPE.
FRANCIS J. PRONESTI
MSME, MSEE, MEMBER IEEE.
PRESIDENT AND OWNER, WORLD ENERGY SERVICES LTD.

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From MicroscopyL-request-at-ns.microscopy.com Sat Sep 11 16:16:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (dmk8533-at-louisiana.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, September 10, 2004 at 14:05:22
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Email: dmk8533-at-louisiana.edu
Name: David Krayesky

Organization: University of Louisiana

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I have a Olympus Vanox fluoresence microscope in my lab. I need a manual for the microscope to explain what all the different markings mean on the various filters, so I can figure out what the filters do. Does anyone know where I can get this information? I haven't had a lot of luck at Olympus's web site or the FSU microscopy Primer web site.

Thanks,

Dave

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From MicroscopyL-request-at-ns.microscopy.com Sat Sep 11 16:17:53 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (burnin1970-at-hotmail.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, September 10, 2004 at 23:17:54
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Email: burnin1970-at-hotmail.com
Name: Andrei Burnin

Organization: Dartmouth College

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Recently, we tried EDS analysis of non-carbon nanotubes (20-30 nm in diameter) in TEM microscope (Tecnai F20).
The signals from compositional elements are very tiny in comparison with the cupper and carbon signals, which makes perfect sense, because we used carbon coated grids.
However, in the literature such EDS spectra from a spot in one (not from a bunch), say, a ZnO nanotube exhibits signals comparable to those from Cu-C background. How it is possible, that people obtain so high intensity of compositional elements from a very small analyzed area?
What should also we do to improve our results of getting EDS from a single nanotube?
Is it necessary to use beryllium grids?
Thank you.

Andrei

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From MicroscopyL-request-at-ns.microscopy.com Sat Sep 11 16:19:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, September 11, 2004 at 04:49:50
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Email: kssim-at-mmu.edu.my
Name: kssim

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear all,

I need help from anyone who know the following question:-

Basically I are going to prove that SE3 (secondary electron generated by BSEs at the pole-piece and the chamber wall from returning to the specimen) does not contribute to SE yield. The pole-piece of the SEM is covered by a 2 by 2 inch aluminum (Al) plate that has been painted with carbon paint to absorb SE3s. I need to know the bethe range of K-O range of the target which is carbon on the Al. I could not find this data from 10kev to 30kev range. I believe that with the thickness of 10um is good enough, but not a good reference. Can anyone help me on this?

But expertise says that the SE yield of both AL and carbon are not so high - refer to DC Joy journal paper. So the true SE3 contribution can be much higher. This is one of the points that I need to prove that SE3 still can be ignored.

Thanks
Ks

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From MicroscopyL-request-at-ns.microscopy.com Sun Sep 12 09:55:36 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, September 12, 2004 at 09:44:09
---------------------------------------------------------------------------

Email: kssim-at-mmu.edu.my
Name: kssim

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear All,

Does any know how to connect x,y and video from Jeol SEM to DT3152 frame grabber card ? Appreciate your help

Thank You
Ks

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From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 03:59:06 2004

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There is a general statement at http://www.amtimaging.com/english_site/faq_e/faq_e.html#3, not specific to the 35 mm port. However, I too would like to learn more on this.

----
Divakar
------
Physical Metallurgy Section,
Indira Gandhi Centre for Atomic Research.
Kalpakkam, TN 603102, India

-----Original Message-----
} From: Ian MacLaren [SMTP:i.maclaren-at-physics.gla.ac.uk]
Sent: Monday, September 13, 2004 9:17 AM
To: Microscopy-at-MSA.Microscopy.Com

Dear all,
Would anyone be kind enough to comment on the relative merits of
lens-coupled and fibre-optic-coupled CCD cameras for use at the wide
angle (35 mm) port? I am currently investigating the best choice for
the recording of diffraction patterns on a FEI Tecnai.

Thanks

--
Ian MacLaren
Department of Physics and Astronomy
University of Glasgow
Glasgow G12 8QQ
Scotland
http://www.ssp.gla.ac.uk/

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 08:06:37 2004

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The job below is for a TEM specialist although you have to read well
through the job particulars
http://www.materials.ox.ac.uk/vacancies/Job-Begbroke.pdf to find that out.

----------------------------------
UNIVERSITY OF OXFORD
Begbroke Science Park
Business-Development Materials Analyst
Academic-Related (Research) Grade RSIa - Salary Range - Ł19,460 - Ł28,128

Applications are invited for the post of Business Development Materials
Analyst for a period of up to two years. The Business Development
Materials Analyst will be working for the Institute of Aerospace and
Automotive Studies, in collaboration with Faraday Advance and the Oxford
Materials Characterisation Service. He or she will be responsible for
customer-oriented provision of industrial and analytical materials
characterisation services, including provision of rapid high-quality
investigations and proposals for materials related problems, and will
work to broaden and strengthen the academic and commercial relationships
of the OMCS.

The successful candidate is likely to have a track record in materials
characterisation, particularly in operating electron microscopes and
interpreting the resultant data, an appreciation of business issues
including Intellectual Property Rights, budgeting, management and
marketing, and the ability to communicate effectively to a range of
audiences. An understanding of the Aerospace and Automotive sectors
would also be beneficial.

Further particulars of the post are available from Mr Michael Sloane,
Begbroke Directorate, Oxford University Begbroke Science Park, Sandy
Lane, Yarnton, Oxfordshrire, OX5 1PF. email:
michael.sloane-at-begbroke.ox.ac.uk.

Applications, including a covering letter indicating how the applicant
meets the requirements of the post together with a detailed curriculum
vitae, should reach Mr. Sloane at the above address, by no later than
September 30th, 2004. Please include full contact details for three
referees, of whom one must be an existing or recent employer. The post
can be discussed informally with Dr Alison Crossley,
alison.crossley-at-materials.ox.ac.uk, 01865 283726.

The University is an equal opportunities employer.

See also http://www.ox.ac.uk/jobs
--
Chris Salter,
Oxford Materials Characterisation Service,
&
Material Science-based Archaeology Group,
&
Electron Microscopy Research Support Group,
Oxford University Begbroke Science Park,
Sandy Lane, Yarnton, Oxford, OX5 1PF
Tel 01865 283722, EPMA 283741, Mobile 07776031608

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 09:14:18 2004

Contents Retrieved from Microscopy Listserver Archives
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I am looking for Windows software that allows me to see crystal structure with
a less expensive cost. I want to use the software for quick check of number of
atoms in a unit cell and distance between atoms, looking at crystal structure,
and making figures for publication. Is there any recommendation?

Thank you,

Hiromi Konishi
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 10:14:59 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello Listers,

I'm interested in hearing opinions (pro/con) from anyone that has
experience with the Aspex PSEM. Please call/e-mail me off
list if you wish. Thanks for your input and time.

Ed Dargelis
Engineering Systems, Inc.
3851 Exchange Ave.
Aurora, Il 60504
(630) 851-4566
evdargelis-at-esi-il.com

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 10:28:30 2004

Contents Retrieved from Microscopy Listserver Archives
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ATOMS is a very good software which I used to do all kinds of work you want to do. But it is a commercial software, I do not know its exact price.

You can go to IUCr's (International Union of Crystallography)Webster and check their software page, you will find a lot of free software.

Best regards,

Ying

-----Original Message-----
} From: hkonishi-at-indiana.edu [mailto:hkonishi-at-indiana.edu]
Sent: Monday, September 13, 2004 9:42 AM
To: Microscopy-at-MSA.Microscopy.Com

I am looking for Windows software that allows me to see crystal structure with
a less expensive cost. I want to use the software for quick check of number of
atoms in a unit cell and distance between atoms, looking at crystal structure,
and making figures for publication. Is there any recommendation?

Thank you,

Hiromi Konishi
Indiana University

****************************************************************************************

Note: The information contained in this message may be privileged and confidential and thus protected from disclosure. If the reader of this message is not the intended recipient, or an employee or agent responsible for delivering this message to the intended recipient, you are hereby notified that any dissemination, distribution or copying of this communication is strictly prohibited. If you have received this communication in error, please notify us immediately by replying to the message and deleting it from your computer. Thank you.

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From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 10:34:54 2004

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Marcus, are you out there?
If anyone knows how to contact Marcus, please respond off line.
Thanks,
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 11:24:25 2004

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Dear Pei & Jorgen,

A tool developed in '99, visit www.Evactron.com actively prevents sample
'image darkening effects' from polymerized hydrocarbon contamination. The
device is commercially available, improves DP & TMP system vacuum levels
safely without damage to SEM/FIB components and eliminates manual iso
swabbing cleanup.

XEI Scientific

-----Original Message-----
} From: j.bilde-at-risoe.dk [mailto:j.bilde-at-risoe.dk]
Sent: Thursday, September 02, 2004 12:16 AM
To: pzou-at-feico.com
Cc: microscopy-at-microscopy.com

Dear Pei Zou,

See section 9.10.6 in Goldstein et al.: Scanning electron microscopy and
X-ray analysis" Plenum Press 1992. It begins: "A sample subjected to
electron bombardment in a diffusion-pumped vacuum gradually becomes ccovered
with a contamination layer due to polymerization, under the action of the
beam, of organic matter adsorbed on the surface".

Ways to reduce the effect are: clean vacuum, clean sample, cold finger.

Best regards,
Jorgen.

{:::} --- {:::} --- {:::} --- {:::} --- {:::} --- {:::}

Joergen B. Bilde-Soerensen
Senior Research Scientist, Ph. D.
Materials Research Department
Risoe National Laboratory
DK-4000 Roskilde
Denmark

e-mail: j.bilde-at-risoe.dk
phone: +45 4677 5802 (direct)
phone: +45 4677 4677 (switchboard)
fax: +45 4677 5758
website: http://www.risoe.dk/afm/Personal/jqbi/jqbi.htm

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:pzou-at-feico.com]
Sent: 2. september 2004 04:16
To: microscopy-at-microscopy.com

Dear Gary,

I use 4 " sorbothane " mounts (stock number: NT35-264).
Usually I use it for holography but it worked well for damping the rot.
pump vibrations.

---
Shock Absorbing Sorbothane®
{http://www.edmundoptics.com/onlinecatalog/displayproduct.cfm?productID=1806&search=1}
Easily Cut to Size • Ideal For Use In Labs and Assembly Shops Absorbs
up to 95.5% of impact energy, then reforms to its original shape.
Sorbothane® is a solid that behaves like a liquid by absorbing...

Sorbothane® Mounts
{http://www.edmundoptics.com/onlinecatalog/displayproduct.cfm?productID=1618&search=1}

Patented Sorbothane® polymer mount absorbs (57% absorption efficiency)
and dissipates energy (70% specific damping). Reduces vibration to other
components by isolating the vibrations within the materi...

Bases and Platforms
{http://www.edmundoptics.com/onlinecatalog/displayproduct.cfm?productID=1255&search=1}

Large Workstation Platform: Hard-coat black anodized aluminum, 13"W x
18"L x 1/2"T platform with sorbothane feet and 3/4" threaded post hole.
Weighs 12 lbs. Small Platform Base: Hard-coated black anod...
---

Best regards
Timo Junker

Gary Gaugler schrieb:

} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} I'm looking for sources of acoustic/anachoic
} blocks of foam to reduce SEM room interference.
}
} These are like standard anechoic chamber panels.
} I'm having trouble getting above 400KX without
} mechanical noise from the scroll pump that is
} located in a separate room. The acoustical
} isolation from one room to the other is not
} all that great, I suppose.
}
} Does anyone have experience with suppliers of
} these panels? I'd like to glue them to drywall.
}
} Supplier responses are welcomed as off-line
} messages.
}
} gary g.

--
Timo Junker Holografie
Lindenstr. 10
97297 Waldbüttelbrunn
Tel: ++49 (0)931 4520655
Fax: ++49 (0)931 4520657
www.holografie.com

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 11:59:54 2004

Contents Retrieved from Microscopy Listserver Archives
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Francis:

I would suggest that you contact John Coyle at Unitron. You can reach
him by email at : johnc-at-unitronusa.com.

DISCLAIMER: South Bay Technology distributes Unitron Microscopes and,
therefore, has a vested interest in promoting their use.

Best regards-

David

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

by way of Ask-A-Microscopist wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 12:56:44 2004

Contents Retrieved from Microscopy Listserver Archives
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It seems that during the summer months, we have no end of troubles with our
plastic not infiltrating the tissue. I've always assumed that this was
because of the humidity rising quite a bit during the summer months, and the
poor air conditioning.

It comes out as sections falling apart when I try to flatten them in the
water boat, or breaking in the electron beam. We have always kept our epoxy
resin in the freezer in 30 ml plastic syringes, but it usually only gives us
a problem during the summer months. During the winter here, the air is
extremely dry.

We do 4 rinses in absolute alcohol, followed by 3 rinses in propylene oxide,
followed by a 50/50 mixture of epon/araldite mixed with propylene oxide over
night with the caps off, for the propylene oxide evaporating overnight and
slowly leaving the specimens in 100% plastic by morning. We polymerize at
70 deg C overnight, keeping a dessicant in our embedding oven to keep the
air as dry as possible too.

Are there any resins which might be used for electron microscopy which are
more tolerant of water, and which would give a good result with human tissue
in the electron microscope?

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 13:13:39 2004

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Thanks everyone. I've found him.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 13:23:55 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I think Mercury is a free viewer. Check out
http://www.ccdc.cam.ac.uk/products/csd_system/mercury/ It is decent and
works in windows.

-----Original Message-----
} From: hkonishi-at-indiana.edu [mailto:hkonishi-at-indiana.edu]
Sent: Monday, September 13, 2004 9:42 AM
To: Microscopy-at-MSA.Microscopy.Com

I am looking for Windows software that allows me to see crystal structure
with
a less expensive cost. I want to use the software for quick check of number
of
atoms in a unit cell and distance between atoms, looking at crystal
structure,
and making figures for publication. Is there any recommendation?

Thank you,

Hiromi Konishi
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 13:30:21 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Andrei,
The subject of EDS spectra in a TEM or STEM is complex and there are many
different configurations of EDS detector in the TEM column. Some of these
account for the differences in relative background and specific element
signal. If you have a horizontal-mount detector and then tilt the sample
towards the detector, this will pick up a lot of grid and carbon x-rays. I
have a TEM with a high-takeoff-angle detector (68 degrees) and that results
in a much lower Cu and C signal when looking at tiny particles on a
carbon-coated copper grid. A 30 mm2 detector will also pick up more counts
than a 10 mm2. The material in the specimen holder and the column above and
below the sample also affects the relative background of your spectrum. A
TEM really needs to be designed for EDS at the factory, with light-element
inserts to reduce the secondary x-ray radiation that generates much of your
background. The better spectra you are referring to may have come from a TEM
or STEM designed or modified to give the best EDS performance, perhaps at
the cost of less performance in other areas. I know my TEM was designed for
analytical work, at the sacrifice of ultimate resolution.
To increase your counts you can try lowering the accelerating voltage,
increasing the spot size, increasing the condenser aperture size and, of
course, increasing the time you count for. Make sure your objective aperture
is removed, the specimen holder is specified for EDS and your EDS detector
is properly aligned.
Good luck,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca

----- Original Message -----
} From: "by way of MicroscopyListserver" {burnin1970-at-hotmail.com}
To: {microscopy-at-microscopy.com}
Sent: Saturday, September 11, 2004 2:43 PM

Hi, David

There are several sources, depending on the optical requirements. Both Chroma and Omega Filters provide an extensive line of filters. If this are fairly simple scopes, you might also try looking at Edmund Scientific.

If you have trouble finding any of the above, please contact me off-line.

Hope this is helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
F: 972-954-8018

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.
At 11:20 PM 9/9/2004, David Burton wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 15:51:36 2004

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Gary;
Your procedure is similar to the one I use here in Houston where we have
very high humidity also. The difference is that my Epon/araldite: PO step
is for one hour followed by one hour in pure resin then embedded in
capsules in fresh resin. This sets at RT for 3-4 hours then in the oven
overnight at 80 degrees C.
I have been using this method for over 20 years with no problems.

Mannie Steglich
Tech Dir E M Lab
M D Anderson Cancer Center

Garry Burgess {GBurgess-at-exchange.hsc.mb.ca}

09/13/2004 01:24 PM

To:
{Microscopy-at-msa.microscopy.com}
cc:

It seems that during the summer months, we have no end of troubles with
our
plastic not infiltrating the tissue. I've always assumed that this was
because of the humidity rising quite a bit during the summer months, and
the
poor air conditioning.

It comes out as sections falling apart when I try to flatten them in the
water boat, or breaking in the electron beam. We have always kept our
epoxy
resin in the freezer in 30 ml plastic syringes, but it usually only gives
us
a problem during the summer months. During the winter here, the air is
extremely dry.

We do 4 rinses in absolute alcohol, followed by 3 rinses in propylene
oxide,
followed by a 50/50 mixture of epon/araldite mixed with propylene oxide
over
night with the caps off, for the propylene oxide evaporating overnight and
slowly leaving the specimens in 100% plastic by morning. We polymerize at
70 deg C overnight, keeping a dessicant in our embedding oven to keep the
air as dry as possible too.

Are there any resins which might be used for electron microscopy which are
more tolerant of water, and which would give a good result with human
tissue
in the electron microscope?

This e-mail and/or any documents in this transmission is intended for the
address(s) only and may contain legally privileged or confidential
information. Any unauthorized use, disclosure, distribution, copying or
dissemination is strictly prohibited. If you receive this transmission in
error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 16:19:13 2004

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Hi, All-

I have two JB-4 microtomes that I would like to repair, even if only to
get one to work. Neither advance. One has electronic advance and the other
doesn't. I have experience in repairing older ultramicrotomes, but I'd
like to have a set of service instructions, a blueprint, or even a users'
manual in hand before tearing them apart!

Does anyone have these documents? More importantly, perhaps, advice?

Mahalo,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 17:29:13 2004

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Osmium was used in the old days for treatment of arthritis. It
appears to be making a comeback......

http://rheumatology.oupjournals.org/cgi/content/abstract/42/9/1036

}
} That's interesting - what was it used for in 1940?
}
} Lesley Weston.
}
} on 07/09/2004 11:03 AM, Tom Phillips at phillipst-at-missouri.edu wrote:
}
} }
} } I have inherited some aged vials of crystalline osmium. They are a tad
} } older than normal which is to say 1940! But they look quite normal and are
} } sealed in glass ampules just like a more modern vintage. I have offered 30
} } x 1 gm vials so it was hard to not accept the gift; this would be a
} } lifetime supply. I intend to try them out in an experiment tomorrow. If
} } anyone knows why this is doomed to failure, please let me know
} } asap. Otherwise I will let the list know how it works out. Tom
} }
} }
} }
} } Thomas E. Phillips, PhD

--
Dr. Steven Barlow
EM Facility/Biology Dept.
San Diego State University
5500 Campanile Drive
San Diego CA 92182-4614
phone: (619) 594-4523
fax: (619) 594-5676
email: sbarlow-at-sunstroke.sdsu.edu
http://www.sci.sdsu.edu/emfacility

Chairman, Educational Outreach subcommittee
promoting microscopy instruction and increased access to microscopes
Microscopy Society of America
http://www.msa.microscopy.com/

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 18:23:35 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (adriana-at-cab.cnea.gov.ar) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 13, 2004 at 13:56:32
---------------------------------------------------------------------------

Email: adriana-at-cab.cnea.gov.ar
Name: Adriana CondŰ

Organization: CONICET, Argentina.

Title-Subject: [Microscopy] [Filtered] MListserver: CCD for TEM in material science

Question:
Dear microscopists,

We are interested in buying a CCD camera for a Philips CM200 TEM with an ultratwin lens for HRTEM. The main use is for materials science.
We would like to hear comments on the performance of the KeenView CCD camera offered by SIS.
We are particularly concerned with the sensibility for HRTEM (for example typical exposure times) and with the performance of the 12 bit camera for diffraction pattern acquisition and for online astigmatism correction using FFT.

All comments will be appreciated.

Thank you for your help.

Adriana

----------------------------------------------------------
Adriana CondŰ
CONICET Researcher
Metals Physics Group
Centro AtŰmico Bariloche
8400 San Carlos de Bariloche
ARGENTINA
e-mail: adriana-at-cab.cnea.gov.ar
Fax: +54 2944 445299
TE: +54 2944 445290
----------------------------------------------------------

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 13 19:30:57 2004

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Alfred Nobel used Osmium in the production of Explosives in the 1860's. He
is best known for discovering Nitroglycerin & Dynamite (TNT). Now of course
his last will & testament funds "The Nobel Prize".

Al Coritz
Electron Microscopy Sciences
www.emsdiasum.com

----- Original Message -----
} From: {sbarlow-at-sunstroke.sdsu.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Monday, September 13, 2004 6:56 PM

}
} It seems that during the summer months, we have no end of
} troubles with our plastic not infiltrating the tissue. I've
} always assumed that this was because of the humidity rising
} quite a bit during the summer months, and the poor air conditioning.
}
} It comes out as sections falling apart when I try to flatten
} them in the water boat, or breaking in the electron beam. We
} have always kept our epoxy resin in the freezer in 30 ml
} plastic syringes, but it usually only gives us a problem
} during the summer months. During the winter here, the air is
} extremely dry.
}
} We do 4 rinses in absolute alcohol, followed by 3 rinses in
} propylene oxide, followed by a 50/50 mixture of epon/araldite
} mixed with propylene oxide over night with the caps off, for
} the propylene oxide evaporating overnight and slowly leaving
} the specimens in 100% plastic by morning. We polymerize at
} 70 deg C overnight, keeping a dessicant in our embedding oven
} to keep the air as dry as possible too.

Is dessicant effective at 70 deg C, or will it release
moisture accumulated at room temperatures?

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 08:15:50 2004

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I've been following this thread of conversation on old OsO4 with great interest.
I know that there are many (?) books, articles written on the history of
microscopes (esp. electron microscopes), but is there an article/book written on
such interesting facts i.e. OsO4 and othere EM fixatives, etc. I would love to
read more......

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Sample Prep [mailto:sampleprep-at-earthlink.net]
Sent: Monday, September 13, 2004 8:56 PM
To: microscopy-at-msa.microscopy.com; sbarlow-at-sunstroke.sdsu.edu

Alfred Nobel used Osmium in the production of Explosives in the 1860's. He
is best known for discovering Nitroglycerin & Dynamite (TNT). Now of course
his last will & testament funds "The Nobel Prize".

Al Coritz
Electron Microscopy Sciences
www.emsdiasum.com

----- Original Message -----
} From: {sbarlow-at-sunstroke.sdsu.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Monday, September 13, 2004 6:56 PM

Hi Tina,

We manufacture the JB-4 and JB-4A here at EBS. It is our policy to
provide user manuals and telephone support for all of our instruments at
no charge. Please send us your contact information and we'll mail a
manual right out to you. Beyond that, we can also provide you with
factory parts and professional repair services, in the event that you
should you need either.

Sincerely,

Michael R. Nesta
General Manager
Energy Beam Sciences, Inc.
800 992-9037
mnesta-at-ebsciences.com
www.ebsciences.com
"Adding Brilliance to Your Vision"

Tina Carvalho wrote:
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi, All-
}
} I have two JB-4 microtomes that I would like to repair, even if only to
} get one to work. Neither advance. One has electronic advance and the other
} doesn't. I have experience in repairing older ultramicrotomes, but I'd
} like to have a set of service instructions, a blueprint, or even a users'
} manual in hand before tearing them apart!
}
} Does anyone have these documents? More importantly, perhaps, advice?
}
} Mahalo,
} Tina
}
} ****************************************************************************
} * Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
} * Biological Electron Microscope Facility * (808) 956-6251 *
} * University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
} ****************************************************************************
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 12:52:37 2004

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Dear Adriana,

as the manufacturer of the KeenView system I would like to provide the
following information:

1) The KeenView has a high anti-bloom factor of about 300. This means that a
pixel can hold 300 times the saturation charge before blooming occurs.

2) A KeenView system is delivered with the analySIS iTEM software, which
includes a Real-time FFT option for focusing and astigmatism correction.

3) Sensitivity is usually not an issue, unless you wish to do low-dose
cryo-TEM. If you let me know what you plan to do, I can see if I have some
images that I could send you.

Please contact me if you have further questions.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: adriana-at-cab.cnea.gov.ar [mailto:adriana-at-cab.cnea.gov.ar]
Sent: Monday, September 13, 2004 17:52
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (adriana-at-cab.cnea.gov.ar) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Monday, September 13, 2004 at 13:56:32
---------------------------------------------------------------------------

Email: adriana-at-cab.cnea.gov.ar
Name: Adriana CondŰ

Organization: CONICET, Argentina.

Title-Subject: [Microscopy] [Filtered] MListserver: CCD for TEM in material
science

Question:
Dear microscopists,

We are interested in buying a CCD camera for a Philips CM200 TEM with an
ultratwin lens for HRTEM. The main use is for materials science.
We would like to hear comments on the performance of the KeenView CCD camera
offered by SIS.
We are particularly concerned with the sensibility for HRTEM (for example
typical exposure times) and with the performance of the 12 bit camera for
diffraction pattern acquisition and for online astigmatism correction using
FFT.

All comments will be appreciated.

Thank you for your help.

Adriana

----------------------------------------------------------
Adriana CondŰ
CONICET Researcher
Metals Physics Group
Centro AtŰmico Bariloche
8400 San Carlos de Bariloche
ARGENTINA
e-mail: adriana-at-cab.cnea.gov.ar
Fax: +54 2944 445299
TE: +54 2944 445290
----------------------------------------------------------

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 13:50:54 2004

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I don't think water may penetrate epoxy resin easily. The picture, you
described is more like you have water in your sample before plastic. As
far as I could see, the 100% Et-OH step may be a problem in your recipe. 4x
100% Et-OH sounds excessive (I always do 2x20 min 100% Et-OH) - so to me it
looks like that your 100% Et-ON is not a 100% (if you still have water
after 4x). You may need to change the batch or use molecular sieve. You
need also to use at least 1 ml of Et-OH per sample. It's better to do it
in hermetic vials like 1.5 ml Eppendorf tube. If I forgot Et-OH bottle to
close immediately after use, I consider it's 95% Et-OH and use it for
30-95% dehydratation steps only. 3x of PO is sounds excessive too. The
trick here is that as more changes you do, as more your sample has exposed
to water (when you emptied the vial). So, 1 exchange of PO (and Et-OH) is
much better than 3 (you still need 2 for Et-OH) in my point of view. You
need to use huge excess of the solvents - at least 1 ml per sample. As soon
as your sample in PO (or epoxy) - it's protected from water by the layer of
solvent (epoxy). PO and epoxy do not dissolve water, therefore it could
not reach your sample. You still may have a droplets of water (from
condensation for instance) but it'll generate a different picture: round
empty spaces in your sample. You may try also Spurr resin - it may
tolerate a few %% of water in your sample. I hope it'll help, Sergey

At 06:38 AM 9/14/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 17:05:46 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (snyderlt-at-newpaltz.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, September 14, 2004 at 08:42:51
---------------------------------------------------------------------------

Email: snyderlt-at-newpaltz.edu
Name: Teresa Snyder-Leiby

Organization: SUNY New Paltz

Title-Subject: [Microscopy] [Filtered] service for philips 300

Question: We have a philips 300 TEM that has been under service contract for the past 4 years. The company is no longer available and I am trying to find a service provider. We are located in New Paltz, NY, about half way between NYC and Albany.

Any suggestions would be greatly appreciated. Teresa

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 17:23:10 2004

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If the problem is caused by high humidity in the air, you could try using a
water-miscible resin such as Durcupan or Aquembed. They're both a lot more
expensive than Epon-substitutes and Araldite and they polymerise to a rather
soft block, which may or may not matter depending on your tissue, but it
would eliminate the problem if that is the cause. Another possibility is
that there might still be a trace of PO left, if you don't do one more 100%
in the morning before transferring to the DMP-30 mix, but I don't know why
that would happen only in summer. Hope this helps.

Lesley Weston.

on 13/09/2004 11:24 AM, Garry Burgess at GBurgess-at-exchange.hsc.mb.ca wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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--} -
}
}
} It seems that during the summer months, we have no end of troubles with our
} plastic not infiltrating the tissue. I've always assumed that this was
} because of the humidity rising quite a bit during the summer months, and the
} poor air conditioning.
}
} It comes out as sections falling apart when I try to flatten them in the
} water boat, or breaking in the electron beam. We have always kept our epoxy
} resin in the freezer in 30 ml plastic syringes, but it usually only gives us
} a problem during the summer months. During the winter here, the air is
} extremely dry.
}
} We do 4 rinses in absolute alcohol, followed by 3 rinses in propylene oxide,
} followed by a 50/50 mixture of epon/araldite mixed with propylene oxide over
} night with the caps off, for the propylene oxide evaporating overnight and
} slowly leaving the specimens in 100% plastic by morning. We polymerize at
} 70 deg C overnight, keeping a dessicant in our embedding oven to keep the
} air as dry as possible too.
}
} Are there any resins which might be used for electron microscopy which are
} more tolerant of water, and which would give a good result with human tissue
} in the electron microscope?
}
} This e-mail and/or any documents in this transmission is intended for the
} address(s) only and may contain legally privileged or confidential
} information. Any unauthorized use, disclosure, distribution, copying or
} dissemination is strictly prohibited. If you receive this transmission in
} error, please notify the sender immediately and return the original.
}

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 19:37:02 2004

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I have to take exception to some of the assertions made in a recent response to Garry Burgess' posting. First, propylene oxide is completely miscible with water. And second, Spurr's resin is much more likely to have polymerization problems caused by high humidity than is Epon/Araldite type resin mixtures. Spurr's should be cured either in sealed plastic capsules, or if you prefer to use flat molds, with ample fresh desiccant present. I place the flat molds in a sealed Tupperware container, along with plenty of desiccant. The first time I used Spurr's in flat molds on a humid day, I didn't use a desiccant, and the blocks were too soft to section. I repeated the embedding using a desiccant, and the same batch of chemicals, and the blocks were perfect.

We routinely cure our specimens in Epon/Araldite/DDSA without using a desiccant, and never have problems despite summer humidities of 70% or more. We use 3 x 10m changes of 100% ethanol, 3 x 10m changes in PO, infiltrate overnight in 50% resin, and 8 hours the next day in 100% resin, but always in sealed vials. Leaving vials of 50% resin/PO open to the atmosphere on a humid day will result in water absorption, and might be the cause of the problem. Also, I suspect that the propylene oxide might not be completely removed. We use commercial 100% ethanol from plastic bottles with no problems. As was discussed recently in this forum, use of a molecular sieve can result in particles embedded in your specimen, and damage to diamond knives.

In the recent discussion of the merits of BDMA I was surprised to see that people are pre-mixing their resin with DMP-30 or BDMA, and freezing it. Your resin mix will last much longer (at least a couple of months) if you leave out the accelerator. We mix up large batches of our resin, and freeze aliquots of various sizes in glass vials. When we need the resin, we warm it to room temperature, add the appropriate amount of DMP-30, and mix thoroughly. You may spend a little more time mixing in the DMP, but you won't have to worry about your resin thickening in the freezer.

Ralph Common
Michigan State University
Division of Human Pathology

--------------
Original posting from Garry Burgess:

It seems that during the summer months, we have no end of troubles with our
plastic not infiltrating the tissue. I've always assumed that this was
because of the humidity rising quite a bit during the summer months, and the
poor air conditioning.

It comes out as sections falling apart when I try to flatten them in the
water boat, or breaking in the electron beam. We have always kept our epoxy
resin in the freezer in 30 ml plastic syringes, but it usually only gives us
a problem during the summer months. During the winter here, the air is
extremely dry.

We do 4 rinses in absolute alcohol, followed by 3 rinses in propylene oxide,
followed by a 50/50 mixture of epon/araldite mixed with propylene oxide over
night with the caps off, for the propylene oxide evaporating overnight and
slowly leaving the specimens in 100% plastic by morning. We polymerize at
70 deg C overnight, keeping a dessicant in our embedding oven to keep the
air as dry as possible too.

Are there any resins which might be used for electron microscopy which are
more tolerant of water, and which would give a good result with human tissue
in the electron microscope?

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 20:11:54 2004

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margaret

while the thread has been very interesting, your question has been the
most helpful to me. there is a book, it is Hayat's Fixation for
Electron Microscopy. publication date was around 1980. it does not
cover some of the history, but it is an excellent book if you can get
your hands on a copy of it. the help to me....if i can just find that
student who borrowed my copy in june.....

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 14 20:56:29 2004

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Hi, Garry-

I am chronicallly plagued by humidity problems here. Besides making sure
the bottles of absolute ethanol, propylene oxide and resin components, are
opened as little as possible, I put my vials with samples over dessicant
whenever I'm using absolute ethanol, PO, or resin. Always. I have a
rotator we made years ago that accommodates film cans with dessicant into
which my vials fit. I keep dessicant in the embedding oven. And,
imortantly, I pre-heat my molds and labels overnight in the oven before
putting in the samples. This preheating of the capsules or molds and paper
labels also keep bubbles from forming so that I never have to pull a
vacuum on them any more. Yes, it's totally anal, but lots of TEM is!

Good luck!

Aloha,
Tina

} } It seems that during the summer months, we have no end of troubles with our
} } plastic not infiltrating the tissue. I've always assumed that this was
} } because of the humidity rising quite a bit during the summer months, and the
} } poor air conditioning.
} }
} } It comes out as sections falling apart when I try to flatten them in the
} } water boat, or breaking in the electron beam. We have always kept our epoxy
} } resin in the freezer in 30 ml plastic syringes, but it usually only gives us
} } a problem during the summer months. During the winter here, the air is
} } extremely dry.
} }
} } We do 4 rinses in absolute alcohol, followed by 3 rinses in propylene oxide,
} } followed by a 50/50 mixture of epon/araldite mixed with propylene oxide over
} } night with the caps off, for the propylene oxide evaporating overnight and
} } slowly leaving the specimens in 100% plastic by morning. We polymerize at
} } 70 deg C overnight, keeping a dessicant in our embedding oven to keep the
} } air as dry as possible too.

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 03:43:01 2004

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Sergey
A propylene oxide layer over the specimen cannot protect against water
penetration.
Water's solubility in 1,2 propylene oxide (=1,2 epoxypropane) is 14.7 wt%.
Conversely, PPO's solubility in water is 40.5 wt%.

Chris

----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
To: {Microscopy-at-microscopy.com}
Sent: Tuesday, September 14, 2004 8:18 PM

How effective is molecular sieve as a desiccant at typical polymerization
temperatures (60-70 oC)?? I suspect not very. Would there be a better
choice?

I would also be interested to know what strategies people now recommend for
drying EM solvents
without getting them contaminated with bits of desiccant.

And another thing - how on earth can one determine whether the desiccant is
still being effective?
Can you trust the blue indicator in molecular sieves? What is the
equilibrium water concentration in ethanol above fresh molecular sieve
(assuming the ethanol contained some water initially), and does this
increase when the MS contains, say, 10% water (half its saturation
capacity)?

Best wishes
Chris

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 05:35:21 2004

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Each time I post a message to the list a flurry of autoforwarded replies is
generated - "I am in the Bay area", I am on holiday", "I can be reached at
blah blah!", "I am canoeing down the Danube", Etc.
Although fascinating at a sociological level, this is not maximally useful
web traffic at the EM level. Might I respectfully suggest that listers try
to prevent these messages from reaching the list?

Best regards
Chris

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 07:47:27 2004

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Dear Listservers: We have a CM-10 we wish to do both EDS and low temp work
with. We have the Be Gatan cryo-blades from a 400 but need to adapt the column
phlange to fit the CM column. Neither Gatan nor FEI have been able to resolve
this as yet. Does anyone have any advice or spare phlanges so we can get on
with this? I am thankful for any and all advice I can get. Bob Harris

Guelph Regional Imaging Facility
Dept. of Microbiology
Rm 1199 Thornbrough Bldg.
Univ of Guelph
Guelph,On, Canada
N1G 2W1
ph: 519-824-4120 ext. 56409
Fax: 519-837-1802

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 08:37:29 2004

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Colleagues.....

The Listserver rules ask you to NOT USE "I'm not in the office" autoreplies,
instead you should unsubscribe when you go on vacation or out of town.

If you job requires you to use "out of the office" messages for your work Email
then can I suggest you ask your local system guru to setup a second Email address
for Microscopy which you can recieve all the message at and NOT set this function.

I will remind you that ALL postings are archived and if you miss something
you can find it at:

http://www.microscopy.com/MicroscopyListserver

It is also possible to have multiple addresses subscribed, so there are alot
of ways to mitigate this problem with only a few minutes of your time.
The rest of the community will appreciate your thoughtfulness and consideration.

Cheers..

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 08:39:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tem_iopb-at-iopb.res.in) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 15, 2004 at 05:15:20
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Email: tem_iopb-at-iopb.res.in
Name: P. V. Satyam

Organization: Institute of Physics, Bhubaneswar,India

Title-Subject: [Microscopy] MListserver: Polymeric Samples: Sample Stage requirements

Question: Dear All,
I would like to do TEM on
(1) Metal/Semiconducting nano-particles dispersed on polymer surfaces
(for example: Ge on PS)
(2)Langmuir-Blodgett Films

We have JEOL 2010 Ultra High Resolution TEM operating at 200kV and LaB6 Filament.

We tried to work at 200 kV using standard double tilt holder (room temperature) but found that polymeric samples started melting upon e-beam irradiation. We dont want to coat any high Z conducting layer on our sample.

As majority of our work (in materials science) is done using 200 kV, I am concerned to work at lower energies.

Does it help having a cooling holder? If so, are there any particulars that should be taken care before purchasing so as enable us to work with polymer and LB films?

I will appreciate your suggestions either directly to me or to the list.

Best regards
Satyam
Institute of Physics, Bhubaneswar, India
Home page: www.iopb.res.in/~tem_iopb

tem_iopb-at-iopb.res.in or satyam-at-iopb.res.in

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From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 08:53:41 2004

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Chris

to avoid the bits in your solvents, try putting your molecular sieve (or whatever) into a length of dialysis tubing. You can fold the ends over and staple them to form a small sausage.

If you get any answers to the rest of your questions I, for one, would be interested to hear them.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Chris Jeffree {c.jeffree-at-ed.ac.uk}

Hi Chris,

I am out of the office and canoeing on the Current River. I will reply
to your email soon, if I don't drown.

Seriously though, I asked a similar question a while back and was told
that molecular sieves can be put in dialysis tubing to keep them from
chunking up your solvents. Basically, we have quit using molecular
sieves just in case they were responsible for what we thought was
excessive wear on our diamond knives. Since we use a lot of microwave
processing, we generally use acetone, rather than ethanol, and mix our
dehydration series fresh each time. When I use ethanol, I usually
finish up with a recently opened bottle of absolute, but after two or
three uses I relegate that bottle to the 90-95% category, and open up a
new one for the final steps.

This seems to work for us, as we rarely have infiltration problems, even
with retinal tissue which can be problematic.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Wednesday, September 15, 2004 5:40 AM
To: microscopy-at-msa.microscopy.com

How effective is molecular sieve as a desiccant at typical
polymerization temperatures (60-70 oC)?? I suspect not very. Would
there be a better choice?

I would also be interested to know what strategies people now recommend
for drying EM solvents without getting them contaminated with bits of
desiccant.

And another thing - how on earth can one determine whether the desiccant
is still being effective?
Can you trust the blue indicator in molecular sieves? What is the
equilibrium water concentration in ethanol above fresh molecular sieve
(assuming the ethanol contained some water initially), and does this
increase when the MS contains, say, 10% water (half its saturation
capacity)?

Best wishes
Chris

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 09:04:23 2004

Contents Retrieved from Microscopy Listserver Archives
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Malcolm
Thanks for this.I have heard it suggested previously, but I am sceptical
about it.

1) Presumably the dialysis tubing has to be wet before it can be loaded?.
OK, so you can re-dry the MS after loading.
2) I wonder what the permeability of dialysis tubing is to water vapour when
very dry and
immersed in ethanol. It that environment it will be in its most
ultra-compact precipitated state
(since ethanol precipitates polysaccharides from aqueous solution).
3) As in my original question, do you really know that it works, and if so,
from what sort of evidence?

Best wishes
Chris

----- Original Message -----
} From: "Malcolm Haswell" {malcolm.haswell-at-sunderland.ac.uk}
To: "Microscopy MSA" {Microscopy-at-microscopy.com}
Cc: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
Sent: Wednesday, September 15, 2004 3:20 PM

I'm curious about this, how was it used and what explosive was made. By the way Dynamite is not TNT. Dynamite is Nitroglycerin soaked into a diatomaceous earth called Kieselguhr (other absorbents have been used too), this is the explosive invented by Nobel that founded his munitions industry. Dynamite Nobel is still one of the worlds largest munitions makers. TNT is Trinitrotoluene, a different explosive, invented by Wilbrand. For more info on this see: http://en.wikipedia.org/wiki/TNT_(explosive)
and http://en.wikipedia.org/wiki/Dynamite

James L. Roberts
Firearm & Toolmark Examiner
Ventura Co. Sheriff's Lab
800 S. Victoria Ave.
Ventura, CA. 93009

(805) 654-2308

James.Roberts-at-mail.co.ventura.ca.us

} } } "Sample Prep" {sampleprep-at-earthlink.net} 09/13/04 05:56PM } } }

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Alfred Nobel used Osmium in the production of Explosives in the 1860's. He
is best known for discovering Nitroglycerin & Dynamite (TNT). Now of course
his last will & testament funds "The Nobel Prize".

Al Coritz
Electron Microscopy Sciences
www.emsdiasum.com

----- Original Message -----
} From: {sbarlow-at-sunstroke.sdsu.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Monday, September 13, 2004 6:56 PM

Chris
Molecular sieve usually used for removing water from the solvents like
Et-OH etc. It has very high capacity and quite effective. Unfortunately
(at my knowledge) molecular sieve does not have indicators signaling it's
time to change sieve. As far as I know, if you add sieve in proportion 10%
from volume, it should work effectively for couple of month (we are talking
about adding molecular sieve to absolute 200 proof ethanol). You may
regenerate molecular sieve at +200-250oC (24-48 h). The disadvantage of
the sieve is that you may have particles in your sample (you right). There
was posting on ListServer a few years ago that people used syringes with
0.22 mkm filters to remove particles. I don't remember details. In my
experience, if I don't disturb solution, it's OK, no particles. Another
popular desiccant is "anhydrous calcium sulfate" - this one do change the
color and may be used for liquids or gases (for some reasons I did not hear
that molecular sieve used for gases). All these materials are capable to
remove the TRACES of water from your solution. If you have 10% water, you
have to distill solvent first and then treat with few portions of
desiccant. Personally, I am using 200 proof ethanol without any
desiccants. I prefer to open new bottle if sample is
important. Otherwise, I am using the bottle a few times as a 100% Et-OH
and then use it for 30-95% dehydratation steps. Have a great day, Sergey

At 03:39 AM 9/15/2004, you wrote:

} ------------------------------------------------------------------------------
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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 12:33:31 2004

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Yes it has to be wetted, but just wet the end and pour the sieve in with a funnel. Trim off the wet part and either tie or staple the ends. As for working, I also make a little packet of cupric sulfate the same way as an indicator and it turns blue indicating it has taken up moisture.

Dry it over a flame until it turns white. Recharge when blue. I generally need to do this once a year up here. all my 100% solutions (ethanol, acetone, and HMDS) are on sieve.

Scott Whittaker
Laboratories of Analytical Biology
Smithsonian Institution
National Museum of Natural History
PO Box 37012 MRC104
Washington DC 20013-7012
***New Number202-633-0891***

} } } "Chris Jeffree" {c.jeffree-at-ed.ac.uk} 09/15/04 10:27AM } } }

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Malcolm
Thanks for this.I have heard it suggested previously, but I am sceptical
about it.

1) Presumably the dialysis tubing has to be wet before it can be loaded?.
OK, so you can re-dry the MS after loading.
2) I wonder what the permeability of dialysis tubing is to water vapour when
very dry and
immersed in ethanol. It that environment it will be in its most
ultra-compact precipitated state
(since ethanol precipitates polysaccharides from aqueous solution).
3) As in my original question, do you really know that it works, and if so,
from what sort of evidence?

Best wishes
Chris

----- Original Message -----
} From: "Malcolm Haswell" {malcolm.haswell-at-sunderland.ac.uk}
To: "Microscopy MSA" {Microscopy-at-microscopy.com}
Cc: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
Sent: Wednesday, September 15, 2004 3:20 PM

We have been using molecular sieve in dialysis tubing for at least
20 years as a means of drying our 100% ethanol and acetone. Note that I am
in Florida where the humidity is quite high for many months out of the
year. Dry dialysis tubing can be opened, in order to fill it, by getting a
small opening at one end and then blowing air through it to force it open
all the way. A little blue indicator silica gel can be added for ethanol,
but not acetone, since the dye is acetone soluble.

Greg Erdos, Hurricane Country

} Malcolm
} Thanks for this.I have heard it suggested previously, but I am sceptical
} about it.
}
} 1) Presumably the dialysis tubing has to be wet before it can be loaded?.
} OK, so you can re-dry the MS after loading.
} 2) I wonder what the permeability of dialysis tubing is to water vapour when
} very dry and
} immersed in ethanol. It that environment it will be in its most
} ultra-compact precipitated state
} (since ethanol precipitates polysaccharides from aqueous solution).
} 3) As in my original question, do you really know that it works, and if so,
} from what sort of evidence?
}
} Best wishes
} Chris
}
} ----- Original Message -----
} } From: "Malcolm Haswell" {malcolm.haswell-at-sunderland.ac.uk}
} To: "Microscopy MSA" {Microscopy-at-microscopy.com}
} Cc: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
} Sent: Wednesday, September 15, 2004 3:20 PM
} Subject: [Microscopy] Re: infiltration problems - suitable desiccants
}
}
} } Chris
} }
} } to avoid the bits in your solvents, try putting your molecular sieve (or
} whatever) into a length of dialysis tubing. You can fold the ends over and
} staple them to form a small sausage.
} }
} } If you get any answers to the rest of your questions I, for one, would be
} interested to hear them.
} }
} } Malcolm
} }
} } Malcolm Haswell
} } e.m. unit
} } School of Health, Natural and Social Sciences
} } Fleming Building
} } University of Sunderland
} } Tyne & Wear
} } SR1 3SD
} } UK
} } e-mail: malcolm.haswell-at-sunderland.ac.uk
} }
} } ----- Original Message -----
} } From: Chris Jeffree {c.jeffree-at-ed.ac.uk}
} } Date: Wednesday, September 15, 2004 11:39 am
} } Subject: [Microscopy] infiltration problems - suitable desiccants
} }
} } }
} } }
} } } -------------------------------------------------------------------
} } } -----------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } AmericaTo Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserverOn-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html--------
} } } -------------------------------------------------------------------
} } } ----
} } }
} } } How effective is molecular sieve as a desiccant at typical
} } } polymerizationtemperatures (60-70 oC)?? I suspect not very. Would
} } } there be a better
} } } choice?
} } }
} } } I would also be interested to know what strategies people now
} } } recommend for
} } } drying EM solvents
} } } without getting them contaminated with bits of desiccant.
} } }
} } } And another thing - how on earth can one determine whether the
} } } desiccant is
} } } still being effective?
} } } Can you trust the blue indicator in molecular sieves? What is the
} } } equilibrium water concentration in ethanol above fresh molecular sieve
} } } (assuming the ethanol contained some water initially), and does this
} } } increase when the MS contains, say, 10% water (half its saturation
} } } capacity)?
} } }
} } } Best wishes
} } } Chris
} } }
} } }
} } }
} }
} }

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 13:10:43 2004

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I use acetone for my dehydrations (prior to SPurr's infiltration). My
professor taught me years ago (and I teach my students now) to dehydrate
acetone with CuSO4. Place about 50-100g of CuSO4 in an evaporating dish
in a muffle furnace for about 6 hrs. The deep aqua crystals will turn to
a white powder with a faint greenish cast. Allow to cool slightly (in the
furnace), add to an empty bottle, add "100%" acetone from a freshly opened
500 mL bottle, shake, and allow to settle over night. As long as the
copper sulfate does not change color, the acetone is assumed to be
adequately desiccated. I've used this with complete success for acetone,
with not apparent affect on specimens from the copper. I have no idea
whether it works for EtOH.

Don

______________________________________________________________________
Donald L. Lovett e-mail: lovett-at-tcnj.edu
Assoc. Professor, Dept. of Biology voice: (609) 771-2876
P.O. Box 7718 fax: (609) 637-5118
The College of New Jersey
Ewing, NJ 08628-0718

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 13:39:19 2004

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Hello Listers
I have been reading the replies with great interest because I too
have been struggling with incomplete dehydration/poor infiltration problems
with 7 day zebrafish brain in very dry California. I am using a combination
of microwave and bench processing. My dehydration steps are done under
vacuum on the stedi-temp in the microwave(power level 3, 40 seconds each
100% 1 minute each)and I do 100% ethanol 4x (bottle used only 3 times
before new one is opened, no molecular sieves.)
Moving to 100% acetone and sometimes even PPO and infiltrating with acetone
-resin mixture or PPO/resin. I include 1 overnight step, in 50-50 on
rotator, then 100% for several hours on rotator. I have tried epon/araldite
(frozen with accelerator-made fresh every 3 months) and recently Embed It
(Polysciences Spurr like formulation).
I have white holes or empty areas -sometimes myelin like figures. I have
looked at conventionally prepared tissue that doesn't have it and was
dehydrated for longer periods so I think it is a dehydration problem. The
microwave fixation is far superior to the bench fixed material so I don't
think it can be blamed on the microwave. I have just ordered new acetone in
smaller bottles thinking that maybe my acetone had taken on water. I
process in dram glass vials and always keep the tissue covered.
It is only this darn fish that gives me this trouble. I.have done mouse
brain, Drosophila, rat heart, 5 day fish all using this protocol with great
results. There must be water somewhere but it is hard to track down. This
fish brain is very dense material, along with the skin around it. I dissect
away the eyes and jaw to improve penetration.
Is there anyone out there who has seen this problem before? I'd love some
advice.
Frustrated in California, JoAnn Buchanan

Department of Molecular and Cellular Physiology
Stanford University School of Medicine
Stanford, CA 94305
650-723-5856

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 13:43:13 2004

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Dear List;

On the subject of humidity causing poor infiltration ....... several
of my colleagues go from 95% ethanol to Epon substitutes without any
problems. No absolute alcohol, no propylene oxide. Yes, extra changes of
epoxy are needed but the results are fine. Hayat's Prin. and Tech of EM,
second ed., vol 1, page 154 reports that Epon is miscible with 70% ethanol.
I was "raised" with the "you must get every last molecule of water
out of the specimen" dogma but eperience had taught me otherwise. I
suggest you look elsewhere for the cause of your difficulties.

Geoff

Chris Jeffree wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 13:56:24 2004

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I want to buy a grinder/polisher that works with Gatan 623 Disc Grinder or SPI
Precision Disc Grinder. Does anyone use "8” Grinder/Polisher" from Electron
Microscopy Sciences with Disc Grinder? Is there any other recommendation? I
would find a grinder around 1-2K.
Thank you,
Hiromi Konishi
Indiana University

Product:
http://www.emsdiasum.com/microscopy/products/materials/polishing.aspx?
mm=9

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 14:10:26 2004

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I've always for the last 20 years used digital balances to measure out
quantities of resin components to mix up plastics, but I'm curious as to why
the manufacturers always specify the amount in volume measures instead of
weight, since it seems to me that it would be a tough job to clean out grad
cylinders full of resin components, vs just filling up a plastic beaker on a
balance, and disposing of it afterwards.

I was just curious as to how others do their measuring, and if they resort
to the horrifying task of cleaning glassware of resin components, which
strikes me as a particularly nasty job.

Garry Burgess

Charge Technologist
Department of Pathology
Health Sciences Centre
Winnipeg, Canada

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 14:25:01 2004

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Dear Satyam,

What, specifically, are you trying to image in these samples? It may be that TEM is not the right tool. An associate of mine has been imaging LB and polymer films with AFM and AFAM (Atomic Force Acoustical Microscopy), with great success and no damage. Contact me off-line if you are interested in details.

Thanks
Barbara Foster
Microscopy/Microscopy Education

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Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.

At 09:07 AM 9/15/2004, tem_iopb-at-iopb.res.in wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 16:40:37 2004

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Garry, we measure in volume equivalents, one ml per gram. Although I
recognize that the differing specific gravities of the various
components means that these are not exactly equivalent measures, it
works well for us.

We use 30 ml syringes sans needles to measure the components---pop out
the plunger (and make sure the syringe cap is on!) and fill the body of
the syringe up to the appropriate mark. Reinsert the plunger and push
out the goo into a plastic mixing cup. Repeat for the other components.
Not only is this quick, easy, and about as mess free as working with
resins ever gets, but you get some interesting sound effects that raise
eyebrows on people not in the know. As an added bonus, if you pour the
mixed resin back in the syringes, they make for nice freezer storage and
easy dispensing. When empty, just throw them into an oven until the
remnants are polymerized and toss the used syringes.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

-----Original Message-----
} From: Garry Burgess [mailto:GBurgess-at-exchange.hsc.mb.ca]
Sent: Wednesday, September 15, 2004 2:38 PM
To: microscopy-at-microscopy.com

I've always for the last 20 years used digital balances to measure out
quantities of resin components to mix up plastics, but I'm curious as to
why the manufacturers always specify the amount in volume measures
instead of weight, since it seems to me that it would be a tough job to
clean out grad cylinders full of resin components, vs just filling up a
plastic beaker on a balance, and disposing of it afterwards.

I was just curious as to how others do their measuring, and if they
resort to the horrifying task of cleaning glassware of resin components,
which strikes me as a particularly nasty job.

Garry Burgess

Charge Technologist
Department of Pathology
Health Sciences Centre
Winnipeg, Canada

This e-mail and/or any documents in this transmission is intended for
the address(s) only and may contain legally privileged or confidential
information. Any unauthorized use, disclosure, distribution, copying or
dissemination is strictly prohibited. If you receive this transmission
in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 16:56:07 2004

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Dear Hiromi,
Because the amount of material removed from 3.05 mm TEM discs with the Gatan
Disc Grinder is very small, I use 600 grit paper stuck to a glass sheet and
carefully hand grind the samples under running water, then finish off with
1200 grit the same way. It only takes a few strokes to remove 50 microns,
then advance the dial and remove another 50 microns. We have spinning wheel
grinders and automatic polishers, but I would not use them for this.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {hkonishi-at-indiana.edu}
To: {Microscopy-at-microscopy.com}
Sent: Wednesday, September 15, 2004 12:23 PM

Dear Garry,
I found that 1 oz. medicine cups, available from medical suppliers in 1000
cup batches, are disposable and marked off in ml. They hold about 30 ml and
do one or two 1-inch mounts. I use the Tri-pour plastic beakers, which my
Stores man assures me are inexpensive, for larger amounts. I have also heard
that some people use disposable syringes.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Garry Burgess" {GBurgess-at-exchange.hsc.mb.ca}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, September 15, 2004 12:37 PM

In dense plant tissues, we generally get problems in embedded tissues not
because of incomplete dehydration, but due to infiltration either too fast
or in steps that are too large. If cell walls are moderately impermeable,
then solvent may diffuse out of the tissue faster than resin can diffuse in,
causing tissue collapse and "airspaces" when remaining traces of solvent
within such tissue vapourise during polymerisation. Slower infiltration,
with smaller increases of % resin in solvent, and holding the tissue longer
at each step, has generally solved this problem, for us, anyway.

As an example, a friend found that the single- to few-celled algal zygotes
she was working on had to be infiltrated in increments of 1-2% resin per day
up to 10% or so, after which the increments could be larger, then above 90%
resin, the increments had to be smaller again (don't remember all the
details). If this wasn't done, the zygotes looked like flat balloons after
resin polymerisation.

Not sure if this applies to animal tissues but is another protocol
modification to try....
cheers,
Rosemary

Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 02-6246 5475
CSIRO Plant Industry mob. 0402 835 973
GPO Box 1600 fax. 02-6246 5000
Canberra, ACT 2601

} From: JoAnn Buchanan {redhair-at-stanford.edu}
} Date: Wed, 15 Sep 2004 12:06:49 -0700
} To: {Microscopy-at-msa.microscopy.com}
} Subject: [Microscopy] Infiltration Problems
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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}
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-
}
} Hello Listers
} I have been reading the replies with great interest because I too
} have been struggling with incomplete dehydration/poor infiltration problems
} with 7 day zebrafish brain in very dry California. I am using a combination
} of microwave and bench processing. My dehydration steps are done under
} vacuum on the stedi-temp in the microwave(power level 3, 40 seconds each
} 100% 1 minute each)and I do 100% ethanol 4x (bottle used only 3 times
} before new one is opened, no molecular sieves.)
} Moving to 100% acetone and sometimes even PPO and infiltrating with acetone
} -resin mixture or PPO/resin. I include 1 overnight step, in 50-50 on
} rotator, then 100% for several hours on rotator. I have tried epon/araldite
} (frozen with accelerator-made fresh every 3 months) and recently Embed It
} (Polysciences Spurr like formulation).
} I have white holes or empty areas -sometimes myelin like figures. I have
} looked at conventionally prepared tissue that doesn't have it and was
} dehydrated for longer periods so I think it is a dehydration problem. The
} microwave fixation is far superior to the bench fixed material so I don't
} think it can be blamed on the microwave. I have just ordered new acetone in
} smaller bottles thinking that maybe my acetone had taken on water. I
} process in dram glass vials and always keep the tissue covered.
} It is only this darn fish that gives me this trouble. I.have done mouse
} brain, Drosophila, rat heart, 5 day fish all using this protocol with great
} results. There must be water somewhere but it is hard to track down. This
} fish brain is very dense material, along with the skin around it. I dissect
} away the eyes and jaw to improve penetration.
} Is there anyone out there who has seen this problem before? I'd love some
} advice.
} Frustrated in California, JoAnn Buchanan
}
} Department of Molecular and Cellular Physiology
} Stanford University School of Medicine
} Stanford, CA 94305
} 650-723-5856
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 17:58:07 2004

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Garry

We have used weight measurement for many years. We have a scale in a hood
and use gloves and all disposable containers so dare not too concerned about
the resin components being hazardous. We mix resins as needed rather than
mix large batches and freeze aliquots since it only takes a few minutes to
mix the resins in the quantity we need. This works fine and we get
consistent resin properties in our blocks.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 9/15/04 2:37 PM, "Garry Burgess" {GBurgess-at-exchange.hsc.mb.ca} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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}
}
} I've always for the last 20 years used digital balances to measure out
} quantities of resin components to mix up plastics, but I'm curious as to why
} the manufacturers always specify the amount in volume measures instead of
} weight, since it seems to me that it would be a tough job to clean out grad
} cylinders full of resin components, vs just filling up a plastic beaker on a
} balance, and disposing of it afterwards.
}
} I was just curious as to how others do their measuring, and if they resort
} to the horrifying task of cleaning glassware of resin components, which
} strikes me as a particularly nasty job.
}
} Garry Burgess
}
} Charge Technologist
} Department of Pathology
} Health Sciences Centre
} Winnipeg, Canada
}
} This e-mail and/or any documents in this transmission is intended for the
} address(s) only and may contain legally privileged or confidential
} information. Any unauthorized use, disclosure, distribution, copying or
} dissemination is strictly prohibited. If you receive this transmission in
} error, please notify the sender immediately and return the original.
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 19:55:36 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Hiromi:

The EMS Polisher you reference would certainly be suitable for use with
the disc grinder. Mary Mager makes a good point that a rotating wheel
may not be necessary - or even desirable - if you don't have a lot of
material to remove. I can offer a few suggestions:

Rotating Wheel
If you do require a rotating wheel, our Model 900 Grinder/Polisher is an
enconomical solution that would be suitable for the disc grinder you
describe.

Hand Polishing
If you decide to go with a manual hand polishing process, I would
suggest our Model 180 Lapping Tray. This is essentially a glass plate
mounted in an aluminum base. It is set up to collect waste water and
debris and comes with a cover that allows you to stack multiple trays
each with a different grit size abrasive.

We also have a wide range of other polishing tools and supplies that may
be of interest. I would be pleased to discuss your application with you
in detail off-line.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

hkonishi-at-indiana.edu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 20:34:08 2004

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Dear Hiromi,
Because the amount of material removed from 3.05 mm TEM discs with the Gatan
Disc Grinder is very small, I use 600 grit paper stuck to a glass sheet and
carefully hand grind the samples under running water, then finish off with
1200 grit the same way. It only takes a few strokes to remove 50 microns,
then advance the dial and remove another 50 microns. We have spinning wheel
grinders and automatic polishers, but I would not use them for this.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {hkonishi-at-indiana.edu}
To: {Microscopy-at-microscopy.com}
Sent: Wednesday, September 15, 2004 12:23 PM

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Garry, we measure in volume equivalents, one ml per gram. Although I
recognize that the differing specific gravities of the various
components means that these are not exactly equivalent measures, it
works well for us.

We use 30 ml syringes sans needles to measure the components---pop out
the plunger (and make sure the syringe cap is on!) and fill the body of
the syringe up to the appropriate mark. Reinsert the plunger and push
out the goo into a plastic mixing cup. Repeat for the other components.
Not only is this quick, easy, and about as mess free as working with
resins ever gets, but you get some interesting sound effects that raise
eyebrows on people not in the know. As an added bonus, if you pour the
mixed resin back in the syringes, they make for nice freezer storage and
easy dispensing. When empty, just throw them into an oven until the
remnants are polymerized and toss the used syringes.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

-----Original Message-----
} From: Garry Burgess [mailto:GBurgess-at-exchange.hsc.mb.ca]
Sent: Wednesday, September 15, 2004 2:38 PM
To: microscopy-at-microscopy.com

I've always for the last 20 years used digital balances to measure out
quantities of resin components to mix up plastics, but I'm curious as to
why the manufacturers always specify the amount in volume measures
instead of weight, since it seems to me that it would be a tough job to
clean out grad cylinders full of resin components, vs just filling up a
plastic beaker on a balance, and disposing of it afterwards.

I was just curious as to how others do their measuring, and if they
resort to the horrifying task of cleaning glassware of resin components,
which strikes me as a particularly nasty job.

Garry Burgess

Charge Technologist
Department of Pathology
Health Sciences Centre
Winnipeg, Canada

This e-mail and/or any documents in this transmission is intended for
the address(s) only and may contain legally privileged or confidential
information. Any unauthorized use, disclosure, distribution, copying or
dissemination is strictly prohibited. If you receive this transmission
in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 20:34:25 2004

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Garry

We have used weight measurement for many years. We have a scale in a hood
and use gloves and all disposable containers so dare not too concerned about
the resin components being hazardous. We mix resins as needed rather than
mix large batches and freeze aliquots since it only takes a few minutes to
mix the resins in the quantity we need. This works fine and we get
consistent resin properties in our blocks.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 9/15/04 2:37 PM, "Garry Burgess" {GBurgess-at-exchange.hsc.mb.ca} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
}
} I've always for the last 20 years used digital balances to measure out
} quantities of resin components to mix up plastics, but I'm curious as to why
} the manufacturers always specify the amount in volume measures instead of
} weight, since it seems to me that it would be a tough job to clean out grad
} cylinders full of resin components, vs just filling up a plastic beaker on a
} balance, and disposing of it afterwards.
}
} I was just curious as to how others do their measuring, and if they resort
} to the horrifying task of cleaning glassware of resin components, which
} strikes me as a particularly nasty job.
}
} Garry Burgess
}
} Charge Technologist
} Department of Pathology
} Health Sciences Centre
} Winnipeg, Canada
}
} This e-mail and/or any documents in this transmission is intended for the
} address(s) only and may contain legally privileged or confidential
} information. Any unauthorized use, disclosure, distribution, copying or
} dissemination is strictly prohibited. If you receive this transmission in
} error, please notify the sender immediately and return the original.
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 20:34:19 2004

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In dense plant tissues, we generally get problems in embedded tissues not
because of incomplete dehydration, but due to infiltration either too fast
or in steps that are too large. If cell walls are moderately impermeable,
then solvent may diffuse out of the tissue faster than resin can diffuse in,
causing tissue collapse and "airspaces" when remaining traces of solvent
within such tissue vapourise during polymerisation. Slower infiltration,
with smaller increases of % resin in solvent, and holding the tissue longer
at each step, has generally solved this problem, for us, anyway.

As an example, a friend found that the single- to few-celled algal zygotes
she was working on had to be infiltrated in increments of 1-2% resin per day
up to 10% or so, after which the increments could be larger, then above 90%
resin, the increments had to be smaller again (don't remember all the
details). If this wasn't done, the zygotes looked like flat balloons after
resin polymerisation.

Not sure if this applies to animal tissues but is another protocol
modification to try....
cheers,
Rosemary

Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 02-6246 5475
CSIRO Plant Industry mob. 0402 835 973
GPO Box 1600 fax. 02-6246 5000
Canberra, ACT 2601

} From: JoAnn Buchanan {redhair-at-stanford.edu}
} Date: Wed, 15 Sep 2004 12:06:49 -0700
} To: {Microscopy-at-msa.microscopy.com}
} Subject: [Microscopy] Infiltration Problems
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Hello Listers
} I have been reading the replies with great interest because I too
} have been struggling with incomplete dehydration/poor infiltration problems
} with 7 day zebrafish brain in very dry California. I am using a combination
} of microwave and bench processing. My dehydration steps are done under
} vacuum on the stedi-temp in the microwave(power level 3, 40 seconds each
} 100% 1 minute each)and I do 100% ethanol 4x (bottle used only 3 times
} before new one is opened, no molecular sieves.)
} Moving to 100% acetone and sometimes even PPO and infiltrating with acetone
} -resin mixture or PPO/resin. I include 1 overnight step, in 50-50 on
} rotator, then 100% for several hours on rotator. I have tried epon/araldite
} (frozen with accelerator-made fresh every 3 months) and recently Embed It
} (Polysciences Spurr like formulation).
} I have white holes or empty areas -sometimes myelin like figures. I have
} looked at conventionally prepared tissue that doesn't have it and was
} dehydrated for longer periods so I think it is a dehydration problem. The
} microwave fixation is far superior to the bench fixed material so I don't
} think it can be blamed on the microwave. I have just ordered new acetone in
} smaller bottles thinking that maybe my acetone had taken on water. I
} process in dram glass vials and always keep the tissue covered.
} It is only this darn fish that gives me this trouble. I.have done mouse
} brain, Drosophila, rat heart, 5 day fish all using this protocol with great
} results. There must be water somewhere but it is hard to track down. This
} fish brain is very dense material, along with the skin around it. I dissect
} away the eyes and jaw to improve penetration.
} Is there anyone out there who has seen this problem before? I'd love some
} advice.
} Frustrated in California, JoAnn Buchanan
}
} Department of Molecular and Cellular Physiology
} Stanford University School of Medicine
} Stanford, CA 94305
} 650-723-5856
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 20:41:51 2004

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Garry

We have always measured our Spurr's resin components by weight, most of the recipes for this resin seem to do this. I agree most of the literature on other resins seems to quote volumes though in the latest edition of Glauerts book on Biological Specimen Preparation weight equivalents are given (proportions are close to but not identical to those using 1g = 1ml)

The reference is
Biological Specimen Preparation for Transmission Electron Microscopy - Audrey M. Glauert and Peter R. Lewis
Practical Methods in Electron Microscopy: Vol 17
Portland Press London 1998

The earlier version of this (1974) only seems to note volumes.

Ian

Ian Hallett
HortResearch
Mt Albert Research Centre, Private Bag 92 169
Auckland, New Zealand
Fax +64 9 815 4201
Telephone +64 9 815 4200
EMail ihallett-at-hortresearch.co.nz

} } } Garry Burgess {GBurgess-at-exchange.hsc.mb.ca} 16/09/2004 7:37:56 a.m. } } }

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I've always for the last 20 years used digital balances to measure out
quantities of resin components to mix up plastics, but I'm curious as to why
the manufacturers always specify the amount in volume measures instead of
weight, since it seems to me that it would be a tough job to clean out grad
cylinders full of resin components, vs just filling up a plastic beaker on a
balance, and disposing of it afterwards.

I was just curious as to how others do their measuring, and if they resort
to the horrifying task of cleaning glassware of resin components, which
strikes me as a particularly nasty job.

Garry Burgess

Charge Technologist
Department of Pathology
Health Sciences Centre
Winnipeg, Canada

This e-mail and/or any documents in this transmission is intended for the address(s) only and may contain legally privileged or confidential information. Any unauthorized use, disclosure, distribution, copying or dissemination is strictly prohibited. If you receive this transmission in error, please notify the sender immediately and return the original.

______________________________________________________

The contents of this e-mail are privileged and/or confidential to the
named recipient and are not to be used by any other person and/or
organisation. If you have received this e-mail in error, please notify
the sender and delete all material pertaining to this e-mail.
______________________________________________________

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 23:12:08 2004

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It works perfectly with Et-OH and this is exactly how they teach me. Yes,
CuSO4 - it was many years ago. Thanks for reminding. Sergey

At 11:37 AM 9/15/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 23:20:35 2004

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Chris, you right.
I am sorry, I was surely believe that PPO does not soluble in the
water. So, my theory that PPO may "protect" sample from the water is
wrong. From another hand I never used desiccants with PPO. PPO comes in
0.5 liter cans and I opened it frequently. Nevertheless, I did not have
problems with water. Anyway, thanks for clarification and have a great
day/night. Sergey

At 02:06 AM 9/15/2004, you wrote:
} Sergey
} A propylene oxide layer over the specimen cannot protect against water
} penetration.
} Water's solubility in 1,2 propylene oxide (=1,2 epoxypropane) is 14.7 wt%.
} Conversely, PPO's solubility in water is 40.5 wt%.
}
} Chris
}
} ----- Original Message -----
} From: "Sergey Ryazantsev" {sryazant-at-ucla.edu}
} To: {Microscopy-at-microscopy.com}
} Sent: Tuesday, September 14, 2004 8:18 PM
} Subject: [Microscopy] Re: RE: Infiltration Problems
}
}
} }
} }
} } --------------------------------------------------------------------------
} ----
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
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} } --------------------------------------------------------------------------
} -----
} }
} } I don't think water may penetrate epoxy resin easily. The picture, you
} } described is more like you have water in your sample before plastic. As
} } far as I could see, the 100% Et-OH step may be a problem in your recipe.
} 4x
} } 100% Et-OH sounds excessive (I always do 2x20 min 100% Et-OH) - so to me
} it
} } looks like that your 100% Et-ON is not a 100% (if you still have water
} } after 4x). You may need to change the batch or use molecular sieve. You
} } need also to use at least 1 ml of Et-OH per sample. It's better to do it
} } in hermetic vials like 1.5 ml Eppendorf tube. If I forgot Et-OH bottle to
} } close immediately after use, I consider it's 95% Et-OH and use it for
} } 30-95% dehydratation steps only. 3x of PO is sounds excessive too. The
} } trick here is that as more changes you do, as more your sample has exposed
} } to water (when you emptied the vial). So, 1 exchange of PO (and Et-OH) is
} } much better than 3 (you still need 2 for Et-OH) in my point of view. You
} } need to use huge excess of the solvents - at least 1 ml per sample. As
} soon
} } as your sample in PO (or epoxy) - it's protected from water by the layer
} of
} } solvent (epoxy). PO and epoxy do not dissolve water, therefore it could
} } not reach your sample. You still may have a droplets of water (from
} } condensation for instance) but it'll generate a different picture: round
} } empty spaces in your sample. You may try also Spurr resin - it may
} } tolerate a few %% of water in your sample. I hope it'll help, Sergey
} }
} } At 06:38 AM 9/14/2004, you wrote:
} }
} }
} }
} } ---------------------------------------------------------------------------
} ---
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
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} }
} } ---------------------------------------------------------------------------
} ----
} } }
} } } }
} } } } It seems that during the summer months, we have no end of
} } } } troubles with our plastic not infiltrating the tissue. I've
} } } } always assumed that this was because of the humidity rising
} } } } quite a bit during the summer months, and the poor air conditioning.
} } } }
} } } } It comes out as sections falling apart when I try to flatten
} } } } them in the water boat, or breaking in the electron beam. We
} } } } have always kept our epoxy resin in the freezer in 30 ml
} } } } plastic syringes, but it usually only gives us a problem
} } } } during the summer months. During the winter here, the air is
} } } } extremely dry.
} } } }
} } } } We do 4 rinses in absolute alcohol, followed by 3 rinses in
} } } } propylene oxide, followed by a 50/50 mixture of epon/araldite
} } } } mixed with propylene oxide over night with the caps off, for
} } } } the propylene oxide evaporating overnight and slowly leaving
} } } } the specimens in 100% plastic by morning. We polymerize at
} } } } 70 deg C overnight, keeping a dessicant in our embedding oven
} } } } to keep the air as dry as possible too.
} }
} }
} } Sergey Ryazantsev Ph. D.
} } Electron Microscopy
} } UCLA School of Medicine
} } Department of Biological Chemistry
} } 10833 Le Conte Ave, Room 33-080
} } Los Angeles, CA 90095
} }
} } Phone: (310) 825-1144 (office)
} } (310) 206-1029 (Lab)
} } FAX (departmental): (310) 206-5272
} } mailto:sryazant-at-ucla.edu
} }
} }
} }
} }
} }

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 23:30:23 2004

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Dear Colleagues:

I’m working with some extremely fastidious
dinoflagelates, which I can’t seam to keep the
flagella in place. I’m after the flagella attachment
of the Pyrodinium Bahamense. On a separate batch I’m
looking to break the armor to take a look inside. I
have modified the dehydration process in order to see
if that preserve the flagella. I’m also thinking to
change the fixative from Paraformaldehyde to
Glutaraldehyde. Any ideas into how to treat these
organisms will be greatly appreciated.

Omayra Velez
New Jersey

__________________________________________________
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Tired of spam? Yahoo! Mail has the best spam protection around
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From MicroscopyL-request-at-ns.microscopy.com Wed Sep 15 23:34:33 2004

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Dear Colleagues:

I'm sorry for the previous email subject heading. It
didnot make any sense. Originaly, I had an osmium
question, about the dinoflagellates but I found the
answer myself.

Omayra Velez
New Jersey

__________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 08:01:18 2004

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Just to add to you potential choices Ladd offers our L900 8"
Grinder/Polisher.

JD Arnott

Disclaimer: Ladd Research is in the business of supplying your microscopy
needs including the products mentioned in this thread.

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: ladres-at-att.net

----- Original Message -----
} From: {hkonishi-at-indiana.edu}
To: {Microscopy-at-microscopy.com}
Sent: Wednesday, September 15, 2004 3:23 PM

I want to buy a grinder/polisher that works with Gatan 623 Disc Grinder or
SPI
Precision Disc Grinder. Does anyone use "8" Grinder/Polisher" from Electron
Microscopy Sciences with Disc Grinder? Is there any other recommendation? I
would find a grinder around 1-2K.
Thank you,
Hiromi Konishi
Indiana University

Product:
http://www.emsdiasum.com/microscopy/products/materials/polishing.aspx?
mm=9

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: ladres-at-att.net

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 08:12:18 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

It's not hard to measure volumes when you use a syringe.

Mannie Steglich
UT MDACC

Garry Burgess {GBurgess-at-exchange.hsc.mb.ca}

09/15/2004 02:37 PM

To:
{microscopy-at-microscopy.com}
cc:

I've always for the last 20 years used digital balances to measure out
quantities of resin components to mix up plastics, but I'm curious as to
why
the manufacturers always specify the amount in volume measures instead of
weight, since it seems to me that it would be a tough job to clean out
grad
cylinders full of resin components, vs just filling up a plastic beaker on
a
balance, and disposing of it afterwards.

I was just curious as to how others do their measuring, and if they resort
to the horrifying task of cleaning glassware of resin components, which
strikes me as a particularly nasty job.

Garry Burgess

Charge Technologist
Department of Pathology
Health Sciences Centre
Winnipeg, Canada

This e-mail and/or any documents in this transmission is intended for the
address(s) only and may contain legally privileged or confidential
information. Any unauthorized use, disclosure, distribution, copying or
dissemination is strictly prohibited. If you receive this transmission in
error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 08:44:56 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Debby,

I only freeze a small amount and only use the stored frozen aliquots for the
intermediate stages: the mixes with propylene oxide. I always use freshly
mixed resin for embedding.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Debby Sherman [mailto:dsherman-at-purdue.edu]
Sent: Wednesday, September 15, 2004 7:25 PM
To: Garry Burgess; microscopy-at-microscopy.com

Garry

We have used weight measurement for many years. We have a scale in a hood
and use gloves and all disposable containers so dare not too concerned about
the resin components being hazardous. We mix resins as needed rather than
mix large batches and freeze aliquots since it only takes a few minutes to
mix the resins in the quantity we need. This works fine and we get
consistent resin properties in our blocks.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 9/15/04 2:37 PM, "Garry Burgess" {GBurgess-at-exchange.hsc.mb.ca} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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-
}
}
} I've always for the last 20 years used digital balances to measure out
} quantities of resin components to mix up plastics, but I'm curious as to why
} the manufacturers always specify the amount in volume measures instead of
} weight, since it seems to me that it would be a tough job to clean out grad
} cylinders full of resin components, vs just filling up a plastic beaker on a
} balance, and disposing of it afterwards.
}
} I was just curious as to how others do their measuring, and if they resort
} to the horrifying task of cleaning glassware of resin components, which
} strikes me as a particularly nasty job.
}
} Garry Burgess
}
} Charge Technologist
} Department of Pathology
} Health Sciences Centre
} Winnipeg, Canada
}
} This e-mail and/or any documents in this transmission is intended for the
} address(s) only and may contain legally privileged or confidential
} information. Any unauthorized use, disclosure, distribution, copying or
} dissemination is strictly prohibited. If you receive this transmission in
} error, please notify the sender immediately and return the original.
}

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 08:51:56 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Randy, et al,

I prepare my resin exactly the same way, Randy, and have not had any problems.
Have raised a few eyebrows with the sound effects also!
I store small aliquots of resin in scintillation vials in the freezer. I don't
process a high volume of tissue, so for me this method works well. I just thaw
a vial and use a plastic disposable pipet to fill my molds. No fuss, no mess.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Laboratories of Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Tindall, Randy D. [mailto:TindallR-at-missouri.edu]
Sent: Wednesday, September 15, 2004 6:07 PM
To: Garry Burgess
Cc: microscopy-at-microscopy.com

Garry, we measure in volume equivalents, one ml per gram. Although I
recognize that the differing specific gravities of the various
components means that these are not exactly equivalent measures, it
works well for us.

We use 30 ml syringes sans needles to measure the components---pop out
the plunger (and make sure the syringe cap is on!) and fill the body of
the syringe up to the appropriate mark. Reinsert the plunger and push
out the goo into a plastic mixing cup. Repeat for the other components.
Not only is this quick, easy, and about as mess free as working with
resins ever gets, but you get some interesting sound effects that raise
eyebrows on people not in the know. As an added bonus, if you pour the
mixed resin back in the syringes, they make for nice freezer storage and
easy dispensing. When empty, just throw them into an oven until the
remnants are polymerized and toss the used syringes.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

-----Original Message-----
} From: Garry Burgess [mailto:GBurgess-at-exchange.hsc.mb.ca]
Sent: Wednesday, September 15, 2004 2:38 PM
To: microscopy-at-microscopy.com

I've always for the last 20 years used digital balances to measure out
quantities of resin components to mix up plastics, but I'm curious as to
why the manufacturers always specify the amount in volume measures
instead of weight, since it seems to me that it would be a tough job to
clean out grad cylinders full of resin components, vs just filling up a
plastic beaker on a balance, and disposing of it afterwards.

I was just curious as to how others do their measuring, and if they
resort to the horrifying task of cleaning glassware of resin components,
which strikes me as a particularly nasty job.

Garry Burgess

Charge Technologist
Department of Pathology
Health Sciences Centre
Winnipeg, Canada

This e-mail and/or any documents in this transmission is intended for
the address(s) only and may contain legally privileged or confidential
information. Any unauthorized use, disclosure, distribution, copying or
dissemination is strictly prohibited. If you receive this transmission
in error, please notify the sender immediately and return the original.

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 08:54:25 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dinoflagellates are not easy to fix properly. My experience with them has been that each species (especially the lightly armored or unarmored ones)can have their own individual reqirements for fixation. When I have problems with fixation I use what has been called Parducz fixative. It was originally developed in the 1960's for work on cilliates by Bela Parducz to study the metachronal wave pattern of the cillia. It consists of a mixture of Osmium tetroxide and mercuric chloride. To prepare the solution according to Parducz, you make a 6:1(V:V) mixture of 2% aqueous Osmium tetroxide(OsO4) with saturated aqueous mercuric chloride(HgCl2). You can adjust the relative mixtures of the two components as I know that I have used 3:2 and perhaps 1:1. This fixative has been referred to as an "instantaneous fix" as it will fix the specimens very, very, rapidly. Parducz fixative was the only way that I could prepare some dinoflagellates for SEM and retain not only their morphology, but flagella as well. It is not as good a fix for TEM. Here are a couple of references that you may want to see:

Small, E.B. 1968. Scanning electron microscopy of fixed, frozen and dried
} protozoa. Science. 163:1064-1065.
}
} and
}
} Bela Parducz. 1966. Ciliary Movement abd Coordination in Cilliates.
} International Review of Cytology. 21:91-128.

Omayra Velez wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 09:10:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear List:

The July/August issue of PhotoTechniquesUSA has a review of the HP
Photosmart 7960 printer. The reviewer, a professional photographer and
printmaker named Ctein, said "it makes the best (and most permanent)
black and white prints of any computer printer I've ever tried." It is
an 8 ink printer that has 3 photo gray inks in addition to the usual
color inks although it seems that the photo gray ink cartridge is an
extra cost option?
The magazine has a website http://www.phototechmag.com/ but I do
not know if the review is available there.

Geoff

Gary Gaugler wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} I was a fan of Epson photo printers for quite
} some time. Notable was the 890 & 980. It is a
} small format printer compared to the 2200.
} I recently (a year or so ago) bought a Epson Stylus
} Photo 2000. It lasted about six months and
} then jammed constantly. In-warranty customer
} service and any idea of repair was on a wish list.
} It never happened. The printer was scrapped.
}
} The 2200 may have solved teething problems
} with large format printers. However, the 2000
} was VERY slooooow using photo paper. When it
} worked, the results were stunning. Many times
} (too many) it would stop printing 1/4 or 1/2
} way through the print and just die. The job
} hung (Win2K Pro) and had to be restarted with
} a new sheet of paper.
}
} The Epson and Canon small format printers seem
} to do a better, more reliable job. As a result
} of being burned by Epson, I now take print jobs
} to a local service bureau. they do a very nice
} job for not much cost. These are mostly for
} 24" x 48" glossy mounted prints. Small ones
} are done on my HP 4550 color laser printer.
} If the color gamut is matched well between
} the monitor and Photoshop, the HP does a nice job
} for reports. For transparencies (not much used
} any longer), the Kodak dye sub is excellent.
}
} Let us know what you find. There are a lot
} of options. Also, check out the Ethernet print
} servers that will connect a non-network printer
} to a LAN and allow all to use it. HP and others
} make these. they usually cost about $100 or so.
}
} gary g.
}
}
} At 11:08 AM 9/2/2004, you wrote:
}
} } Email: jtd1-at-psu.edu
} } Name: Tom Doman
} }
} } Organization: Penn State University
} }
} } Title-Subject: [Microscopy] [Filtered] MListserver:
} }
} } Question: Our lab is considering various photo printers (} $1K) for
} } production of electron micrographs. Currently the Epson 2200 is the
} } stromg favorite. Are there any recomendations for other printers
} } which we should consider? What are your reasons for the recomended
} } printer?
} }
} } Thanks in advance!
} }
} } Tom
} }
} } ---------------------------------------------------------------------------
} }
}
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 10:44:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Greg, Omayra

i wonder if the following is relevant - narcotize the critters before fixing
them.
see, for example:

May L. (1985) The use of procaine hydrochloride in the preparation
of rotifer samples for counting. Verh.Internat.Verein.Limnol. 22, 2987-2990.

Abstract: Although many rotifer species are easily recognized when
killed and fixed in formalin, some of the soft-bodied forms contract
violently on contact with the chemical and become unrecognizable.
In samples from Loch Leven this situation occurred most commonly with
Synchaeta kitina Rousselet and several possible methods of killing
the species in a relaxed from were considered (May, 1980).
Narcotizing the animals with procaine hydrochloride
(NH2.C6H4.COO.CH2.CH2.N(C2H5)2.HCl) before adding formalin was
found to be the most succesful method. This paper describes the
development of the method and examines its effect on rotifer
density estimates

Chris

----- Original Message -----
} From: "Greg Strout" {gstrout-at-ou.edu}
To: "Omayra Velez" {mayas003-at-yahoo.com}
Cc: {Microscopy-at-MSA.Microscopy.com}
Sent: Thursday, September 16, 2004 3:21 PM

I am looking for a "micrometer" that can work with optical microscope. I think
that it read the difference of dial for focusing and convert to actual
distance (um). I want to use it for determining the thickness of disc during
disc grinding if it is not so expensive.
Please advise on website or product information.
Thank you,

Hiromi Konishi
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 11:06:46 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

List,

I own 2 of these printers and they actually come with all 4 cartridges,
color, photo, black & grey. The unit has a storage compartment for the
cartridge not in use (either the grey or the black). I agree with the
review it does an outstanding job of both color and B&W. When printing
at its highest resolution an 8X10 print can take 11 minutes to print
and will need (temporarly) 400 Mb of hard disk space. When I got mine
the were selling at 300 USD, they are now selling at about 200 USD.

Love 'em
Robert Schoonhoven

Geoff McAuliffe wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Dear List:
}
} The July/August issue of PhotoTechniquesUSA has a review of the HP
} Photosmart 7960 printer. The reviewer, a professional photographer and
} printmaker named Ctein, said "it makes the best (and most permanent)
} black and white prints of any computer printer I've ever tried." It is
} an 8 ink printer that has 3 photo gray inks in addition to the usual
} color inks although it seems that the photo gray ink cartridge is an
} extra cost option?
} The magazine has a website http://www.phototechmag.com/ but I do
} not know if the review is available there.
}
} Geoff
}
} Gary Gaugler wrote:
}
} }
} }
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } I was a fan of Epson photo printers for quite
} } some time. Notable was the 890 & 980. It is a
} } small format printer compared to the 2200.
} } I recently (a year or so ago) bought a Epson Stylus
} } Photo 2000. It lasted about six months and
} } then jammed constantly. In-warranty customer
} } service and any idea of repair was on a wish list.
} } It never happened. The printer was scrapped.
} }
} } The 2200 may have solved teething problems
} } with large format printers. However, the 2000
} } was VERY slooooow using photo paper. When it
} } worked, the results were stunning. Many times
} } (too many) it would stop printing 1/4 or 1/2
} } way through the print and just die. The job
} } hung (Win2K Pro) and had to be restarted with
} } a new sheet of paper.
} }
} } The Epson and Canon small format printers seem
} } to do a better, more reliable job. As a result
} } of being burned by Epson, I now take print jobs
} } to a local service bureau. they do a very nice
} } job for not much cost. These are mostly for
} } 24" x 48" glossy mounted prints. Small ones
} } are done on my HP 4550 color laser printer.
} } If the color gamut is matched well between
} } the monitor and Photoshop, the HP does a nice job
} } for reports. For transparencies (not much used
} } any longer), the Kodak dye sub is excellent.
} }
} } Let us know what you find. There are a lot
} } of options. Also, check out the Ethernet print
} } servers that will connect a non-network printer
} } to a LAN and allow all to use it. HP and others
} } make these. they usually cost about $100 or so.
} }
} } gary g.
} }
} }
} } At 11:08 AM 9/2/2004, you wrote:
} }
} } } Email: jtd1-at-psu.edu
} } } Name: Tom Doman
} } }
} } } Organization: Penn State University
} } }
} } } Title-Subject: [Microscopy] [Filtered] MListserver:
} } }
} } } Question: Our lab is considering various photo printers (} $1K) for
} } } production of electron micrographs. Currently the Epson 2200 is the
} } } stromg favorite. Are there any recomendations for other printers
} } } which we should consider? What are your reasons for the recomended
} } } printer?
} } }
} } } Thanks in advance!
} } }
} } } Tom
} } }
} } } ---------------------------------------------------------------------------
} } }
} }
} }
} }
} }
}

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 11:05:30 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

If a rotating platen is used with a hand grinder, the flat surface of the hand grinder is usually rounded off and can become facetted. However, you can use a polishing station, just don't turn it on; keep it stationary. I have used the South Bay Technology Lapping tray with all of the common hand grinders, South Bay's, Fischione's, and Gatan's. This is my preferred way of thinning TEM samples down to 100 um or less. I have also used the Gatan lapping tray. I found this one too small and I don't like using the PSA backing on the disks (besides the high costs of the disks). With the lapping tray, I use 8" SiC disks without the PSA backing and hold them down by hand. They don't last long enough to go through the hassle of pasting them down. In addition, the lapping tray works very well with the 3M diamond films and they can last a very long time depending on your material. For III-V compounds, I have used a single 30 um disk for months. These work well, because the water used
for lubrication can be kept on the pad because they are hydrophobic. (Careful, not all diamond films are the same and other brands are not hydrophobic and have this property.) They stay put when water is used to hold them down. As in the Tripod(TM) polishing technique, you hold them down by putting a puddle of water on the plate and then carefully put the pad down moving it around so that no air bubbles get under the pad and then squeegee the water out. It will stay put like that for over 1/2 hr if you do not let any water get under it.

A word about the glass used in the lapping tray, since I work at the Glass Technology Center. Glass has two sides, the air side and the tin side. The tin side is the smoothest and is less sensitive to corrosion. You can tell the Sn side because it will fluoresce under UV. If you can determine it, this is the side that you should put your 3M papers on. You do not want water with any of the ground material to dry on the glass. If there are any silicates present, they will bond with the glass when it dries and you will not be able to remove it. I always use distilled water with the lapping trays, but that may not always be possible.

Another word of caution, don't drop your hand grinder on the glass plate! Not everyone can replace it as easily as I did.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Mary Mager [mailto:mager-at-interchange.ubc.ca]
Sent: Wednesday, September 15, 2004 6:23 PM
To: hkonishi-at-indiana.edu
Cc: Microscopy

Dear Hiromi,
Because the amount of material removed from 3.05 mm TEM discs with the Gatan
Disc Grinder is very small, I use 600 grit paper stuck to a glass sheet and
carefully hand grind the samples under running water, then finish off with
1200 grit the same way. It only takes a few strokes to remove 50 microns,
then advance the dial and remove another 50 microns. We have spinning wheel
grinders and automatic polishers, but I would not use them for this.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {hkonishi-at-indiana.edu}
To: {Microscopy-at-microscopy.com}
Sent: Wednesday, September 15, 2004 12:23 PM

Members,
In my opinion, the HP 7960 is a great photo printer. It has it all -
dedicated gray level ink cartridge, tiny ink droplet size, low cost ( { $200
at the typical warehouse club stores) and has all of the various memory card
slots on the front panel for your digital camera along with a color LCD
display for previewing the images. Even on standard copy paper, the images
really come out nice.

Disclaimer:
I do not work for HP nor have any financial interest in said company. I
do however, bundle this printer (at the end user's request) with the SEM
Digital Image Capture Systems that I do sell.

Gary M. Easton
Scanners Corporation
Third Party SEM Service/Digital Imaging/EDS Sales
410-857-7633 x102

----- Original Message -----
} From: "Geoff McAuliffe" {mcauliff-at-umdnj.edu}
To: "Gary Gaugler" {gary-at-gaugler.com}
Cc: "by way of MicroscopyListserver" {jtd1-at-psu.edu} ; "MSA listserver"
{Microscopy-at-MSA.Microscopy.Com}
Sent: Thursday, September 16, 2004 1:33 PM

Recently I acquired an HP 6540 printer, not a photo printer as such (no built in card reader or LCD screen), but I have been extremely impressed with its quality and speed in printing my SEM images (formerly used an HP 970). It is very quick - prints two 4x5" photos on one sheet of HP Premium inkjet paper in 30 seconds (standard print quality setting). I compared the output quality with printing at the top quality setting and found little if any visible improvement for the doubling in output time.

It also takes gray or photo color cartridges in place of the black one. I have not been impressed with either of these, the colors seem weak and don't match the ones on my monitor, which are gray scale. So for all that I'm sticking with the standard black and color cartridges for the best results here.

I had been looking at the HP 7960, but purchasing wrinkles pointed me to the 6540 and I'm happy they did. Was a bit cheaper too ($150).

Richard Shalvoy
Arch Chemicals, Inc.
350 Knotter Drive
Cheshire, CT 06410
(203) 271-4394
rbshalvoy-at-archchemicals.com

-----Original Message-----
} From: rschoon [mailto:rschoon-at-email.unc.edu]
Sent: Thursday, September 16, 2004 12:32 PM
To: Geoff McAuliffe
Cc: Gary Gaugler; by way of MicroscopyListserver; MSA listserver

Hi Omayra,
We have used Parducz since 1967 and it works wonders on bacteria,
protozoa, and many other critters especially those with flagella and
cilia. Two things that we have found important in its use are:
1. Make it FRESH just before use
We keep a saturated solution of HgCl2 around in a brown 50 ml bottle
which has been as old as one year. To make it we put a bit of HgCl2 into
distilled water until we see that it is saturated i.e. with a ppt on the
bottom. We also keep a bottle of 2% aq OsO4 in the refrigerator (usually
double jarred to prevent vapors from escaping).
JUST before use then we mix 6 ml of 2% OsO4 and 1 ml of the saturated
HgCl2 (taken from the top of the bottle). We then fix whatever we are
fixing for an hour or so. Obviously if more fix is needed, larger
amounts can be made.
2. Wash WELL after the Parducz fixation. Otherwise you get starfish
shaped crystals on the surface of your prep. They may look neat but
obviously are not part of the specimen.
Other than that, it is a great hardening fix for SEM.

Good Luck,
Judy Murphy
Stockton, CA

Omayra Velez wrote:

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 13:30:40 2004

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Greetings Hiromi,
A good solution would be a linear encoder for upright microscopes with a
digital readout. We use a unit from Hiedenhain
(www.heidenhain.com/product.html) on our stereology rig. There may be a
way to set one up for inverted bases as well. Digital length gauge
systems or linear encoders can measure z position with very high
precision. You may wish to contact the folks at MicroBrightfield
(www.microbrightfield.com) as they sell such solutions specifically for
microscopes.
Simply calibrating the markings on focus knobs to displacement of
the stage in z may not be very precise in some instances. Older
axiovert bases have a friction based focusing system which can slip
depending on the speed or distance through which the knob is turned.
Other bases may have similar issues with the focus mechanism.
Calibration strategies in which the top and bottom of a z calibration
standard are imaged to determine endpoints will have to take into
account the uncertainty due to depth of focus of a particular objective
lens as well. The linear encoder avoids this uncertaintly.
Regards,
Karl

hkonishi-at-indiana.edu wrote:

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--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 14:08:21 2004

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We just purchased a Canon i9900. The initial test prints are beautiful. It
uses eight cartridges and when using Canon's Pro Paper, you would not know
that they are computer prints rather than high quality true photographs. We
elected to have a larger format capacity (13" x 19") as we like to decorate
our lab and office walls with our favorites.

Al Stone
ASTON Metallurgical Services

At 01:02 PM 9/16/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 16:20:53 2004

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Dear All EM Specialists:

I really enjoy being on this forum and am educated a lot. Now I have a question about how often we need to flash our field emission SEM's tip.

We have a brand new Hitachi 4700 which has a cold field emission tip. When it was first installed, the service engineer told us to record the initial extraction voltage each time right after flashing, during the use if the increase of extraction voltage is more than 1.4 KV, we need to do a flash. We follow this rule strictly. Several weeks ago Hitachi's application engineer visited us and said by doing that we flashed too much and would short our tip's lifetime. We do not need to flash until we see the tip noise. I never see any tip noise in my image by following his suggestion so I am forced to flash by the instrument setting (every 48 hours).

Could you please kindly share your experience with me?

Thanks

Ying Shi

Analytic Scientist
Delphi Catalyst
ying.shi-at-delphi.com

****************************************************************************************

Note: The information contained in this message may be privileged and confidential and thus protected from disclosure. If the reader of this message is not the intended recipient, or an employee or agent responsible for delivering this message to the intended recipient, you are hereby notified that any dissemination, distribution or copying of this communication is strictly prohibited. If you have received this communication in error, please notify us immediately by replying to the message and deleting it from your computer. Thank you.

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 16:28:53 2004

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Hello All,

I have a BioScan Ted Pella microwave with a cold-spot and vacuum chamber
that I would like to use for fixation and embedding insect eggs and larvae
for TEM.

The project includes mosquito larvae, pupae and fly eggs. I worked on this
same project many years ago using traditional benchtop methods. The eggs
and larvae were difficult, if not impossible, to infiltrate. Now that I
have a MW with vacuum I am trying this project again.

I would greatly appreciate any suggestions, advice or direct me to references?

My first attempt at MW didn't go so well.
I MW fixed the larvae with 2% glut in cacodylate in 1.5ml centrifuge tubes
at 20mmHg vacuum -at- 250W 1' on, 1' off. Repeated several times removing the
vacuum to observe the larvae. At first when vacuum was applied the larvae
floated to the top and squirmed around a bit, then after several attempts
at that they finally all stopped moving and didn't float. Buffer washed on
benchtop then used the vacuum again at the same settings for the buffered
osmium tetroxide. Just the ends of the larvae turned black. I tried it
again without any change. I finally got tired of messing with them and
placed them into a KFeCN + OsO4 overnight at 4C and have had them stored in
buffer. ( I have used the overnight KFeCN + OsO4 with success for hard to
infiltrate nematodes). Dehydrated with MW 40s -at- 250W no vacuum 40 s on, 1'
off, infiltrated 50% acetone/Embed no vac at 250W 3', 100% Embed -at- 450W
with vac (20mm Hg). The larvae had areas of collapse after the 100% with
vacuum so I'm concerned that they are not infiltrating as I had hoped.

Karen L. Kelley
ICBR Electron Microscopy Manager
University of Florida
ICBR Electron Microscopy Core Lab
Bartram Hall Room 214
Box 118525 Gainesville Florida
Lab: 352-392-1184 fax: 352-846-0251
Email: klk-at-biotech.ufl.edu
Southeastern Microscopy Society Treasurer
http://www.biotech.ufl.edu/EM/

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 17:18:35 2004

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Dear colleague,
I remember some discussion about CD-R storage. Some CD are not good at all
and in many cases some CD become unreadable after 3 years.
I would like to know what is the best brand or type of CD for storing
images

Keep care and be of good cheer

Regards

(name) Vratislav Richard Eugene Maria John Baptist
(surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

Tenebrionidae of the World, incl. Alleculinae and Lagriinae,
higher taxonomy, Australian beetles.
websites:
http://www.coleoptera.org. and
http://www.egroups.com/group/coleoptera

University of Sydney
The Wentworth Bldg., B 62
NSW 2006
AUSTRALIA
phone : +61 414 540 465
email: ricardo-at-ans.com.au
vratislav-at-bigfoot.com
ICQ: 13610107

Only after the last tree has been cut down,
only after the last river has been poisoned,
only after the last fish has been caught,
only then will you find that money can not be eaten.'
CREE INDIAN PROPHECY.

Incoming mail is certified Virus Free.
Checked by AVG anti-virus system (http://www.grisoft.com).

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 17:23:42 2004

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We have been using a digital length gauge from Heidenhain. the readout
unit has an RS-232 port so that we can record depth with a computer.
It uses an optical encoder that has been clamped in a holder so that it
can be placed below the stage.

Our cost was about $1500, but that was about 1993.

Regards,
Glen
On Sep 16, 2004, at 9:11 AM, hkonishi-at-indiana.edu wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} I am looking for a "micrometer" that can work with optical microscope.
} I think
} that it read the difference of dial for focusing and convert to actual
} distance (um). I want to use it for determining the thickness of disc
} during
} disc grinding if it is not so expensive.
} Please advise on website or product information.
} Thank you,
}
} Hiromi Konishi
} Indiana University
}
}
}
Glen MacDonald
Core for Communication Research
Virginia Merrill Bloedel Hearing Research Center
Box 357923
University of Washington
Seattle, WA 98195-7923 USA
(206) 616-4156
glenmac-at-u.washington.edu

************************************************************************
******
The box said "Requires Windows 95 or better", so I bought a Macintosh.
************************************************************************
******

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 17:32:22 2004

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Can you make an estimate how much a high quality print, letter size in full
color and b/w costs (probably just ink and paper)?

I'd be interested also for the HP that was mentioned in the original post.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Alan Stone [mailto:as-at-astonmet.com]
Sent: Thursday, September 16, 2004 13:36
To: microscopy-at-microscopy.com

We just purchased a Canon i9900. The initial test prints are beautiful. It
uses eight cartridges and when using Canon's Pro Paper, you would not know
that they are computer prints rather than high quality true photographs. We
elected to have a larger format capacity (13" x 19") as we like to decorate
our lab and office walls with our favorites.

Al Stone
ASTON Metallurgical Services

At 01:02 PM 9/16/2004, you wrote:

} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 18:53:41 2004

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IMO, Mitsui is the absolute best for CD-R or
DVD-R:

http://www.mitsuicdr.com/

gary g.

At 03:46 PM 9/16/2004, you wrote:

} Dear colleague,
} I remember some discussion about CD-R storage. Some CD are not good at all
} and in many cases some CD become unreadable after 3 years.
} I would like to know what is the best brand or type of CD for storing
} images
}
} Keep care and be of good cheer
}
} Regards
}
} (name) Vratislav Richard Eugene Maria John Baptist
} (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 20:26:25 2004

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(9/17/04 8:46) Vr.R.E.M.J..-B. BEJSAK-COLLOREDO-MANSFELD {ricardo-at-ans.com.au} wrote:

} Dear colleague,
} I remember some discussion about CD-R storage. Some CD are not good at all
} and in many cases some CD become unreadable after 3 years.
} I would like to know what is the best brand or type of CD for storing
} images
}
} Keep care and be of good cheer
}
} Regards
}
} (name) Vratislav Richard Eugene Maria John Baptist
} (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

I would recommend Mitsui. Remember, the ideal conditions for storage of CDs is very similar to negatives: cool, dark, and dry.

It is essential to remember that a CDR is -absolutely not- an archival copy of your data.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 16 22:43:50 2004

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One thing of note....

DO NOT use sharpie markers or any other acid base pen to label cd's or
dvd's. The acid in these pens etches through the top of the disk destroying
your data.

Dave Crone B.E. (Mechanical)
Engineer-in-Training
Department Assistant
Metallurgical Lab
Mechanical Engineering
College of Engineering
University of Saskatchewan
57 Campus Drive
Saskatoon, SK
S7N 5A9
Phone: (306) 966-5461
Fax: (306) 966-5427
E-mail: dgc132-at-mail.usask.ca
-----Original Message-----
} From: Brent Neal [mailto:brent-at-reindeergraphics.com]
Sent: Thursday, September 16, 2004 7:54 PM
To: Vr.R.E.M.J..-B. BEJSAK-COLLOREDO-MANSFELD
Cc: MICROSCOPY

(9/17/04 8:46) Vr.R.E.M.J..-B. BEJSAK-COLLOREDO-MANSFELD
{ricardo-at-ans.com.au} wrote:

} Dear colleague,
} I remember some discussion about CD-R storage. Some CD are not good at all
} and in many cases some CD become unreadable after 3 years.
} I would like to know what is the best brand or type of CD for storing
} images
}
} Keep care and be of good cheer
}
} Regards
}
} (name) Vratislav Richard Eugene Maria John Baptist
} (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

I would recommend Mitsui. Remember, the ideal conditions for storage of CDs
is very similar to negatives: cool, dark, and dry.

It is essential to remember that a CDR is -absolutely not- an archival copy
of your data.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 01:24:07 2004

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Hi all

We use on an old OPL inverted microscope (~1950) a Mitutoyo digital
workshop micrometer (Digimat IDF 543 serie, ref 543-511) witch gives 1
micron as last digit. It's easy to put in on inverted microscope, a bit
more complicate for a upright one. Very useful and reliable enough for all
samples thinning job for TEM (before tripod polishing or dimpler
thinning). I don't remember the price, we bought it 6-7 years ago, but
it's ŕ workshop stuf, not a laboratory one. So it should not be much
expensive. Some models can be interface to record measurements.

No interest in that manufacturer, just satisfied from that product.

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

On Thu, 16 Sep 2004 hkonishi-at-indiana.edu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I am looking for a "micrometer" that can work with optical microscope. I think
} that it read the difference of dial for focusing and convert to actual
} distance (um). I want to use it for determining the thickness of disc during
} disc grinding if it is not so expensive.
} Please advise on website or product information.
} Thank you,
}
} Hiromi Konishi
} Indiana University
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 06:30:11 2004

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For archival quality:
you should always finalise the disk and don't bother with multisession, consider copying at a slower than maximum speed for the drive and disk. Run the disk check software and maybe check some images on the CD (or just the disk directory) because problems may happen at the copying stage. I have used those special CD markers (I know TDK make some) for about two to three years without problem.

Make 2 (or 3) copies instead of one and store separately and check one periodically - at least if one fails you have a reasonable chance that the other(s) may survive.

Make sure that you will be able to read them in the next few years - with the advance of technologies such as 'Blu-ray' DVD writers how long will CD compatibility be maintained? You only have to look at 8, 5 1/4, & 3 inch floppies and some of the older magneto optical formats to realize that the format may have a shorter useful lifetime than its archival quality.

Malcolm

PS I don't always practice what I preach.

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Dave Crone {dgc132-at-mail.usask.ca}

So what should be used to archive electronic data?

Richard Doelle
Dofasco Inc.
richard_doelle-at-dofasco.ca

-----Original Message-----
} From: Brent Neal [mailto:brent-at-reindeergraphics.com]
Sent: Thursday, September 16, 2004 9:54 PM
To: Vr.R.E.M.J..-B. BEJSAK-COLLOREDO-MANSFELD
Cc: MICROSCOPY

HI Garry,
I too, mix by weight but I have a friend who uses disposable syringes
to measure by volume. No cleaning, since she uses each syringe once
and discards it (adding to the trash load...we just can't win).
She sets up her resin component bottles with stoppers and tubing that
she can seal off when not measuring and which she can just hook up to
the syringes and then draw out the volume she needs. I know that she
got this method from her first employer and that between them the
method has worked beautifully for 30 years or more.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 08:02:17 2004

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At 4:47 PM -0500 9/16/04, Ying.Shi wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Ying Shi,

We have had a Hitachi S4700 since 10/1996. We typically only flash
the tip only once in the morning each day. If I remember correctly,
the instrument was originally programmed to make you flash about
every eight hours. We had the service engineer change the required
flash time to 16 hours. This allows us to have a stable beam current
for XEDS line scans and maps in the afternoon. We record the current
at each flash, when this gets above a certain level it indicates to
the service engineer that the column needs to be baked, typically
twice a year. We are still using our original tip!! Good luck with
your S4700.

--
David R. Hull
NASA Glenn Research Center at Lewis Field
Advanced Metallics Branch
Mail Stop 49-1
21000 Brookpark Road
Cleveland, OH 44135

(216) 433-3281
fax (216)977- 7132
david.r.hull-at-nasa.gov
http://www.lerc.nasa.gov/WWW/AdvMet/ASGWEB2000/asghome.html

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 08:02:08 2004

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Ying;

I think you would be safe in doing as the applications engineer tells
you, i.e. every 48 hrs. Of course, if you have samples that outgas,
this may need to be more frequent. If the emission current is stable,
and the extraction voltage is stable, just let it run.

We have 2 4700's and a 4500 here at Agere, Allentown, PA.

Hope that is of some help.

Peter Tomic
Agere System

-----Original Message-----
} From: Ying.Shi [mailto:Ying.Shi-at-delphi.com]
Sent: Thursday, September 16, 2004 5:48 PM
To: Microscopy-at-MSA.Microscopy.com

Dear All EM Specialists:

I really enjoy being on this forum and am educated a lot. Now I have a
question about how often we need to flash our field emission SEM's tip.

We have a brand new Hitachi 4700 which has a cold field emission tip.
When it was first installed, the service engineer told us to record the
initial extraction voltage each time right after flashing, during the
use if the increase of extraction voltage is more than 1.4 KV, we need
to do a flash. We follow this rule strictly. Several weeks ago Hitachi's
application engineer visited us and said by doing that we flashed too
much and would short our tip's lifetime. We do not need to flash until
we see the tip noise. I never see any tip noise in my image by following
his suggestion so I am forced to flash by the instrument setting (every
48 hours).

Could you please kindly share your experience with me?

Thanks

Ying Shi

Analytic Scientist
Delphi Catalyst
ying.shi-at-delphi.com

************************************************************************
****************

Note: The information contained in this message may be privileged and
confidential and thus protected from disclosure. If the reader of this
message is not the intended recipient, or an employee or agent
responsible for delivering this message to the intended recipient, you
are hereby notified that any dissemination, distribution or copying of
this communication is strictly prohibited. If you have received this
communication in error, please notify us immediately by replying to the
message and deleting it from your computer. Thank you.

************************************************************************
****************

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 08:10:25 2004

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Ying,

We have a Hitachi S4700, too, and were told by our service engineer to
flash about 1.3 KV above the starting extraction voltage. We have had
the same tip since installation in 1999 and since then the starting
extraction voltage (i.e., right after flashing) has increased from 4.1
to 4.3 KV at 5.0 KV accelerating voltage at 10ua beam current.

My impression from this is that the tip is relatively robust and
long-lasting, even under frequent flashing. This included one period of
VERY frequent flashing due to a bad connection to the gun which
prevented flashing from occurring at the proper strength. When this was
discovered and repaired, the first flash was so powerful it gave us a
reading of 72, rather the recommended 20, before we dialed down the
flash intensity! We were afraid that we'd taken the end right off the
tip with this one, but there was no apparent harm and resolution has
remained fine since then.

Whether or not this is better than flashing only when the software tells
you to is unclear to me, but this is how we were told to do it.

Hope this helps.

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

-----Original Message-----
} From: Ying.Shi [mailto:Ying.Shi-at-delphi.com]
Sent: Thursday, September 16, 2004 4:48 PM
To: Microscopy-at-MSA.Microscopy.com

Dear All EM Specialists:

I really enjoy being on this forum and am educated a lot. Now I have a
question about how often we need to flash our field emission SEM's tip.

We have a brand new Hitachi 4700 which has a cold field emission tip.
When it was first installed, the service engineer told us to record the
initial extraction voltage each time right after flashing, during the
use if the increase of extraction voltage is more than 1.4 KV, we need
to do a flash. We follow this rule strictly. Several weeks ago Hitachi's
application engineer visited us and said by doing that we flashed too
much and would short our tip's lifetime. We do not need to flash until
we see the tip noise. I never see any tip noise in my image by following
his suggestion so I am forced to flash by the instrument setting (every
48 hours).

Could you please kindly share your experience with me?

Thanks

Ying Shi

Analytic Scientist
Delphi Catalyst
ying.shi-at-delphi.com

************************************************************************
****************

Note: The information contained in this message may be privileged and
confidential and thus protected from disclosure. If the reader of this
message is not the intended recipient, or an employee or agent
responsible for delivering this message to the intended recipient, you
are hereby notified that any dissemination, distribution or copying of
this communication is strictly prohibited. If you have received this
communication in error, please notify us immediately by replying to the
message and deleting it from your computer. Thank you.

************************************************************************
****************

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 08:11:19 2004

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Ying,

We have a Hitachi S-900 field-emission SEM, and I agree with the 2nd
engineer's comment. Flash when you see noise, not by hours or
extraction voltage. If the extraction voltage gets excessive, then
I'd consider flashing, but "excessive" depends on your instrument and
operating variables. 1.4kV may not be "excessive". For us it would be
-- but we rarely seen that much increase in extraction V.

Phil

} Dear All EM Specialists:
}
} I really enjoy being on this forum and am educated a lot. Now I have
} a question about how often we need to flash our field emission SEM's
} tip.
}
} We have a brand new Hitachi 4700 which has a cold field emission
} tip. When it was first installed, the service engineer told us to
} record the initial extraction voltage each time right after
} flashing, during the use if the increase of extraction voltage is
} more than 1.4 KV, we need to do a flash. We follow this rule
} strictly. Several weeks ago Hitachi's application engineer visited
} us and said by doing that we flashed too much and would short our
} tip's lifetime. We do not need to flash until we see the tip noise.
} I never see any tip noise in my image by following his suggestion so
} I am forced to flash by the instrument setting (every 48 hours).
}
} Could you please kindly share your experience with me?
}
} Thanks
}
} Ying Shi
}
} Analytic Scientist
} Delphi Catalyst
} ying.shi-at-delphi.com
}
}
} ****************************************************************************************
}
} Note: The information contained in this message may be privileged
} and confidential and thus protected from disclosure. If the reader
} of this message is not the intended recipient, or an employee or
} agent responsible for delivering this message to the intended
} recipient, you are hereby notified that any dissemination,
} distribution or copying of this communication is strictly
} prohibited. If you have received this communication in error, please
} notify us immediately by replying to the message and deleting it
} from your computer. Thank you.
}
} ****************************************************************************************

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 08:33:55 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bgorman-at-unt.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, September 16, 2004 at 09:59:31
---------------------------------------------------------------------------

Email: bgorman-at-unt.edu
Name: Brian Gorman

Organization: University of North Texas

Title-Subject: [Microscopy] [Filtered] H-9000 Gun Housing

Question: Dear Listers,

We are dismantling our H-9000 TEM, and have a brand new (never installed) gun housing with retro fit kit available to anyone interested. Please contact me for more details.

If anyone wants other parts of this microsope, please contact me as well.

Regards,
Brian

Brian P. Gorman, PhD
Assistant Professor
Dept. of Materials Science and Engineering
University of North Texas
Denton, TX 76203
bgorman-at-unt.edu
ph: 940-891-6778
fax: 940-565-4824

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 09:10:17 2004

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richard_doelle-at-dofasco.ca wrote:

}
} So what should be used to archive electronic data?
}

I recommend a stylus and clay tablets. Stored under
proper conditions, these have been shown to last
several thousand years.

Rick Mott

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 10:34:55 2004

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Depending on your definition of archival, Mitsui DVD-R
media ought to work for you. Their media is rated at
75 year retention. Their Gold Archival CD-R is rated
at 100 years. Obviously, don't expect these results
if you leave them on the rear deck of your car for
twenty years.

I believe that this topic has been discussed before
and archived. If not, it will get archived now.

My belief and strategy is to have four, redundant backups.
The first backup is either dual CD-R or dual DVD-R.
Second backup is dual hard drives. These are typically
120GB IDE/ATAPI. Third backups are two SNAP/NAS
servers, 340GB-1TB. Fourth backup are two identical
Ultrium 1 or Ultrium 2 LTO tapes.

The hard drives are in removeable bays and are real time
storage and retrieval media. The SNAP/NAS servers are
about the same but are slower due to LAN speed. Once a
directory of data on a drive will fill a CD or DVD, it is written to
the optical media. At this point, the last backup is to
the optical media. The first backup is to hard drive, then
to NAS, then to LTO and finally, optical.

The LTO 1 media will hold 100GB of un-compressed data.
The LTO 2 holds 200GB. Since the image data is either
TIFF or JPEG, it does not really compress much more
at all. LTO is backward compatable to LTO 1. The drives
are wide SCSI and work with most all operating systems.
NovaStore and Veritas make backup software for these
drives.

A most important aspect of backing up is to actually do it.

gary g.

At 06:05 AM 9/17/2004, you wrote:

} So what should be used to archive electronic data?
}
} Richard Doelle
} Dofasco Inc.
} richard_doelle-at-dofasco.ca
}
}
} -----Original Message-----
} } From: Brent Neal [mailto:brent-at-reindeergraphics.com]
} Sent: Thursday, September 16, 2004 9:54 PM
} To: Vr.R.E.M.J..-B. BEJSAK-COLLOREDO-MANSFELD
} Cc: MICROSCOPY
} Subject: [Microscopy] Re: Brand / type of CD-R disk for sImages
}
}
}
}
} I would recommend Mitsui. Remember, the ideal conditions for storage of
} CDs is very similar to negatives: cool, dark, and dry.
}
} It is essential to remember that a CDR is -absolutely not- an archival
} copy of your data.
}
} Brent
}
} --
} Brent Neal, Ph.D.
} Reindeer Graphics, Inc.
} brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 10:42:03 2004

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I'm really not sure that I should say this, but for some serious archiving
requirements, one could always convert the digital files to film.

Damian

So what should be used to archive electronic data?

Richard Doelle
Dofasco Inc.
richard_doelle-at-dofasco.ca

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 12:03:50 2004

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For all you aficionados of classic, operating ultramicrotomes---this is
your chance! We are disposing of four LKB Ultratome III's (control and
main units), which, when last assembled, comprised three operating units
plus one for spare parts. Included are numerous separate spare parts,
including chucks, belts, fuses, etc., etc., etc.

We also have a operating Pyramitome 11800 and an LKB Historange 2218
Microtome.

The catch: whoever gets these units is responsible for supplying packing
materials and shipping costs. The machines themselves are free.

We had been using this equipment for all of our ultramicrotomy until the
last couple years and had planned to keep using them as teaching units,
but we are desperately short on space. We hope we can find a good home
for them out there in EM land, because our alternative is surplusing
them with our beat up filing cabinets and broken computer monitors.

Any takers?

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 12:30:56 2004

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On Sep 16, 2004, at 3:46 PM, Vr.R.E.M.J..-B. BEJSAK-COLLOREDO-MANSFELD
wrote:

} I remember some discussion about CD-R storage. Some CD are not good at
} all
} and in many cases some CD become unreadable after 3 years.
} I would like to know what is the best brand or type of CD for storing
} images
}
} Keep care and be of good cheer
}
Dear Vratislav,
We are using Imation disks. Since the cost is small, we get the best
combination of brand name and price. If someone like Computer Shopper
has done a test for the reliability of various brands of CD-R or DVD-R
disks, I'd be interested in the results.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 14:25:05 2004

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Agree on this interest point. I've bought brand-name CD-R that show a rating of "48X Multispeed" and found that my recorder (rated up to 24X) can only record at 4X on these CDs. Curiously, other CD-R from the same manufacturer with nominally the same rating and price can go at the full 24X of my recorder. I asked the fellow at our local computer shop and he gave me the blank stare of ignorance followed by a shoulder shrug.

If anyone can explain how I can determine which CD-R will record "fast" (and as Vratislav suggests, will also have a long life) I'm all ears. I suppose speed ratings on CDs are like mileage ratings on cars - your results may vary from the sticker...

Bill
William A. Heeschen, Ph.D.
Microscopy, Digital Imaging
The Dow Chemical Company
Midland, MI 48674
waheeschen-at-dow.com

-----Original Message-----
} From: Bill Tivol [mailto:tivol-at-caltech.edu]
Sent: Friday, September 17, 2004 2:07 PM
To: microscopy-at-msa.microscopy.com

Wow, there's a big demand for Ultratome III's out there. I think I have
enough takers for now, so early next week I'll sort through the replies
and see what I can do, starting with the first ones.

Correction: The Historange microtome is not included, after all. I
almost gave away my boss's machine by mistake....

Thanks for responding.

Randy

-----Original Message-----
} From: Tindall, Randy D. [mailto:TindallR-at-missouri.edu]
Sent: Friday, September 17, 2004 1:31 PM
To: microscopy-at-microscopy.com
Cc: Katz, Martin

For all you aficionados of classic, operating ultramicrotomes---this is
your chance! We are disposing of four LKB Ultratome III's (control and
main units), which, when last assembled, comprised three operating units
plus one for spare parts. Included are numerous separate spare parts,
including chucks, belts, fuses, etc., etc., etc.

We also have a operating Pyramitome 11800 and an LKB Historange 2218
Microtome.

The catch: whoever gets these units is responsible for supplying packing
materials and shipping costs. The machines themselves are free.

We had been using this equipment for all of our ultramicrotomy until the
last couple years and had planned to keep using them as teaching units,
but we are desperately short on space. We hope we can find a good home
for them out there in EM land, because our alternative is surplusing
them with our beat up filing cabinets and broken computer monitors.

Any takers?

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 17:39:54 2004

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I don't think the terms "Archival" and CD-R/DVD-R technologies are
compatible and should not be used in the same sentence unless associated
with the phrase "do not count on".

Yes, manufacturers will offer ratings of 75 or 100 years.

If the media is not exposed to _ANY_ variations in temperature,
humidity, etc. and never handled, I expect you could see that life. I
know of very few places on earth that meet those requirements.

There are a number of potential things that will render the media
unusable. This includes not only the recordable, but also the
"pre-recorded" or "permanent" versions.

The permanent versions especially are susceptible to the aluminum layer
(the LABEL side) oxidizing, and then falling apart.

As the disks go through thermal cycling, there can also be problems with
de-lamination.

Scratches on the "bottom" side of the media are relatively harmless.
Some media is VERY susceptible to scratching and damage on the top or
label side. In addition to avoiding the acidic "Sharpies", avoid
pencils, ball point pens, etc. I would also caution against trying to
"undo" any pressure sensitive label.

DVD-R may prove to be more stable then their CD-R counterparts. I would
still be cautious. Many of the vulnerabilities of CDs (permanent and
recordable) were not realized until recently. There may be unknown
vulnerabilities to DVD-Rs that we don't know about yet either.

Probably the most reliable "archive" media is still magnetic tape. I
have know people that have taken a tape from a "fireproof" safe, where
the tape cartridge was melted beyond use (due to longer than rated
exposure), and even appeared "melted into" the tape. The tape was sent
out to a recovery specialist and 90% plus of the data was recovered.
The stuff takes a beating and keeps on winding.

John W. Raffensperger, Jr.
IT Manager
Apache Stainless

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 17:55:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwadgaobkar-at-mail.mcg.edu) from http://www.msa.microscopy.org/Ask-A-Microscopist/Ask-A-Microscopist.html on Friday, September 17, 2004 at 13:15:12
---------------------------------------------------------------------------

Email: bwadgaobkar-at-mail.mcg.edu
Name: Bakul wadgaonkar

Organization: Medical College of Georgia

Education: Graduate College

Location: Augusta, GA

Question: We are studying a polymer (poly e-caprolactone)thats semicrystelline. We were wondering how to stain just the crystelline lamella to eatimate the crystillinity and study the morphology.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 19:45:34 2004

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I concur with what all that was said. But still cd's are cheap, 25 cents a
piece here, and at 40x or faster you are looking at 5 to 6 min burn. A
non-acidic marker is $2, so backup your data and if you are unsure back it
up again in 6 months. If it is dvd-r they are $0.46 and you can fit 4.2 GB
on them, so back up often! If you have problems with data backup feel free
to contact me I will help you out as much as I can.

Dave Crone B.E. (Mechanical)
Engineer-in-Training
Department Assistant
Metallurgical Lab
Mechanical Engineering
College of Engineering
University of Saskatchewan
57 Campus Drive
Saskatoon, SK
S7N 5A9
Phone: (306) 966-5461
Fax: (306) 966-5427
E-mail: dgc132-at-mail.usask.ca
-----Original Message-----
} From: Chiphead [mailto:chiphead-at-sbcglobal.net]
Sent: Friday, September 17, 2004 5:07 PM
To: 'Microscopy MSA'

I don't think the terms "Archival" and CD-R/DVD-R technologies are
compatible and should not be used in the same sentence unless associated
with the phrase "do not count on".

Yes, manufacturers will offer ratings of 75 or 100 years.

If the media is not exposed to _ANY_ variations in temperature,
humidity, etc. and never handled, I expect you could see that life. I
know of very few places on earth that meet those requirements.

There are a number of potential things that will render the media
unusable. This includes not only the recordable, but also the
"pre-recorded" or "permanent" versions.

The permanent versions especially are susceptible to the aluminum layer
(the LABEL side) oxidizing, and then falling apart.

As the disks go through thermal cycling, there can also be problems with
de-lamination.

Scratches on the "bottom" side of the media are relatively harmless.
Some media is VERY susceptible to scratching and damage on the top or
label side. In addition to avoiding the acidic "Sharpies", avoid
pencils, ball point pens, etc. I would also caution against trying to
"undo" any pressure sensitive label.

DVD-R may prove to be more stable then their CD-R counterparts. I would
still be cautious. Many of the vulnerabilities of CDs (permanent and
recordable) were not realized until recently. There may be unknown
vulnerabilities to DVD-Rs that we don't know about yet either.

Probably the most reliable "archive" media is still magnetic tape. I
have know people that have taken a tape from a "fireproof" safe, where
the tape cartridge was melted beyond use (due to longer than rated
exposure), and even appeared "melted into" the tape. The tape was sent
out to a recovery specialist and 90% plus of the data was recovered.
The stuff takes a beating and keeps on winding.

John W. Raffensperger, Jr.
IT Manager
Apache Stainless

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 20:18:09 2004

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(9/17/04 9:01) Gary Gaugler {gary-at-gaugler.com} wrote:

} Depending on your definition of archival, Mitsui DVD-R
} media ought to work for you. Their media is rated at
} 75 year retention. Their Gold Archival CD-R is rated
} at 100 years. Obviously, don't expect these results
} if you leave them on the rear deck of your car for
} twenty years.
}
} I believe that this topic has been discussed before
} and archived. If not, it will get archived now.
}
} My belief and strategy is to have four, redundant backups.
} The first backup is either dual CD-R or dual DVD-R.

}
} The hard drives are in removeable bays and are real time
} storage and retrieval media. The SNAP/NAS servers are
\
}
} The LTO 1 media will hold 100GB of un-compressed data.

}
} A most important aspect of backing up is to actually do it.
}
} gary g.

Of course, in 20 years, no drives will exists that will read any of the above media, so it really doesn't matter how long the supposed "archival" DVDs last, now does it. How many DECtape readers have -you- seen recently?

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 17 23:55:33 2004

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} From: "Brent Neal" {brent-at-reindeergraphics.com}
:
: (9/17/04 9:01) Gary Gaugler {gary-at-gaugler.com} wrote:
:
: } Depending on your definition of archival, Mitsui DVD-R
: } media ought to work for you. Their media is rated at
: } 75 year retention. Their Gold Archival CD-R is rated
: } at 100 years. Obviously, don't expect these results
: } if you leave them on the rear deck of your car for
: } twenty years.
: }
: } I believe that this topic has been discussed before
: } and archived. If not, it will get archived now.
: }
: } My belief and strategy is to have four, redundant backups.
: } The first backup is either dual CD-R or dual DVD-R.
:
: }
: } The hard drives are in removeable bays and are real time
: } storage and retrieval media. The SNAP/NAS servers are
: \
: }
: } The LTO 1 media will hold 100GB of un-compressed data.
:
: }
: } A most important aspect of backing up is to actually do it.
: }
: } gary g.
:
:
:
: Of course, in 20 years, no drives will exists that will read any
of the above media, so it really doesn't matter how long the
supposed "archival" DVDs last, now does it. How many DECtape readers
have -you- seen recently?
:
If you want to preserve your work, data, photos, notes and such
forever there is no computer media up to the task. Only a system
that relies on copies of the data sorted in geographically diverse
location that are recopied to new media and updated media as it
becomes available. This quickly becomes a very large difficult
problem much like putting one grain of wheat on the first square of
a chess board, 2 on the second, 4 on the third, ..... and you exceed
the world capacity to grow wheat before the chess board is full. It
is more practical with computer data but not a lot and any of us the
are truly confident of the integrity our back ups are few and far
between.

I still contend that black and white silver halide film is the least
expensive longest lived option available. We can all do it and
afford it and the technology is well tested an proven. Building a
device to put digital information on 35 mm film would be trivial and
we all have the equipment for our images. Adding a copy stand covers
notes and printed matter. With today's technology that we can use
that is proven to have a 150 year life stored in a shoe box. Modern
film substrates probably fixed and toned stored in a controlled
atmosphere should last a very long time indeed.

Digital images, data and writing are sure a lot more convenient but
they are sure not as reliable or as long lived as conventional
photography.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 18 07:40:53 2004

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Gordon Couger writes ...

} : Of course, in 20 years, no drives will exists that will read any
} of the above media, so it really doesn't matter how long the
} supposed "archival" DVDs last, now does it. How many DECtape readers
} have -you- seen recently?

I don't know that I'd agree. Today's optical media and drives appear to
offer a means for total backward compatibility ... e.g., DVD drive which can
read CDs. This is of course up to the manufacturers sticking to it and
supporting its application toward archiving.

That said ... I believe this thread should be as much about the
dependability of the software. It isn't so much about the media ... e.g.,
if an archive was written today, what software would be able to restore it
in 20 years? What can I use with confidence? ... which will write archives
identical to the original directory structure, without splitting files, and
verify the archive integrity??? Will the software maintain any database
characteristics of the original collection of files?? What software would
support and manage redundant archives across multiple devices (as Gary
Gaugler suggested as required)??

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 18 08:29:08 2004

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Perhaps we're way too obsessed with saving everything.
-Michael

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 18 08:43:29 2004

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(9/18/04 9:54) Michael Cammer {cammer-at-aecom.yu.edu} wrote:

} Perhaps we're way too obsessed with saving everything.
} -Michael

You try doing a patent defense 15 years later without the original micrographs.

B
--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Sat Sep 18 10:34:43 2004

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I have a DEC TK-70, circa 1990. I don't have
any VAX systems any more so the drive is not
really being used. That said, it is a DLT-II
tape unit. This format is still offered, and
media is still available. It is not a huge
repository of data. So from a hardware standpoint,
this is a viable option. But the point of selecting
a long lived platform is valid.

The longer the media type and drives stay around,
it is all that much longer before the data needs to
be migrated to newer methods. If one picks reliable
and solid backup software from either NovaStore or
Veritas, they very much seem to be fully backwards
compatible regardless of the OS that was used to
host the app. Furthermore, these apps will backup
to drives, tapes, CDs and DVDs. So, it gets back
to the hardware media set. Once written, the app's
format does not change. The new app will have new
features but it allows reading older media that used
earlier versions of the app.

The most long lasting standard as I recall is SCSI.
If the drive works, it can still be read today.
SCSI has evolved to SCSI-II and more exotic types
like LVD (low voltage differential). Even Adaptec
LVD adapters will work with single ended narrow SCSI
devices. They have made dual channel adapters so
each side can work with either type of media.

SCSI is fast but it is costly. Hence, this is why
I prefer the IDE/ATAPI drives at about 1/3 the cost
of a similar SCSI drive. MFM was around at first
but gave way to IDE, and IDE is still here. What is
happening now is that the parallel IDE/ATAPI is
evolving to serial ATA (SATA). They are not plug
compatible. Even if mother boards drop parallel
IDE, there are SATA-to-IDE adapters. In fact, current
versions of SATA drives include a SATA-to-IDE adapter
since true SATA drives are just now coming to market.

My selection of backup was carefully made to support
archiving tens of thousands of digital images. Many
of these are 30MB-250MB TIFF each. As was pointed out,
technology moves on. Consequently, a one time archive
is not going to last indefinitely into the future.
But it potentially could if properly designed. I'm
not taking that chance.

How many specimens do you all prepare and archive? What
about this facet of preservation? If the captured
data was lost, having the specimen would allow re-doing
the imaging. A pain for sure but not fatal. Properly
prepared specimens stored in a vacuum seem to hold up
for a long, long time with no discernable effects.
So, archive the specimens (this can get overwhelming
for sure) and archive the image results.

BTW, I use a fine point Sharpie to write on CDs and DVDs.
I never have a problem. The big felt markers are a no-no.

gary g.

At 06:08 AM 9/18/2004, you wrote:

} Gordon Couger writes ...
}
} } : Of course, in 20 years, no drives will exists that will read any
} } of the above media, so it really doesn't matter how long the
} } supposed "archival" DVDs last, now does it. How many DECtape readers
} } have -you- seen recently?
}
} I don't know that I'd agree. Today's optical media and drives appear to
} offer a means for total backward compatibility ... e.g., DVD drive which can
} read CDs. This is of course up to the manufacturers sticking to it and
} supporting its application toward archiving.
}
} That said ... I believe this thread should be as much about the
} dependability of the software. It isn't so much about the media ... e.g.,
} if an archive was written today, what software would be able to restore it
} in 20 years? What can I use with confidence? ... which will write archives
} identical to the original directory structure, without splitting files, and
} verify the archive integrity??? Will the software maintain any database
} characteristics of the original collection of files?? What software would
} support and manage redundant archives across multiple devices (as Gary
} Gaugler suggested as required)??
}
} cheerios ... shAf :o)

From MicroscopyL-request-at-ns.microscopy.com Sun Sep 19 12:03:15 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, September 19, 2004 at 11:37:16
---------------------------------------------------------------------------

Email: kssim-at-mmu.edu.my
Name: kssim

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone know tell me whether there is stigmatism problem or auto focusing problem at high resolution on optical misroscope? How to solve this problem?? Let me know ...

Many thanks
Ks

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 02:43:22 2004

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Hi,

A nice introduction to astigmatism in microscopy can be found at:

http://micro.magnet.fsu.edu/primer/java/aberrations/astigmatism/

Autofocusing on a digital microscope works fine, even at high
magnification (63x, 1.4 NA) in both brightfield as well as fluorecence
microscopy, as was published in:

Geusebroek J.M., Cornelissen F., Smeulders A. W. M., and Geerts H.,
Robust autofocusing in microscopy.
Cytometry, 36(1), pp. 1-9, (2000).

Regardless of which algortihm you use, it is important to sample your
Z-stack at the appropriate interval (see Geusebroek et al.).

Regards,

Peter

----------------------------------------------
Peter Van Osta

Director Imaging
MAIA SCIENTIFIC (formerly Union Biometrica NV)
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
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} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, September 19, 2004 at 11:37:16
} ---------------------------------------------------------------------------
}
} Email: kssim-at-mmu.edu.my
} Name: kssim
}
} Organization: mmu
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: Does anyone know tell me whether there is stigmatism problem or auto focusing problem at high resolution on optical misroscope? How to solve this problem?? Let me know ...
}
} Many thanks
} Ks
}

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 08:06:05 2004

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Peter Van Osta provided a reference to a very helpful article. Sadly, there was a typo in the reference. The correct citation is

Geusebroek J.M., Cornelissen F., Smeulders A. W. M., and Geerts H.,
Robust autofocusing in microscopy.
Cytometry, 39(1), pp. 1-9, (2000).

The article is worth the look...

I also found the following article helpful:
A. Santos et. al., "Evaluation of autofocus functions in molecular
cytogenic analysis," J. Microsc., 188(3), 264-272 (1997)

In particular, I found the functions "F4" and "F5", attributed to Vollath,
to be robust.

Hope this helps.

John Minter

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 17:13:11 2004

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That's a good point about the software needed to access these archived
CD's remaining available. I now have a number of CD's of data that were
made using Roxio's "Direct CD" that I do not have on my new computer.
And Win XP's CD handler won't access the files. The data isn't so
important for me to take the trouble to find Direct CD and load it onto
my new computer just to off load data from old CD's. But it made me
aware of the fact that Win XP's CD handler isn't going to be around
forever either. When the new "Big Thing" shows up, we need to be ready
to transfer anything that's important to the new media. Come to think of
it, I have a bunch of stuff on Jazz cartridges too.

Joiner Cartwright, Jr., Ph.D.
Baylor College of Medicine
Houston, Texas U.S.A.

-----Original Message-----
} From: michael shaffer [mailto:michael-at-shaffer.net]
Sent: Saturday, September 18, 2004 7:09 AM
To: MSA listserver

Gordon Couger writes ...

} : Of course, in 20 years, no drives will exists that will read any of
} the above media, so it really doesn't matter how long the supposed
} "archival" DVDs last, now does it. How many DECtape readers have -you-

} seen recently?

I don't know that I'd agree. Today's optical media and drives appear
to offer a means for total backward compatibility ... e.g., DVD drive
which can read CDs. This is of course up to the manufacturers sticking
to it and supporting its application toward archiving.

That said ... I believe this thread should be as much about the
dependability of the software. It isn't so much about the media ...
e.g., if an archive was written today, what software would be able to
restore it in 20 years? What can I use with confidence? ... which will
write archives identical to the original directory structure, without
splitting files, and verify the archive integrity??? Will the software
maintain any database characteristics of the original collection of
files?? What software would support and manage redundant archives
across multiple devices (as Gary Gaugler suggested as required)??

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 19:22:33 2004

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Hello everyone,

Previously I worked for a GLP accredited CRO, and we had some guidelines
on using CDs for backups. At that time I was the Systems Administrator
(Bask in Zoology, go figure...) and wrote most of their Standard
Operating Procedures. Generally this can be summed up:

- Buy gold or silver CD-Rs, and buy a reputable brand. 'Gold' or
'silver' CDs usually use a reactive metal coating to store data, rather
than a photoreactive dye as seen in 'green' or 'blue' CDs. The metal
based CD-R is more stable and (usually) better quality. I'd trust these
for 5 years. Good brands are Kodak, Imation, Verbatium, TDK, Sony,
Mitsubishi. Other brands may be good too, if you trust their VHS or
Audio tapes then you can trust their CD-Rs.

- Never ever CR-RW. Untrustworthy and expensive. CD-Rs are cheap, use
it, store it, throw it away. Better than losing data.

- Buy a good CD writer. This is hard for those not savvy with PCs. Buy a
good brand, and not all the good brands are well-known brands. Asus,
Sony, Pioneer, and Plextor are considered the best. Never use HP CD
writers, though this is mostly from poor personal experience. Finally,
buy a new one every two years, or more often if you use it lots. Make
sure that it has a 2MB buffer or bigger (8MB is best) and some form of
'underrun protection'.

- Get good software and use it. Forget the widgets built into Windows
2000/XP, too easy to stuff up. Don't use DirectCD. Don't use ROXIO (some
versions of Roxio software had some serious bugs that put your whole
hard drive at risk! I'm not forgiving enough to start using their
software again). I recommend Nero Burning ROM. It's cheap, easy, and
often comes bundled with a CD-Writer. CloneCD is a good package for just
copying CDs.

- Keep your CDs safe. A cool dry dark place. A cupboard is fine. Do not
keep CDs in the fridge or freezer, some brands get very brittle at low
temperatures and will shatter in the CD drive. Keep them out of direct
sunlight and don't store them in a car.

Finally for the really paranoid. Don't use CDs, use tapes, or even
better arrange for a reputable archiving company to do your backups for
you and store them off site. If you have to use CDs, make multiple
copies and keep one set off site. Use more than one brand of CD-R and
alternate, so if one brand packs it in, the next month/week CD will
still be Ok.

More will probably come to me later.

Aaron Hicks
Electron Microscopy Preparation Technician

Comparative Physiology and Anatomy
Institute of Veterinary, Animal, and Biomedical Sciences
Massey University

PN-412
Private Bag 11 222
Palmerston North
New Zealand

Phone +64 06 350 4470

At 03:46 PM 9/16/2004, you wrote:

} Dear colleague,
} I remember some discussion about CD-R storage. Some CD are not good at
} all and in many cases some CD become unreadable after 3 years.
} I would like to know what is the best brand or type of CD for storing

} images
}
} Keep care and be of good cheer
}
} Regards
}
} (name) Vratislav Richard Eugene Maria John Baptist
} (surname) of Bejsak (Bayshark)-Colloredo-Mansfeld

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 22:33:34 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (patljg-at-gwumc.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 20, 2004 at 11:47:56
---------------------------------------------------------------------------

Email: patljg-at-gwumc.edu
Name: lesley graham

Organization: george washington university

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Recently, I have been having problems with my thick sections lying flat. Nothing has been changed in the protocol; section, stain, and rinse. No matter how carefully I place the section on the slide, it will not be flat after the slide has dried.

Lesley Graham

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 22:33:58 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jameen-at-rohmhaas.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 20, 2004 at 16:05:08
---------------------------------------------------------------------------

Email: jameen-at-rohmhaas.com
Name: Joseph G. Ameen

Organization: Rohm and Haas Electronic Materials

Title-Subject: [Microscopy] [Filtered] MListserver: electronic Magnetic Cancellation Systems

Question: Does any one know if the Electromagnetic Compensation Systems or Magnetic Active Compensation systems work on an SEM? Our company is about to purchase a new SEM and the site survey showed AC fields in the 11 - 29 milliGauss range and DC fields in the 2 mG range. Vibration testing was fine. The stray fields are at least an order of magnitude higher then the recommended levels. Has anyone had experience with these cancellation systems?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 20 22:34:16 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (cmeyer911-at-yahoo.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 20, 2004 at 22:23:28
---------------------------------------------------------------------------

Email: cmeyer911-at-yahoo.com
Name: Chris Meyer

Organization: Boeing

Title-Subject: [Microscopy] [Filtered] [TEM] Selected Area Diffraction ZA Deconvolution

Question: I would like to hear any suggestions as to what is the best free software or web-based solutions site, for de-convoluting zone axis for selected-area diffraction patterns based on angles and length ratios. I'm specifically looking for some help beyond the FCC, BCC and HCP (with Ti c/a ratio)that I find in textbooks.

Any suggestions?

Thank you

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 11:12:26 2004

Contents Retrieved from Microscopy Listserver Archives
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RE: Plastic Membrane Boxes, Gel Sticky Box, Wafer Containers (see website
below)

I am looking for containers of ion-milling samples and small pieces in
progress of sample preparation. I found three types of containers: Membrance
Box, Stickey gel box, and just small containers. Is there any suggestion,
regarding advantage or disadvantage. I am using this when I trip by car or
airplane.

I know that some people use TEM grid boxes that come with carbon films when
you buy it. I don't like this because sometimes I break ion-thinned samples
when I close the cover.

Thank you,

Hiromi Konishi
Indiana University

Products websites:

http://www.mtixtl.com/index.asp?PageAction=VIEWCATS&Category=212

http://www.tedpella.com/box_html/membox.htm

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 11:23:55 2004

Contents Retrieved from Microscopy Listserver Archives
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Lesley,
I presume that you have already stained your semi-thin sections at that
point, when you notice that the section is no longer flat. One thing that I
have noticed, is that a person needs to wait a bit longer after the section
has dried on the hot plate before they start staining. So when the section
is drying, I am busy typing my slide labels, but even then, when the slide
looks dry and ready to go, it isn't in fact ready to go, and you need to
give it a few more minutes, otherwise you won't have a good bond of the
section to the slide, and it will start to lift off during the staining, and
especially the washing after the staining. This could be the most
frustrating thing in the universe if this happens.

If on the other hand, you give your slide some time to BOND to the slide, (a
few minutes) even after it has dried down, then the sections will refrain
from lifting up and folding over during the staining process.

If you allow it this extra time, you can be quite rough with the slide
during the staining and washing, and those sections won't lift off and fold.
And not only that, but you won't have to use coated slides to make sure that
the sections won't wash off, because they won't be going anywhere.

Garry

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (patljg-at-gwumc.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Monday, September 20, 2004 at 11:47:56
---------------------------------------------------------------------------

Email: patljg-at-gwumc.edu
Name: lesley graham

Organization: george washington university

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Recently, I have been having problems with my thick sections
lying flat. Nothing has been changed in the protocol; section, stain, and
rinse. No matter how carefully I place the section on the slide, it will
not be flat after the slide has dried.

Lesley Graham

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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 13:11:54 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello,
I have some Kodak EM film SO-163 and the expiration date was July 2003.
It has been stored in the freezer. What are the odds that it is still
useable? Any advice would be appreciated.
thanks in advance,
Beth

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 13:28:48 2004

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Hello Lesley,
When I cut resin thick sections (0.5 - 5.0 microns) I transfer the
sections to a drop of water on a slide and set the slide on a slide warmer
under a large Petri dish cover with a cotton swab dipped in toluene. The
toluene vapor softens and smooths the resin sections so that they flatten
and adhere to the slide.

At 10:32 PM 9/20/2004 -0500, you wrote:
} Email: patljg-at-gwumc.edu
} Name: lesley graham
} Organization: george washington university
} Title-Subject: [Microscopy] [Filtered] MListserver:
} Question: Recently, I have been having problems with my thick sections
} lying flat. Nothing has been changed in the protocol; section, stain, and
} rinse. No matter how carefully I place the section on the slide, it will
} not be flat after the slide has dried.
} Lesley Graham

Dean Abel
Biological Sciences 143 BB
University of Iowa
Iowa City IA 52242-1324

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 14:55:49 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Definitely useable
Chris

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "Beth Richardson" {beth-at-plantbio.uga.edu}
To: "microscopy microscopy" {microscopy-at-msa.microscopy.com}
Sent: Tuesday, September 21, 2004 7:10 PM

On Sep 21, 2004, at 11:10 AM, Beth Richardson wrote:

} I have some Kodak EM film SO-163 and the expiration date was July
} 2003. It has been stored in the freezer. What are the odds that it is
} still useable? Any advice would be appreciated.
} thanks in advance,

Dear Beth,
When I was at Albany, we had both 4489 and LoDose films that had been
refrigerated for some years when I got there, so was from the 70s or
before. When I used either film and developed it according to
instructions, there was no loss of contrast compared to fresh film, and
the fog level--especially with the LoDose, which is about 1.5 orders of
magnitude more sensitive than SO163--was not measurable; i.e., one
could detect only a few grains in a 10 x 10 um field, and the
microdensitometer reading was 0.000 OD. Unless the quality control has
gotten much worse, I expect that the SO163 should be indistinguishable
in response from brand new film.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 16:19:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Hiromi,
I use flat silicon rubber plates to hold ion-milled samples. These are flat
slabs of silicon rubber that fit in a petri plate and the pieces or grids
stick to them, then release them cleanly. They are available from Canemco
(Canada) and probably other EM suppliers and are marked off in numbered
squares. I have also made my own out of the castable silicon rubber kits.
Good luck,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {hkonishi-at-indiana.edu}
To: {Microscopy-at-microscopy.com}
Sent: Tuesday, September 21, 2004 9:10 AM

Hiromi: I like the membrane boxes for thin, non-mechanically strong
things. They hold tightly but when you take the lid off, the parts can
be handled w/ ease. I love the sticky-gel-type boxes for most
everything else but things do STICK in them and can be damaged when
trying to remove them. For what you're doing, I recommend the membrane
boxes.

hkonishi-at-indiana.edu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 17:46:49 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (donaldawbrey-at-texashealth.org) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, September 21, 2004 at 09:05:20
---------------------------------------------------------------------------

Email: donaldawbrey-at-texashealth.org
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Harrris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] Printers for diagnostic quality images.

Question: Dear fellow mico netters,

We are checking into purchasing a monochrome laser printer that will be used to print EM photos for diagnostic purposes.

The ones we are looking at are at 1200 X 1200 dpi and have a 16-32MB expanded memory. We are not neccessarily interested in print speed.

We will be using a 2K camera on our TEM.

Will this printer give us the quality for photographs that will be used for pathology diagnosis in a clinical setting? Will these prints be of good quality to pass any laboratory inspection (i.e. CAP)?

Thank you in advance for any info.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 18:14:48 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Karen,
There was some discussion of microwave protocols for insect larvae in January 2004. Try the Listserver archives for these. Myself, I found that much trial and error was necessary. Some things you may want to try include:

- Karnovsky's fixative (glutaraldehyde & paraformaldehyde in phosphate buffer)
- injecting the fixative into the specimen
- using the vacuum (I draw the vacuum to 20" Hg and leave it for 5 minutes before MWing. MW with vacuum on.)

Using cooled Karnovsky's, I draw up a vacuum, leave it for 5 min and then MW with an initial sequence at 100 W (2 min 0% power, 2 min 100% power, 3 min 0% power), cool my specimen to 20 deg C, draw up a vacuum and MW for a second sequence at 450 W (30 sec 0% power, 30 sec 100% power, 30 sec 0% power). I repeat the 450 W sequence 3 times. After I let my specimens sit in fix for 5 min.

For my osmium step, with a vacuum and cooled solution, I MW at 100 W for a sequence of 2 min 0% power, 2 min 100% power, 3 min 0% power. I also let the samples sit in osmium for a few minutes (10-20 min).

I've used this on larvae larger than mosquitos (specifically, diamond back moth and Colorado potato beetle) and it has yielded good results. I've also found that processing several samples will yield some with good quality fixation and the others can be discarded.

If you have any questions, feel free to contact me. I'd be interested in hearing how things worked out for you.

Shannan

Shannan Little
Research Technician/Technicien de recherche
Electron Microscopy and Image Analysis /Microscopie électronique et Analyse d'images
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 403-317-3446
Facsimile/Télécopieur: 403-382-3156
P.O. Box 3000 / CP 3000
Lethbridge, Alberta T1J 4B1
littlesm-at-agr.gc.ca
http://res2.agr.ca/lethbridge/emia/index_e.htm

-----Original Message-----
} From: Karen Kelley [mailto:klk-at-biotech.ufl.edu]
Sent: Thursday, September 16, 2004 4:06 PM
To: Microscopy-at-MSA.Microscopy.Com

Hello All,

I have a BioScan Ted Pella microwave with a cold-spot and vacuum chamber
that I would like to use for fixation and embedding insect eggs and larvae
for TEM.

The project includes mosquito larvae, pupae and fly eggs. I worked on this
same project many years ago using traditional benchtop methods. The eggs
and larvae were difficult, if not impossible, to infiltrate. Now that I
have a MW with vacuum I am trying this project again.

I would greatly appreciate any suggestions, advice or direct me to references?

My first attempt at MW didn't go so well.
I MW fixed the larvae with 2% glut in cacodylate in 1.5ml centrifuge tubes
at 20mmHg vacuum -at- 250W 1' on, 1' off. Repeated several times removing the
vacuum to observe the larvae. At first when vacuum was applied the larvae
floated to the top and squirmed around a bit, then after several attempts
at that they finally all stopped moving and didn't float. Buffer washed on
benchtop then used the vacuum again at the same settings for the buffered
osmium tetroxide. Just the ends of the larvae turned black. I tried it
again without any change. I finally got tired of messing with them and
placed them into a KFeCN + OsO4 overnight at 4C and have had them stored in
buffer. ( I have used the overnight KFeCN + OsO4 with success for hard to
infiltrate nematodes). Dehydrated with MW 40s -at- 250W no vacuum 40 s on, 1'
off, infiltrated 50% acetone/Embed no vac at 250W 3', 100% Embed -at- 450W
with vac (20mm Hg). The larvae had areas of collapse after the 100% with
vacuum so I'm concerned that they are not infiltrating as I had hoped.

Karen L. Kelley
ICBR Electron Microscopy Manager
University of Florida
ICBR Electron Microscopy Core Lab
Bartram Hall Room 214
Box 118525 Gainesville Florida
Lab: 352-392-1184 fax: 352-846-0251
Email: klk-at-biotech.ufl.edu
Southeastern Microscopy Society Treasurer
http://www.biotech.ufl.edu/EM/

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 19:12:31 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I also swear by the membrane boxes. I use the small 1 x 1 size. For very brittle samples, such as II-Vi and III-V compounds, I don't put the membrane boxes together with full force. Just tight enough so that they can't go from edge to edge. I also re-use them. I use 1" white Post-it tape and tear off long enough to use as a label.

One thing that you must be very careful with using these and that is that the sample must be thoroughly dried from any solvents that you may have used, especially acetone. If the sample is even slightly damp when you put it in, it will stick to the membrane.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: hkonishi-at-indiana.edu [mailto:hkonishi-at-indiana.edu]
Sent: Tuesday, September 21, 2004 12:11 PM
To: Microscopy-at-microscopy.com

RE: Plastic Membrane Boxes, Gel Sticky Box, Wafer Containers (see website
below)

I am looking for containers of ion-milling samples and small pieces in
progress of sample preparation. I found three types of containers: Membrance
Box, Stickey gel box, and just small containers. Is there any suggestion,
regarding advantage or disadvantage. I am using this when I trip by car or
airplane.

I know that some people use TEM grid boxes that come with carbon films when
you buy it. I don't like this because sometimes I break ion-thinned samples
when I close the cover.

Thank you,

Hiromi Konishi
Indiana University

Products websites:

http://www.mtixtl.com/index.asp?PageAction=VIEWCATS&Category=212

http://www.tedpella.com/box_html/membox.htm

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 21 21:29:25 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear All:

When we use our TEM at low magnification (below 4,000X), we sometimes
get a bright spot in the middle of pictures we take. I always thought
the microscope setting was the only thing responsible for this
problem. But when I checked into a latest episode, I found pictures
from one particular specimen (thin sections on Formvar coated grid) had
it, but others from a different specimen (negative staining on
Farmvar/carbon coated grid) did not, even though all pictures were
taken with the same scope setting. Has anyone else experienced the
same? Can anyone explain to me thoroughly how this problem occurs, and
how to avoid it. Thank you very much in advance.

Hong
Emory EM

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 22 07:45:41 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (dieter-at-genetik.uni-bielefeld.de) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 22, 2004 at 06:14:11
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Email: dieter-at-genetik.uni-bielefeld.de
Name: Dieter Kapp

Organization: Academic/University

Title-Subject: [Microscopy] [Filtered] MListserver: Which Deconvolution Software?

Question: Hello Listers!

We are currently searching for a deconvolution software.
Mainly we look at GFP-fusions in single cells, monolayers (Sf9) or cell aggregates (tobacco BY2), up to 100 µm on a Olympus IX81.

What are your experiences with such a software tool?
How are the results compared to confocal images of the same specimen (...okay, deconvolution can be applied to confocal images too)?
Is it worth the money?

The two major competitors in the market are SVI/Huygens and AutoQuant. Which product did you choose and why?
Is there a side by side test of both softwares available? Do they differ in image quality?
We only need deconvolution, since our imaging software is doing well.
Do you have other recommendations/suggestions?

Any comment on this issue will be warmly welcomed!
Thank you in advance,

Dieter

------------------------------------------------------------
Dr. Dieter Kapp
Lehrstuhl fuer Genetik
Postfach 100131
Universitaet Bielefeld PHONE: +49 (0)521 106 5620
D-33501 Bielefeld FAX: +49 (0)521 106 5626
GERMANY Email: dieter-at-genetik.uni-bielefeld.de

------------------------------------------------------------

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From MicroscopyL-request-at-ns.microscopy.com Wed Sep 22 10:19:59 2004

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Pacific Northwest Microscopy Society (PNMS) announces its annual meeting
held this year in Hillsboro, OR during two half-day sessions on
September 30 and October 1st.

The FEI company generously offered its new facility for the meeting
location, and largely contributed to its program.
Two parallel platform sessions will run in biological and material
sciences. Besides the scientific program, demonstrations of the FIB and
a Technai TEM will be available, as well as the FEI factory tour. The
evening social at the historical Cornelius House and Brewery will
include a barbecue dinner, and it is covered with the registration. The
second day morning biological session will take place in the OSHU
Primate Center including its tour.
Due to the space limitation (50 people), we require advanced
registration. Registration is free of charge to the current PNMS
members, and $10 for non-members.

Program:

Fall 2004 Annual Meeting
When: Thursday Sept. 30th, and Friday October 1st, 2004
Where: FEI Company, Hillsboro, Oregon
OHSU National Primate Research Center

Thursday Sept 30, 2004
11:30am - Arrival to FEI, registration
12:00 - Lunch
12:30 - Welcome note
- 2 keynote speakers provided by FEI
Speaker I - DualBeam Applications in Biological and Materials Science
Speaker II - Tomography Applications in Biological and Materials Science
1:45pm - break

2:00 - Demonstrations of DualBeam Focused Ion Beam (FIB) instrument, and
the Tomography capability on a Technai TEM (split into 2 groups)
2:45 - break

3:00 - Split into 2 sessions - Biological and Material Science platforms
will
run in parallel.

Material Science:
3:00 - Jun Jiao, Portland State University
3:20 - Joe Robinson Ascend
3:40 - David Basile, HP
4:00 Break
4:10 - Barbara Miner, Intel
4:30 - Eric Sanchez, Portland State U
4:50 - Jeff McDowell, Rontec

Biological Sciences:
3:00 - Elaine Humphrey, University of British Columbia - "Microwave
Processing In a Modern Microscopy Facility"
3:30 - Glen MacDonald, University of Washington Seattle, Virginia
Merrill Bloedel Hearing Research Center
4:00 - mini workshop: "Coloring Electron Micrographs With PhotoShop"
presented by the image processing guru Jim Young

5:15 -6:00 - Poster session
We are soliciting poster presentations in both areas, and strongly
encouraging students to participate in the poster session.
6:00 - Dinner social at the Cornelius Pass Road House and Brewery
(McMenamins).
Poster winners announcement.

Friday Oct. 1, 2004
9:00 Arrival at FEI
9:15 - FEI factory tour (!!!), talk: Emitters and Optics by FEI Beam
Technology.
10:15am Depart from FEI, commute (only minutes drive) to the OSHU's
Primate Research Center.
10:30 - 11am Tour of the Primate Center.
11am -2pm Biological session at the conference room, tour of Imaging
and Morphology Core Facility (Anda Cornea lab director). Lunch will be
arranged in the cafeteria within the PC.
2pm - departure.

Alice Dohnalkova
PNMS President
Environmental Microbiology
Pacific Northwest National Laboratory
Richland, WA 99352
(509) 372-0692 office
(509) 376-3654 TEM lab

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 22 12:20:41 2004

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I work for JEOL in the UK. We use them fairly frequently and they
generally work pretty well.

Normally, the standard systems only cancel AC fields - DC
cancellation is usually an option, although it is very rare that DC
fields need to be cancelled - the SEM alignment does that for you
unless the DC field is very high.

You need to look at the wave form of the AC fields - a coil and an
oscilloscope is all you need. If the wave form is fairly stable and
changes only relatively slowly, then cancellation will work well. If
it is changing a lot, then you may have problems - the control box on
the system we use has a LED to indicate when the field is cancelled
or if it is still calculating the wave form. In some cases, it will
help if you have two sensor boxes - these need to be placed as near
to the sample as possible, usually on either side of the chamber.
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 22 12:20:23 2004

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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

If you want top quality photo-standard prints, you really need a
dye-sublimation printer. Quite a bit more expensive to purchase and
to run than a laser printer but the results are much better. Codonics
make several printers aimed specifically at the medical imaging
market.
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 22 13:15:45 2004

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} When we use our TEM at low magnification (below 4,000X), we
} sometimes get a bright spot in the middle of pictures we take. I
} always thought the microscope setting was the only thing responsible
} for this problem. But when I checked into a latest episode, I found
} pictures from one particular specimen (thin sections on Formvar
} coated grid) had it, but others from a different specimen (negative
} staining on Farmvar/carbon coated grid) did not, even though all
} pictures were taken with the same scope setting. Has anyone else
} experienced the same? Can anyone explain to me thoroughly how this
} problem occurs, and how to avoid it. Thank you very much in advance.
}
} Hong
} Emory EM

The most likely cause is removal of the plastic due to the beam --
resulting in an area of lowered density. This is quite common (and
can sometimes be used to enhance the contrast of sectioned
specimens). What is probably happening is that someone is
investigating the specimen at high magnification with the beam
condensed to a small spot. When you then go to a lower magnification,
you will see the area where the beam spot has etched away the
plastic. Also, some people focus the image with the condenser reduced
in size (since it much brighter). If too much time is spent in this
condition, you will see the etching of the plastic after the beam is
spread.

One work-around would be to record the images at low mag FIRST and
then do the high mag work (where the condenser is reduced in size)
AND avoid focusing at crossover.

We sometimes use this with specimens of low contrast (LR White and
Spurr's, for example). As the plastic is removed by the beam, the
remaining specimen appears with greater contrast. In fact, our TEM
even has this capability programmed in by the manufacturer (the beam
is traversed over the specimen to "stabilize" the plastic--and it
also improves contrast).
--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 22 13:17:35 2004

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} When we use our TEM at low magnification (below 4,000X), we
} sometimes get a bright spot in the middle of pictures we take. I
} always thought the microscope setting was the only thing responsible
} for this problem. But when I checked into a latest episode, I found
} pictures from one particular specimen (thin sections on Formvar
} coated grid) had it, but others from a different specimen (negative
} staining on Farmvar/carbon coated grid) did not, even though all
} pictures were taken with the same scope setting. Has anyone else
} experienced the same? Can anyone explain to me thoroughly how this
} problem occurs, and how to avoid it. Thank you very much in advance.
}
} Hong
} Emory EM

The most likely cause is removal of the plastic due to the beam --
resulting in an area of lowered density. This is quite common (and
can sometimes be used to enhance the contrast of sectioned
specimens). What is probably happening is that someone is
investigating the specimen at high magnification with the beam
condensed to a small spot. When you then go to a lower magnification,
you will see the area where the beam spot has etched away the
plastic. Also, some people focus the image with the condenser reduced
in size (since it much brighter). If too much time is spent in this
condition, you will see the etching of the plastic after the beam is
spread.

One work-around would be to record the images at low mag FIRST and
then do the high mag work (where the condenser is reduced in size)
AND avoid focusing at crossover.

We sometimes use this with specimens of low contrast (LR White and
Spurr's, for example). As the plastic is removed by the beam, the
remaining specimen appears with greater contrast. In fact, our TEM
even has this capability programmed in by the manufacturer (the beam
is traversed over the specimen to "stabilize" the plastic--and it
also improves contrast).
--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 05:45:26 2004

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FYI, here is a current job opening at the GE Global Research Center in
Niskayuna, NY. To apply, please go to www.gecareers.com
{http://www.gecareers.com} and enter job #372689.

Materials Scientist/ Microscopist

Business Unit:

GE Global Research

Function:

Engineering/Technology

Location:

NISKAYUNA, NY

Job #:

372689
Posted: Aug 12, 2004

Job Description:
Responsibilities

The Microstructural and Surface Sciences Laboratory is involved in research
into the structure and composition of materials in support of development
programs both at GEGR and at GE businesses. Staff members are expected to
work independently with a high level of expertise, and to become involved
with a number of major project teams. The successful candidate will execute
research projects using advanced electron beam analysis of bulk materials
(e.g., HRSEM, EDS, EBSD, FIB) to study the structure and composition of
materials, including metals, ceramics, composites, polymers, and electronic
materials. Lead in the development of new advanced techniques for materials
characterization. Participate in or lead project teams with the goal of
developing new processes and materials.

Qualifications

BS required, MS preferred in Materials Science, Chemistry, or Physics.
Extensive training and experience in cutting-edge materials characterization
techniques, particularly electron beam techniques. Demonstrated technical
leadership capabilities with excellent teaming and communication skills.
THIS POSITION REQUIRES UNRESTRICTED U.S. WORK AUTHORIZATION (US citizen or
permanent resident status required).

General
We offer a competitive salary, outstanding benefits package and the
professional advantages of an environment that supports your development and
recognizes your achievements. We are an Equal Opportunity Employer.

****************************************************************************
**************************************
Katharine Dovidenko, Ph.D.
Materials Scientist
Microstructural and Surface Sciences Laboratory
GE Global Research Center
K-1-2C12, 1 Research Circle
Niskayuna, NY 12309
Phone: 518-387-4759
Fax: 518-387-6972
Email: dovidenk-at-research.ge.com {mailto:dovidenk-at-research.ge.com}

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 08:34:28 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rdesilva-at-ipn.mx) from on Wednesday, September 22, 2004 at 08:59:35
---------------------------------------------------------------------------

Email: rdesilva-at-ipn.mx
Name: Claudia Douriet

Organization: CIIDIR

Education: Graduate College

Location: Guasave, Sinaloa, MČxico

Question: Hi!
I just started to use a Leica stereomicroscope for my Bachelor degree work and unfortunately I never used one before. I am taking pictures of zooplanktonic organisms and I dont know how much magnification does a picture has. I am not sure if you have to multiply the zomm, by the objective and by the ocular numbers. Can you help me? Thank you very much.

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 08:55:24 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (zerfasp-at-ors.od.nih.gov) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 22, 2004 at 15:24:37
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Email: zerfasp-at-ors.od.nih.gov
Name: Patricia Zerfas

Organization: NIH

Title-Subject: [Microscopy] [Filtered] MListserver: Bone Fixation

Question: Does anyone have a protocol for fixing mouse bone tissue? The investigator does not have a microwave nor does she plan to profuse the animals.
Thanks.

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 08:55:37 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (john.dumont-at-ctel.net) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 22, 2004 at 16:26:34
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Email: john.dumont-at-ctel.net
Name: John dumont

Organization: Continental Consulting

Title-Subject: [Microscopy] [Filtered] Olympus EHT Scope

Question: I'm presently refurbishing an older Olympus Model EHT with a DO head. I require a lower and upper lamp assemblies, as well as an owner/operator's manual.

Any suggestions would be appreciated.

Thanks

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 11:06:25 2004

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Thank you for your input. I definitely have seen this removal of the
plastic phenomenon on scope. But I am not convinced that is all what
was happening here. The spot was there even if we moved away from
etched area. Also, the spot sometimes was so intense that it could be
seen on phosphor screen. Someone suggested that it has something to do
with the distance between the pole piece and the objective aperture. I
think I agree, but it seemed that the type of sample prep played a role
in it too.

Thank you all.

Hong

On Sep 22, 2004, at 2:14 PM, John J. Bozzola wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
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}
} } When we use our TEM at low magnification (below 4,000X), we
} } sometimes get a bright spot in the middle of pictures we take. I
} } always thought the microscope setting was the only thing responsible
} } for this problem. But when I checked into a latest episode, I found
} } pictures from one particular specimen (thin sections on Formvar
} } coated grid) had it, but others from a different specimen (negative
} } staining on Farmvar/carbon coated grid) did not, even though all
} } pictures were taken with the same scope setting. Has anyone else
} } experienced the same? Can anyone explain to me thoroughly how this
} } problem occurs, and how to avoid it. Thank you very much in advance.
} } Hong
} } Emory EM
}
} The most likely cause is removal of the plastic due to the beam --
} resulting in an area of lowered density. This is quite common (and can
} sometimes be used to enhance the contrast of sectioned specimens).
} What is probably happening is that someone is investigating the
} specimen at high magnification with the beam condensed to a small
} spot. When you then go to a lower magnification, you will see the area
} where the beam spot has etched away the plastic. Also, some people
} focus the image with the condenser reduced in size (since it much
} brighter). If too much time is spent in this condition, you will see
} the etching of the plastic after the beam is spread.
}
} One work-around would be to record the images at low mag FIRST and
} then do the high mag work (where the condenser is reduced in size) AND
} avoid focusing at crossover.
}
} We sometimes use this with specimens of low contrast (LR White and
} Spurr's, for example). As the plastic is removed by the beam, the
} remaining specimen appears with greater contrast. In fact, our TEM
} even has this capability programmed in by the manufacturer (the beam
} is traversed over the specimen to "stabilize" the plastic--and it also
} improves contrast).
} --
} ##############################################################
} John J. Bozzola, Ph.D., Director
} I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
} 750 Communications Drive - MC 4402
} Southern Illinois University
} Carbondale, IL 62901 U.S.A.
} Phone: 618-453-3730
} Email: bozzola-at-siu.edu
} Web: http://www.siu.edu/~image/
} ##############################################################
}
}
======================
Hong Yi
Emory School of Medicine Microscopy Core
Emory University
6215 Woodruff Memorial Research Building
101 Woodruff Circle
Atlanta, GA 30322

Tel: (404) 727-8692 (Office), (404) 712-8491 (Lab)
Fax: (404) 727-3157
Email: hyi-at-emory.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 11:47:17 2004

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} } When we use our TEM at low magnification (below 4,000X), we
} } sometimes get a bright spot in the middle of pictures we take. I
} } always thought the microscope setting was the only thing
} } responsible for this problem. But when I checked into a latest
} } episode, I found pictures from one particular specimen (thin
} } sections on Formvar coated grid) had it, but others from a
} } different specimen (negative staining on Farmvar/carbon coated
} } grid) did not, even though all pictures were taken with the same
} } scope setting. Has anyone else experienced the same? Can anyone
} } explain to me thoroughly how this problem occurs, and how to avoid
} } it. Thank you very much in advance.
} } Hong
} } Emory EM
} =============
} The most likely cause is removal of the plastic due to the beam --
} resulting in an area of lowered density. This is quite common (and
} can sometimes be used to enhance the contrast of sectioned
} specimens). What is probably happening is that someone is
} investigating the specimen at high magnification with the beam
} condensed to a small spot. When you then go to a lower
} magnification, you will see the area where the beam spot has etched
} away the plastic. Also, some people focus the image with the
} condenser reduced in size (since it much brighter). If too much time
} is spent in this condition, you will see the etching of the plastic
} after the beam is spread.
}
} One work-around would be to record the images at low mag FIRST and
} then do the high mag work (where the condenser is reduced in size)
} AND avoid focusing at crossover.
}
} We sometimes use this with specimens of low contrast (LR White and
} Spurr's, for example). As the plastic is removed by the beam, the
} remaining specimen appears with greater contrast. In fact, our TEM
} even has this capability programmed in by the manufacturer (the beam
} is traversed over the specimen to "stabilize" the plastic--and it
} also improves contrast).
}
} John J. Bozzola, Ph.D., Director
} I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
} 750 Communications Drive - MC 4402
} Southern Illinois University
} Carbondale, IL 62901 U.S.A.
} Phone: 618-453-3730
} Email: bozzola-at-siu.edu
} ########################
Hong,
I knew what you were referring to on the low power magnification and
just checked it out on my old Philips 200.

The spot is evident on the screen when in low mag. and hence would be
on the negative if I took a picture. It even shows up on the grid
bar when I scan ONLY when the image is out of focus!

If you have a WOBBLER on your scope use it to get into focus and see
if the light spot disappears. If you do not have a wobbler, put in a
holey grid or of course a thicker section that has a hole or two and
focus on the hole to the point where it is in focus and look for the
spot.
I bet it is no longer there.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu
***********************

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Greetings all,
I'm helping with a project which requires dehydration/clearing of the
specimen for observation using laser scanning using both reflected light
and fluorescence detection. Also, we need to minimize mounting agent
shrinkage in order to preserve the z axis aspect ratio of the specimen.
I've suggested using an ethanol dehydration followed by clearing and
mounting in clove oil, but I'm not sure what problems we might encounter
from auto-fluorescence of the clove oil. Oil of wintergreen would work
also, I've just read that clove oil is a little more tolerant of
incomplete dehydration (and seeing as I'm not performing the dehydration
I figured a little margin for error would be a good idea). Any input on
the relative merits of clove oil/oil of wintergreen or even immersion
oil as a penetrating mounting agent would be appreciated. Thanks.
-Karl

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 14:42:10 2004

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We use clove oil routinely to clear spider genitalia that is preserved in
ethanol 75%, without any previous dehydration. It works very well. Larger
pieces take longer, but I guess you will be working with very small
preparations.

Other labs use lactic acid or methyl salicylate, but I prefer clove oil.

Martín J. Ramírez
División Aracnología
Museo Argentino de Ciencias Naturales
Av. Angel Gallardo 470
C1405DJR Buenos Aires
Argentina
tel +54 11 4982-8370 int. 168
fax +54 11 4982-4494

At 03:24 PM 9/23/2004, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 21:47:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Tammy-at-kbwiz.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Thursday, September 23, 2004 at 16:19:04
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Email: Tammy-at-kbwiz.com
Name: Tammy Schwalb

Organization: Schwalb Research

Education: Graduate College

Location: Irvine, CA

Question: I am lookig for an embedding media for a delicate tissue membrane encasing a small sensor surface. The device material is epo fix. I would prefer a hydrophilic material that is easy to cut. Any advice?

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From MicroscopyL-request-at-ns.microscopy.com Thu Sep 23 21:48:24 2004

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Name: sailesh pradhan

Organization: southern illinois university, carbondale

Education: Graduate College

Location: carbondale,illinois,USA

Question: i have been thinking about building an experimental setup to test the mechanical properties of thin films under loading using speckle pattern interferometry with electron microscopy...i would like to observe the speckle patters using the electron microscopy facility we have here(S-2460N hitachi)...it seems however that i might have problems placing the loading unit inside the chamber primarily owing to the contract they have here regarding the maintainence of the microscope with hitachi and also due to the fact that there arent supposed to be any EM fields or unapproved active devices inside the chamber...in this regard, i would be glad if you could help me out by providing ways to circumvent the problems involved....have people done that kind of work before? if so then how....how can u replace the motor, for example, to load the specimen?
i shall look forward to your reply...

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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 07:54:31 2004

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Dieter:

We are currently using the Slidebook by Inteligent Imaging Inc. (3I) with
an Olympus IX-81.
[http://www.intelligent-imaging.com/slidebook/overview.php ]

It integrates and operates the IX-81 fully, comes with all its available camera
drivers, and does little other than deconvolution. 3I seems to be readily
working with the camera vendors and Olympus to continually update the
drivers and software. I think it maybe a little less costly than the others but
came as a larger package deal. I've not tried the others - Slide book seems to
work well - makes use of multiple processors and available memory (4GB
RAM) to run pretty fast.

Deconvolution: We're just basic users in deconvolution but it does seem
to me that there has been plenty of published justification that the transition
from confocal to deconvolution is at 15-micrometers, i.e. below 15
deconvolution is better, thicker than 15 confocal is better. For 100um samples
you maybe far better served by confocal.

}
} Email: dieter-at-genetik.uni-bielefeld.de
} Name: Dieter Kapp
}
} Organization: Academic/University
}
} Title-Subject: [Microscopy] [Filtered] MListserver: Which Deconvolution
} Software?
}
} Question: Hello Listers!
}
} We are currently searching for a deconvolution software.
} Mainly we look at GFP-fusions in single cells, monolayers (Sf9) or cell
} aggregates (tobacco BY2), up to 100 µm on a Olympus IX81.
}
} What are your experiences with such a software tool?
} How are the results compared to confocal images of the same specimen (...okay,
} deconvolution can be applied to confocal images too)? Is it worth the money?
}
} The two major competitors in the market are SVI/Huygens and AutoQuant. Which
} product did you choose and why? Is there a side by side test of both softwares
} available? Do they differ in image quality? We only need deconvolution, since
} our imaging software is doing well. Do you have other
} recommendations/suggestions?
}
} Any comment on this issue will be warmly welcomed!
} Thank you in advance,
}
} Dieter
}
} ------------------------------------------------------------
} Dr. Dieter Kapp
} Lehrstuhl fuer Genetik
} Postfach 100131
} Universitaet Bielefeld PHONE: +49 (0)521 106 5620
} D-33501 Bielefeld FAX: +49 (0)521 106 5626
} GERMANY Email: dieter-at-genetik.uni-bielefeld.de
}
} ------------------------------------------------------------
}
}
}
} ---------------------------------------------------------------------------
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 08:10:01 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (John H. Cross-at-lmco.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, September 23, 2004 at 13:31:31
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Email: John H. Cross-at-lmco.com
Name: John H. Cross, CIH

Organization: Lockheed Martin Space Operations

Title-Subject: [Microscopy] [Filtered] MListserver: Occupational Health Aspects of Microscope Usage

Question: We have a group of technicians using microscopes to solder electronic components 10-12 hours per day 6-7 days a week.

Does any professional, academic, or industry organization publish occupational health guidelines for the use of microscopes? A sample of questions I need to address are: How often must an individual take a break from looking through a microscope. Is exposure to light coming through the eyepieces a problem? Has anyone described ergonomically-correct work stations for microscopists?

All comments will be welcome. I particularly need objective standards that I can present to management to justify work practice adjustments.

Thanks,

John Cross

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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 09:04:29 2004

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When doing semi-thin sectioning I face off my block to cut, when the
specimen comes across the knife it takes an obscenely thick section and
ruins my block face. I have had problems before where the first section is a
little too thick, but simply backing the knife off a little bit helped. No
matter what I do or change the section is still cutting too thick, are there
any suggestions before I go crazy!

Thanks,

Todd M. Hamm
Oklahoma Medical Research Foundation
825 NE 13th St
OKC, OK 73132
tmhamm09-at-yahoo.com

_________________________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 11:47:29 2004

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Todd

what sort of microtome are you using? If it's an LKB/Reichert ultramicrotome you could be aligning specimen and knife when the knife is retracted - this is part of the normal cutting cycle to prevent the block snagging the knife when it returns to the top of its travel. When you complete the first cutting cycle the microtome knife stage jumps forward at least 10s of microns. So when setting up for semi-thin sectioning make sure that this isn't happening - it's quite easy to do when you know how.

I haven't gone into detail in case this is not your problem, but it should be easy enough to check. Let me know if you need more info.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: todd hamm {ripbnowell-at-hotmail.com}

Dear Claudia,

The best way to define magnification is to set-up the microscope to a prescribed magnification and zoom (one which is reproducible) then to take a picture of either a ruler with mm or a stage micrometer. If you are viewing the image on a screen, you can lay an overhead transparency on the screen and draw the length of some convenient "marker bar" (ex: 50 micrometers). You will then always have the magnification available. Also, if you are going to capture digital images, most software gives you the ability to calibrate the magnification.

Because of the nature of both the focusing and zoom mechanism on the stereo microscope, it is more difficult to establish exact magnification, so you may need to repeat this calibration for each test run.

Good hunting!
Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
F: 972-954-8018

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.

At 08:33 AM 9/23/2004, rdesilva-at-ipn.mx wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 12:22:53 2004

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Dear Claudia,

The best way to define magnification is to set-up the microscope to a prescribed magnification and zoom (one which is reproducible) then to take a picture of either a ruler with mm or a stage micrometer. If you are viewing the image on a screen, you can lay an overhead transparency on the screen and draw the length of some convenient "marker bar" (ex: 50 micrometers). You will then always have the magnification available. Also, if you are going to capture digital images, most software gives you the ability to calibrate the magnification.

Because of the nature of both the focusing and zoom mechanism on the stereo microscope, it is more difficult to establish exact magnification, so you may need to repeat this calibration for each test run.

Good hunting!
Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
F: 972-954-8018

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.

At 08:33 AM 9/23/2004, rdesilva-at-ipn.mx wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 12:29:05 2004

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When doing semi-thin sectioning I face off my block to cut, when the
specimen comes across the knife it takes an obscenely thick section
and ruins my block face. I have had problems before where the first
section is a little too thick, but simply backing the knife off a
little bit helped. No matter what I do or change the section is still
cutting too thick, are there any suggestions before I go crazy!
______________________________________

Todd,
Could you give a little more info?

What microtome are you using? The "newer" ones (less than 20 years
old) have back lighting that makes approaching the block so much
easier.

I know that this may be a silly question, but are you sure that
everything is tight? (knife stage, knife holder, specimen chuck,
specimen arm)

How are you approaching the block face? I normally creep up on it
slowly using the knife advance while watching through the binoculars
until I'm shaving off little bits. Then I set up my section thickness
and cut a few thicks manually (rather than with the motor drive).

When you bring your knife up to the block are you sure that the
specimen arm is in the cutting stroke and not in the retracted phase
of the cycle?

Have you had your microtome checked to be sure that the calibration
for the thick sectioning mode is OK?

That pretty much covers all of the mistakes I've made over the years...
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 12:30:50 2004

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Dear Salish,

Again, this might be better done as a scanning probe experiment rather than an SEM experiment. You can readily measure force, adhesion, and viscoelasticity directly.

Contact me offline for details.

Best regards,
Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
F: 972-954-8018

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.

At 09:47 PM 9/23/2004, spradhan-at-siu.edu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 13:56:58 2004

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_________________________________________________________________
Get ready for school! Find articles, homework help and more in the Back to
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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 14:07:15 2004

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Sorry I was a little vague before, the ultramicrotome is a fairly new LKB
model. I found that when I take the semi-thins manually the problem isn't
as bad. Is it possible that the belt that controls the specimen advancement
has been worn, I thought that might be possible since the thickness varies
considerably from section to section. But like I said when section manually
it is much less of a problem.

Todd Hamm

_________________________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 14:39:01 2004

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Hello all,

We're looking at mouse embryos in the early
stages using quadrature tomographic microscopy.
What I want to do is rotate an embryo in specific
increments and image at these increments at
various time points (total ‰ 48 hrs). This will
be done in a Bioptechs chamber (no affiliation)
with additional atmospheric control.

My first thought is to "attach" the embryo to a
"tube" via a syringe, with slight negative
pressure. Then, attach a goniometer somehow to
the tube or the syringe.

These lists have been extremely useful in the
past and I thank you all in advance for your
input.

Best,

Gary
--

Gary Laevsky, Ph.D.
Keck Facility Manager, CenSSIS
Northeastern University
302 Stearns
360 Huntington Ave.
Boston, MA 02115

voice (617) 373-8570
fax (617) 373-7783

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 17:51:40 2004

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Hi:

Can anyone fill me in on the details of the EMSA file format for EDS spectra.

Mostly I need to know how to help someone strip out the header so they can
look at it in Excel.

The file I see when I look at it has the header info, followed by what
looks like 4 columns of numbers. I was expecting 2 columns, x and y. What's
up?

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 22:49:11 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (timandcathy-at-mho.com ) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Micro-Form.html on Friday, September 24, 2004 at 13:04:20
---------------------------------------------------------------------------

Email: timandcathy-at-mho.com
Name: Timothy Personett

School: NA

State: CO

Question: Hi I am looking for a microscope -at- 1600x to look at bacteria, I have seen oil immersion does the microscope need a oil lense or can you just use the oil on the slides ? and any ideas on good brands for the max power ?

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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 23:14:00 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (necipunlu-at-yahoo.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, September 24, 2004 at 08:51:18
---------------------------------------------------------------------------

Email: necipunlu-at-yahoo.com
Name: necip unlu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hey guys,

I need JEOL2000EX alignment procedure if you have that kind of knowledge, i will be grateful to you.

Thanks alot.

Necip.

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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 23:14:34 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rangari0-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, September 24, 2004 at 22:21:53
---------------------------------------------------------------------------

Email: rangari0-at-yahoo.com
Name: vijay

Organization: tuskegee university

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi
Members
pl let me know where I can buying the glass knifes for microtoming.
Thanks

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From MicroscopyL-request-at-ns.microscopy.com Fri Sep 24 23:23:50 2004

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Jon

The header is a text field which describes how the data is formated.
You should be able to read the entire spectrum in any text editor.
XY columns is only one of many possible formats which are legal
forms for the data set to be output.

The program that is exporting the data into the MSA-MAS file format
should ask the individual how many columns and what format to export
the file into. It sounds like the person requested 4 column format. I'd suggest
that you read the header closely it should explain how the data is
output. You can then edit it as appropriate.

Alternatively have the data re-exported into XY format.

The details of the format can be found here:

http://www.amc.anl.gov/ANLSoftwareLibrary/02-EMMPDL/Xeds/EMMFF/

Nestor

Your Friendly Neighborhood SysOp

Title :EMSAMASFF
Keywords :XEDS,EELS,AES,WDS,CLS,GAM,XRF,PES
Computer :IBM, MAC, DEC
Operating System :ALL
Programming Language :Fortran 77
Hardware Requirements :None
Author(s) :EMSA/MAS TASK FORCE
Ray Egerton ,Charles E. Fiori ,John A. Hunt ,Mike S. Isaacson, Earl J. Kirkland ,Nestor J. Zaluzec
Correspondence Address : R.F. EGERTON CHAIRMAN
University of Alberta
Dept. of Physics
Alberta, Canada,
Abstract:

A simple format for the exchange of digital spectral data is
presented, and proposed as an EMSA/MAS standard. This format is readable by both humans and computers and is suitable for transmission through various electronic networks (BITNET, ARPANET), the phone system (with modems) or on physical computer storage
devices (such as floppy disks). The format is not tied to any one computer, programming language or computer operating system. The adoption of a standard format would enable different laboratories to freely exchange spectral data, and would help to standarize data
analysis software. If equipment manufacturers were to support a common format, the microscopy and microanalysis community would avoid duplicated effort in writing data-analysis software. This version of EMSAMASFF contains two subroutines which read and write spectral data files Version 1.0 data format. The data are stored as simple ASCII characters at a user defined number of columns per line for the length of the data file. The spectral data is preceeded by a series of header lines, which tell the user about the parameters of the spectrum. The header lines are identified by the first character in the line being the symbol (#) followed by a descriptor and if appropriate its units. An example of a data file format can be found in the EMSAMASFF.DOC file.

}
} Hi:
}
} Can anyone fill me in on the details of the EMSA file format for EDS spectra.
}
} Mostly I need to know how to help someone strip out the header so they can
} look at it in Excel.
}
} The file I see when I look at it has the header info, followed by what
} looks like 4 columns of numbers. I was expecting 2 columns, x and y. What's
} up?
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Sun Sep 26 10:59:11 2004

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Hi, Tim

There is a new technology coming from a company called AETOS which is probably just what you need. Contact Sam Lawrence at 334-749-0134. The technology is called "CytoViva". I had a chance to run it last week and was imaging particles at the 100nm level (I think a combo of both detection and resolution).

Hope this is helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education

We've Moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
F: 972-954-8018

^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&^&
Need a good general text on light microscopy? MME still has copies of Optimizing Light Microscopy available, with discounts for class-sized orders (10 or more). Visit www.MicroscopyEducation.com for details.

At 10:48 PM 9/24/2004, timandcathy-at-mho.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 06:42:23 2004

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Hi Todd,
I had a similar problems while cutting semi-thin sections. What I've
noticed it always happend after rough triming. I talked to Leica
representative and he expalained to me that the problem was how
I've been trimming blocks. I advanced knife towards the block and
always at the same time I moved the block in the specimen arm up
and down, but I was not making a full rotation with the wheel. He told
me that even though I do not rotate the specimen arm and it is not
advancing it builds up the distance, meaning that every time I
moved block up and down it advanced the specimen setting without
advancing it physically.( I am not sure if I explained well.) Then when
I switch to an automatic mode all this "build up" adds up and
microtome jumps the specimen forward cutting a big chunk. I
changed my method of trimming and I do not have any problems
anymore.
I hope my explanation will be of help to you.
Dorota

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 07:51:46 2004

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Greetings,
We are submitting a purchase requisition for an image capture system for
our SEM that has an older Microspec WDS spectrometer (pre-Oxford).
Due to budget requirements we are unable to upgrade the WDS system and
the need to capture the data stream from the spectrometer and bring it
into our image capture database is great.
Are there any suggestions to accomplish this capture of the data stream
from the spectrometer and bring it into the computer for further
processing?

Thanks for any help.
Robb

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 08:55:45 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 27, 2004 at 08:30:04
---------------------------------------------------------------------------

Email: kssim-at-mmu.edu.my
Name: kssim

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear all,

Can we do real-time signal-to-noise ratio value of SEM image ? What is the advantages after obtaining SNR value? If you have the solutions, please kindly email me.

Thanks
Ks

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From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 09:19:33 2004

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Hi all,

I just ran across this reference in our local newspaper about the care and
storage of CDs and DVDs. It is copublished by CLIR (Council on Library and
Information Resources) and NIST, so it should be reliable info.

http://www.clir.org/pubs/reports/pub121/contents.html

From my quick run through of the article, it appears that DVDs may be
inherently more stable than CDs.

Cheers,
Henk

Hendrik O. Colijn colijn.1-at-osu.edu
Campus Electron Optics Facility Ohio State University
(614) 292-0674 http://www.ceof.ohio-state.edu
Time is that quality of nature which keeps events from happening all at
once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 10:34:19 2004

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Hi all,
Despite pending budget cuts, I've been asked to submit an equipment
wish list. Go figure;-)
So wishfully thinking, I'd really like to hear your thoughts on the
various microwave ovens that are available from the EM supply
companies. Any great machines out there? Giving great results!
thanks in advance,
Beth

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 10:43:24 2004

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Hello Rob,

I am in a similar situation...
SEM: Hitachi S-3500H
EDS: IXRF Systems (Full)
WDS: Microspec 2A w/ Kevex Sesame24 Controller

My WDS controller has an analog ratemeter output for line scans and a
"digital" output for mapping. These signals are input to the "x-ray_1 and
x-ray_2 external inputs on the SEM. Maps and line scans are captured and
stored directly using Hitachi/Quartz software.
FWIW:
Image brightness/contrast manipulation may be required if your SEM works
like my Hitachi. In the mapping mode, I must use slow recursive imaging to
have sufficient integration time (other modes too fast) for most work. The
3500 software does not handle this gracefully. The finished map is usually
totally black because each "dot" luminosity is divided (I infer) by the
number of (recursive) passes and the data summed for presentation. Since
dots may not occur at the same exact location for each pass, they are too
dim to see. Thus, contrast/brightness expansion, using Photoshop, IrFan
View, or the like, is required to see the result. In the linescan mode
dynamic range is about half of what would be expected. The software limits
graphical amplitude excursions of half (or less) of the vertical range of
the crt image.

I often run "spectrum - scans" also, generating data (spectrum graphic)
within a limited wavelength range. My Sesame system has a serial data port
which will allow me to upload the wavelength positions and x-ray intensities
to my EDS PC. Any serial terminal program should work. The saved data can
be sent to a spreadsheet, or wherever.

If you have a 3PC? instead of the Kevex Sesame, I cannot be so specific...

Hope this is helpful.

Woody

-----Original Message-----
} From: Robb Westby [mailto:robbw-at-mxim.com]
Sent: Monday, September 27, 2004 8:51 AM
To: microscopy-at-msa.microscopy.com

Greetings,
We are submitting a purchase requisition for an image capture system for
our SEM that has an older Microspec WDS spectrometer (pre-Oxford).
Due to budget requirements we are unable to upgrade the WDS system and
the need to capture the data stream from the spectrometer and bring it
into our image capture database is great.
Are there any suggestions to accomplish this capture of the data stream
from the spectrometer and bring it into the computer for further
processing?

Thanks for any help.
Robb

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 11:06:06 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

I think there was an article in some magazine months ago on how
reliable CD-R are for archival. Depending on the brand (or no-brand if you
prefer) it can fail after less than 2 years. That was much less than the
20-100 years promised by the maker. People were recomending to use CD-RW
for archival purpose instead. Since it doesn't use a dye for recording the
data should be less affected by the problem. I suppose the same applies
for DVD+/-R and DVD+/-RW. Regards,

Carlos

On Mon, 27 Sep 2004, Hendrik O. Colijn wrote:

}
} Hi all,
}
} I just ran across this reference in our local newspaper about the care and
} storage of CDs and DVDs. It is copublished by CLIR (Council on Library and
} Information Resources) and NIST, so it should be reliable info.
}
} http://www.clir.org/pubs/reports/pub121/contents.html
}
} From my quick run through of the article, it appears that DVDs may be
} inherently more stable than CDs.
}
} Cheers,
} Henk
}
}

o-------------------------------------------------------o
| Carlos Kazuo Inoki |
| Department of Physics - University at Albany |
| 1400 Washington Ave.- Albany - NY - 12222 |
o-------------------------------------------------------o

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 12:26:47 2004

Contents Retrieved from Microscopy Listserver Archives
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Henk,

That's an extremely informative and useful article. Thank you!

It was interesting to learn that CD RW and DVD RW (bits encoded in metal structure
by a phase change from crystalline to amorphous) are less stable over time than CD
R and DVD R (bits encoded in degradable organic dyes). And that RW discs that are
"cycled" a lot (many re-writes) will degrade faster.

The best advice seems to be to use R (write once) discs (CD or DVD) and store them
vertically in a cool, low-light environment. Of course, transferring to fresh
media every year or so couldn't hurt...

Mike

"Hendrik O. Colijn" wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi all,
}
} I just ran across this reference in our local newspaper about the care and
} storage of CDs and DVDs. It is copublished by CLIR (Council on Library and
} Information Resources) and NIST, so it should be reliable info.
}
} http://www.clir.org/pubs/reports/pub121/contents.html
}
} From my quick run through of the article, it appears that DVDs may be
} inherently more stable than CDs.
}
} Cheers,
} Henk
}
} Hendrik O. Colijn colijn.1-at-osu.edu
} Campus Electron Optics Facility Ohio State University
} (614) 292-0674 http://www.ceof.ohio-state.edu
} Time is that quality of nature which keeps events from happening all at
} once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 12:54:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

} Name: John H. Cross, CIH
} Organization: Lockheed Martin Space Operations
} Title-Subject: [Microscopy] [Filtered] MListserver: Occupational
} Health Aspects of
} Microscope Usage
} Question: We have a group of technicians using microscopes to solder
} electronic
} components 10-12 hours per day 6-7 days a week.
}
} Does any professional, academic, or industry organization publish
} occupational health
} guidelines for the use of microscopes? A sample of questions I need
} to address are:
} How often must an individual take a break from looking through a microscope.
} Is exposure to light coming through the eyepieces a problem?
} Has anyone described ergonomically-correct work stations for microscopists?
}
} All comments will be welcome. I particularly need objective
} standards that I can present
} to management to justify work practice adjustments.
}
} John Cross
Email: John H. Cross-at-lmco.com
==============
John,
I am not aware of the reference that you requested. However now that
I am in my mid-50's ,
I recently have gotten several work related physical problems.

When I am using any scope for an extended period of time my eyes fail
to focus properly
for distance. This I first noticed after nearly a whole day on my
TEM, doing a lot of
scanning for a particular cell type in sections. When I left the
building for the night I
could not see properly anything that was more than a few yards in
front of me. I realized
that this had been happening over an extended period of time but it
was not so disturbing as
it had become. I consulted my eye doctor and he said that this was
not abnormal for people
my age. The eye muscles are not as elastic as they were a few years
ago hence they do not
snap back like they used to. I need to stop "scoping" every 15
minutes or so and give my
muscles a workout by focusing on a particular object in the distance
for a short while.
This has been working great for me after I got used to the short
interruptions and my concentration was improved because of the short
distraction from what can be very boring,
when what I am looking for is difficult to find.

A second problem is the nerve that goes through my elbow. Everyone
has heard of carpel
tunnel syndrome. There is a similar area in the elbow. The test for
this is to extend the
arms straight out to the front, at shoulder height with the backs of
the hands facing
upwards.
Make a fist, flex the wrist to raise just the fist upwards. If there
is no pain, it is OK,
but if you are truly having a problem the pain can be quite intense.
I would suggest that
one contact the doctor about this. My case was already very painful
when I went to the
doctor, thinking that it would get better itself - mistake! I
received several shots into the
area over an 8 week period because I can not take oral anti-inflammatory drugs.
I also had to do exercises several times a day to strengthen the
surrounding muscles.
In the mean time I took several older mouse-pads, cut them in half,
stacked them so that
my lower arm/elbow is at least as high as my hand when using the controls.
When using the hands to solder, one may just need more cushioning
under the elbow.
I have seen advertised scopes that claim to be more ergonomical but
at the moment
I can not recall the make.

If this is not already being done, I should expect that the fumes
from the solder should be
sucked away from the scope and go through a suitable filter so that
they are not inhaled
by the tech.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 13:16:21 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear John,
I am the Ergonomics Representative for our department at UBC and the
guidelines I was given for people working at computer terminals all day was:
a one minute break every ten minutes and a ten-minute break every hour. The
short break was just to ease the eye strain of looking at a fixed focus for
extended periods and just consists of focussing out the window or at a
longer distance and relaxing arms, hands, neck, etc. The longer hour break
was to stand up, stretch, move around and relax. These were just a
guideline. There are also things about the setup to check, such as the angle
of arms, wrists, hips, knees, the height of chair and height of monitor.
Your case is special, but you should be able to work out, with the people
doing the work, a checklist of things to adjust to make the work
ergonomically sound or as least-damaging as possible. Good support chairs
with lots of adjustment, microscopes that can adjust eyepiece spacing,
armrests are just some of the things that might help.
The light coming from the microscope should not be a problem, but should be
controlled by the user so it can be adjusted to a comfortable level. The
breaks are important to relieve eye-strain.
Good luck,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "by way of MicroscopyListserver" {John.H.Cross-at-lmco.com}
To: {microscopy-at-microscopy.com}
Sent: Friday, September 24, 2004 6:08 AM

Pat;

Have you tried contacting OSHA [Occupational Safety and Health
Aministration]? OSHA is a US Gov't agency. http://www.osha.gov

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Pat Connelly [mailto:psconnel-at-sas.upenn.edu]
Sent: Monday, September 27, 2004 1:54 PM
To: by way of MicroscopyListserver
Cc: microscopy-at-msa.microscopy.com

} Name: John H. Cross, CIH
} Organization: Lockheed Martin Space Operations
} Title-Subject: [Microscopy] [Filtered] MListserver: Occupational
} Health Aspects of
} Microscope Usage
} Question: We have a group of technicians using microscopes to solder
} electronic
} components 10-12 hours per day 6-7 days a week.
}
} Does any professional, academic, or industry organization publish
} occupational health guidelines for the use of microscopes? A sample of

} questions I need to address are:
} How often must an individual take a break from looking through a
microscope.
} Is exposure to light coming through the eyepieces a problem?
} Has anyone described ergonomically-correct work stations for
microscopists?
}
} All comments will be welcome. I particularly need objective standards
} that I can present to management to justify work practice adjustments.
}
} John Cross
Email: John H. Cross-at-lmco.com
==============
John,
I am not aware of the reference that you requested. However now that
I am in my mid-50's ,
I recently have gotten several work related physical problems.

When I am using any scope for an extended period of time my eyes fail
to focus properly
for distance. This I first noticed after nearly a whole day on my
TEM, doing a lot of
scanning for a particular cell type in sections. When I left the
building for the night I
could not see properly anything that was more than a few yards in
front of me. I realized
that this had been happening over an extended period of time but it
was not so disturbing as
it had become. I consulted my eye doctor and he said that this was
not abnormal for people
my age. The eye muscles are not as elastic as they were a few years
ago hence they do not
snap back like they used to. I need to stop "scoping" every 15
minutes or so and give my
muscles a workout by focusing on a particular object in the distance
for a short while.
This has been working great for me after I got used to the short
interruptions and my concentration was improved because of the short
distraction from what can be very boring,
when what I am looking for is difficult to find.

A second problem is the nerve that goes through my elbow. Everyone
has heard of carpel
tunnel syndrome. There is a similar area in the elbow. The test for
this is to extend the
arms straight out to the front, at shoulder height with the backs of
the hands facing
upwards.
Make a fist, flex the wrist to raise just the fist upwards. If there
is no pain, it is OK,
but if you are truly having a problem the pain can be quite intense.
I would suggest that
one contact the doctor about this. My case was already very painful
when I went to the
doctor, thinking that it would get better itself - mistake! I
received several shots into the
area over an 8 week period because I can not take oral anti-inflammatory
drugs. I also had to do exercises several times a day to strengthen the
surrounding muscles.
In the mean time I took several older mouse-pads, cut them in half,
stacked them so that
my lower arm/elbow is at least as high as my hand when using the
controls. When using the hands to solder, one may just need more
cushioning
under the elbow.
I have seen advertised scopes that claim to be more ergonomical but
at the moment
I can not recall the make.

If this is not already being done, I should expect that the fumes
from the solder should be
sucked away from the scope and go through a suitable filter so that
they are not inhaled
by the tech.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 15:38:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

John,

Try these websites. Maybe they will help you.

http://www.office-ergo.com/
http://www.niehs.nih.gov/odhsb/ergoguid/home.htm
http://www.dehs.umn.edu/ergo/lab/
http://www.osha.gov/SLTC/laboratories/index.html

I will also send you a ppt-presentation that I did for a lab 'safety'
meeting.

Kelly A. Ramos
Metallurgical Engineer / Supervisor
Argo-Tech Materials Laboratories
23555 Euclid Avenue
Cleveland, OH 44117
216-692-5904 or 216-692-5446
(fax) 216-692-5816
http://www.atclabs.com

****************************************************************

JOHN WROTE:
------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

} Name: John H. Cross, CIH
} Organization: Lockheed Martin Space Operations
} Title-Subject: [Microscopy] [Filtered] MListserver: Occupational
} Health Aspects of
} Microscope Usage
} Question: We have a group of technicians using microscopes to solder
} electronic
} components 10-12 hours per day 6-7 days a week.
}
} Does any professional, academic, or industry organization publish
} occupational health
} guidelines for the use of microscopes? A sample of questions I need
} to address are:
} How often must an individual take a break from looking through a
microscope.
} Is exposure to light coming through the eyepieces a problem?
} Has anyone described ergonomically-correct work stations for
microscopists?
}
} All comments will be welcome. I particularly need objective
} standards that I can present
} to management to justify work practice adjustments.
}
} John Cross
Email: John H. Cross-at-lmco.com

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 19:50:02 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear all;

Can someone tell me if such a data base exist? I am hoping to get
information on rates and annual budget of university EM facilities in
the US. Specifically, I am hoping to know the percentage of charge
based income vs. university support. If there is not such a data base,
would you EM facility directors mind emailing me and giving me some
idea about the case in your facility. Thank you all very much in
advance.

Hong
Emory EM.

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 20:56:57 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (walter.bobrowski-at-pfizer.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 27, 2004 at 15:31:59
---------------------------------------------------------------------------

Email: walter.bobrowski-at-pfizer.com
Name: Walt Bobrowski

Organization: Pfizer Global R&D

Title-Subject: [Microscopy] [Filtered] Osmium Substitutions

Question: A colleague is asking if anyone has permanently removed buffered osmium tetroxide out of the routine processing of mammalian tissues for EM, and substituted with another, equally good reagent? I thought it was still the standard post-fix, but maybe I'm behind the times! TIA.

Walt

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Sep 27 20:58:00 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mdawes-at-scu.edu.au) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, September 27, 2004 at 19:33:49
---------------------------------------------------------------------------

Email: mdawes-at-scu.edu.au
Name: Maxine Dawes

Organization: Southern Cross University

Title-Subject: [Microscopy] [Filtered] Fluorochrome stain - Light Microscope

Question: We have a Reflected light fluorescence attachment CX-RFL which fits onto our Olympus Compound microscope CX 40. The Cube Dichroic Mirror/Filter combinations are: a). CX-DMB (Mirror cube), Exciter filter BP475, Barrier filter 05151F and b). CX-DMG (Mirror cube), Exciter filter BP545, Barrier filter 0590. My question is:
We are trying to stain some pollen tubes to photograph the pollen tube growth - all papers that I have read seem to use the fluorescing stain Analine Blue which stains the cellulose ń we do not have a Mirror cube to view this stain and after doing some research with our suppliers we cannot use Aniline blue with the set up we have. We can use the fluorochrome FITC . As there seem to be several stains Fluoresceine diacetate FDA (which appears to stain for protein) and Fluoresceine isothiocyanates FITC (which also appears to stain for protein), my question is can we use either of these stains with our system to photograph pollen tube growth and which one is the easier of the two and is there a tried and tested procedure that someone might be willing to share with us.

Regards
Maxine

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 03:13:37 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I´m worried about my health too.
My question: Is there any harmful radiation working with
JEOL 100-S electron microscope?

Kärt Padari
University of Tartu
kartp-at-ut.ee

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 03:20:12 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I´m worried about my health too.
My question: Is there any harmful radiation working with
JEOL 100-S electron microscope?

Kärt Padari
University of Tartu
kartp-at-ut.ee

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 04:39:52 2004

Contents Retrieved from Microscopy Listserver Archives
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Torino 28 September 2004
(ITALY)

Hi all,

Does anyone have an experience or some information about how to realize a sharp cutting edge by hand working an iron piece?
I’d like to use it for cutting wax in an hand microtome.
I’d like to know the cutting angle, the abrasive powders to use and the operating steps.
Thank you.
Kindly Regards,

Massimo

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 08:19:14 2004

Contents Retrieved from Microscopy Listserver Archives
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Maxine,
It was probably a typo in your post, but analine blue stains
callose (as well as some other polysaccharides), not cellulose. You
probably also know that Biosupplies in Mebourne sells a cleaned up
version of the dye called Sirofluor that is more speciific for
callose, and often gives nicer images, but is still uv excited.

Have you tried imaging analine blue stained stuff with your
blue cube? It just might work--I think that analine blue has a pretty
broad excitation spectrum.

HTH,
Tobias

}
}
} Email: mdawes-at-scu.edu.au
} Name: Maxine Dawes
}
} Organization: Southern Cross University
}
} Title-Subject: [Microscopy] [Filtered] Fluorochrome stain - Light Microscope
}
} Question: We have a Reflected light fluorescence attachment CX-RFL
} which fits onto our Olympus Compound microscope CX 40. The Cube
} Dichroic Mirror/Filter combinations are: a). CX-DMB (Mirror cube),
} Exciter filter BP475, Barrier filter 05151F and b). CX-DMG (Mirror
} cube), Exciter filter BP545, Barrier filter 0590. My question is:
} We are trying to stain some pollen tubes to photograph the pollen
} tube growth - all papers that I have read seem to use the
} fluorescing stain Analine Blue which stains the cellulose ń we do
} not have a Mirror cube to view this stain and after doing some
} research with our suppliers we cannot use Aniline blue with the set
} up we have. We can use the fluorochrome FITC . As there seem to be
} several stains Fluoresceine diacetate FDA (which appears to stain
} for protein) and Fluoresceine isothiocyanates FITC (which also
} appears to stain for protein), my question is can we use either of
} these stains with our system to photograph pollen tube growth and
} which one is the easier of the two and is there a tried and tested
} procedure that someone might be willing to share with us.
}
} Regards
} Maxine
}
}
} ---------------------------------------------------------------------------

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 08:20:03 2004

Contents Retrieved from Microscopy Listserver Archives
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Your service engineer should monitor radiation leaking
during operation. After 23yrs our SEM has just started to
leak (at 30kV only). I am having a lead shield fitted to
block the leak.

Dave

On Tue, 28 Sep 2004 11:21:35 +0300 (EEST) Kart Padari
{kartp-at-ut.ee} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
}
} I´m worried about my health too.
} My question: Is there any harmful radiation working with
} JEOL 100-S electron microscope?
}
} Kärt Padari
} University of Tartu
} kartp-at-ut.ee
}
}
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 08:45:09 2004

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Hong,
You can see the rates for my 2 facilities (EM and Optical Microscopy)
on the school's website at:
http://www.med.cornell.edu/research/cores/index.html

We are subsidized by the College to help cover staff salaries, we are
not charged "overhead" costs. Otherwise, the 2 facilities that I'm
involved with cover all other costs.

Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 09:10:54 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Kärt Padari wrote:
=====================================================
I´m worried about my health too.
My question: Is there any harmful radiation working with
JEOL 100-S electron microscope?
=====================================================
My first exposure to an EM was in 1963, the round screen "horizontal"
Philips 100 TEM. I was told (but don't know from my own knowledge that
this was true) that some of these earliest models were manufactured with
ordinary instead of lead glass. I also had contact with an early RCA TEM,
I think it was an EMU-1 (or something close to that). Those are the only two
EMs I have ever heard about that had inherent radiation problems and once
the problem was recognized, retrofits were installed, taking away the
problems. I have met operators of those early RCA instruments who
literally did their work wearing a lead apron. My sense if that there are
none of these old generation EMs in use any more.

Instruments manufactured after that era were designed such that the mass of
the column itself would be sufficiently massive and absorbing of x-rays,
that raditation just could not escape during operation. True, one could
envision that a column could be sufficiently misaligned that x-rays could
possibly get out, but the instruments seem to be designed in a way that if
they really were misaligned by that extent, there would be a vacuum leak and
the high voltage would automatically shut down. Some very many years ago,
we tried this with a JEOL 100CX and could not get the microscope
sufficiently misaligned to allow x-rays to get out. With a JSM-U3 SEM, at
that same time, the column would lose vacuum before it could be misaligned
sufficiently to allow x-rays to come through.

But there are at least several circumstances in which radiation can escape:

a) Someone breaks the lead glass viewing screen of a TEM and thinking they
are saving money, replaces the broken glass with ordinary glass. I have
heard of this very thing happening, on occasion over the years. Such a
replacement of the glass would be picked up instantly during any kind of a
radiation survey, however. Without such a survey, it is not possible to
differentiate, by appearance, lead vs. non-lead glass.

b) Adjustment knobs for the lenses seem to be slightly (x-ray) "leaky" in
some instruments, but the exposure is localized to the area of the knobs,
and therefore also to the fingers. With modern instruments where this is
done by the computer, this risk is much less and might no longer be present.
I have heard of people wrapping lead foil around their several fingers when
adjusting the knobs but I don't know if that is necessarily a "recommended"
procedure. But a general room survey would not necessarily reveal this
exposure risk.

c) Home made or radically altered commercial instruments which do not have
the "safety engineering" built into them that would otherwise be found in a
commerical instrument. I have always thought that this type of instrument
should be surveyed quite frequently because of the frequency that changes
seem to be made to the basic instrument.

Much of the motivation for those who do radiation surveys involving
commercially purchase instruments is to protect the organization from
lawsuits from former or present employees who make the claim that some
medical condition was either caused or aggrivated by their operation of
their TEM or SEM. Considering all the persons who have used both SEMs and
TEMs over the years, if there was some health issue, I would have thought
that it would have shown up clinically by now. When considering all the
risks in an EM loboratory, I have always thought that exposure to the
embedding resin chemicals would represent a far greater health risk than
operating a column instrument.

This is a very important topic and if there are other perspectives on this,
I would surely like to hear them.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 10:15:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I would hope that these rates are not for the general public and are
restricted to in-house use. Those of us in the private commercial labs are
not subsidized by our own tax dollars. This is always an issue for us with
faculty taking on outside work and using school resources.

My $0.02 as a local professor was soliciting his services only
yesterday's. My associate was a upset with the lack of awareness and
sensitivity to the unfair tax advantage.

Alan Stone
ASTON

At 08:45 AM 9/28/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 10:43:01 2004

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Dave,
Could you please elaborate? I'm having a little trouble imagining what
could change (other than physical modifications) that would allow leakage.

Is the newest survey perhaps simply more sensitive than previous surveys?

What brand and model?

Where has it started leaking?

What kind of intensity?

I service a lot of older scopes (as much as 10 years older than yours) and
need to know if this should be more closely watched.

Thanks for your time and help.

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

-----Original Message-----
} From: Patton, David [mailto:David.Patton-at-uwe.ac.uk]
Sent: Tuesday, September 28, 2004 9:20 AM
To: Kart Padari
Cc: microscopy-at-msa.microscopy.com

Your service engineer should monitor radiation leaking
during operation. After 23yrs our SEM has just started to
leak (at 30kV only). I am having a lead shield fitted to
block the leak.

Dave

On Tue, 28 Sep 2004 11:21:35 +0300 (EEST) Kart Padari
{kartp-at-ut.ee} wrote:

}
}
}
----------------------------------------------------------------------------
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
}
}
} I´m worried about my health too.
} My question: Is there any harmful radiation working with
} JEOL 100-S electron microscope?
}
} Kärt Padari
} University of Tartu
} kartp-at-ut.ee
}
}
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and
any virus detected has been removed using McAfee anti-virus software

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected
has been removed using McAfee anti-virus software

___________________________________________________________
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From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 10:54:28 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dave,
Could you please elaborate? I'm having a little trouble imagining what
could change (other than physical modifications) that would allow leakage.

Is the newest survey perhaps simply more sensitive than previous surveys?

What brand and model?

Where has it started leaking?

What kind of intensity?

I service a lot of older scopes (as much as 10 years older than yours) and
need to know if this should be more closely watched.

Thanks for your time and help.

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

-----Original Message-----
} From: Patton, David [mailto:David.Patton-at-uwe.ac.uk]
Sent: Tuesday, September 28, 2004 9:20 AM
To: Kart Padari
Cc: microscopy-at-msa.microscopy.com

Your service engineer should monitor radiation leaking
during operation. After 23yrs our SEM has just started to
leak (at 30kV only). I am having a lead shield fitted to
block the leak.

Dave

On Tue, 28 Sep 2004 11:21:35 +0300 (EEST) Kart Padari
{kartp-at-ut.ee} wrote:

}
}
}
----------------------------------------------------------------------------
--
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
---
}
}
}
} I´m worried about my health too.
} My question: Is there any harmful radiation working with
} JEOL 100-S electron microscope?
}
} Kärt Padari
} University of Tartu
} kartp-at-ut.ee
}
}
}
}
}
}
} This incoming email to UWE has been independently scanned for viruses and
any virus detected has been removed using McAfee anti-virus software

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected
has been removed using McAfee anti-virus software

___________________________________________________________
$0 Web Hosting with up to 120MB web space, 1000 MB Transfer
10 Personalized POP and Web E-mail Accounts, and much more.
Signup at www.doteasy.com

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 12:36:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Alan, and others
My rates are for grant-funded "in house" personnel...we add a
whopping surcharge to outside users to compensate for the fact that
they don't contribute to the overhead costs of the College as do our
grant-funded people.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 13:00:53 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Leona,

Thank you for clarifying that.

Alan

At 12:37 PM 9/28/2004, you wrote:
} Alan, and others
} My rates are for grant-funded "in house" personnel...we add a whopping
} surcharge to outside users to compensate for the fact that they don't
} contribute to the overhead costs of the College as do our grant-funded people.
} Lee
} --
} Leona Cohen-Gould, M.S.
} Sr. Staff Associate
} Director, Electron Microscopy Core Facility
} Manager, Optical Microscopy Core Facility
} Joan & Sanford I. Weill Medical College
} of Cornell University
} voice (212)746-6146
} fax (212)746-8175

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 13:58:37 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Sep 28, 2004, at 1:12 AM, Kart Padari wrote:

} IŽm worried about my health too.
} My question: Is there any harmful radiation working with
} JEOL 100-S electron microscope?
}
Dear Kärt,
There should not be any radiation problems; however, not all EMs have
been properly maintained, so it is best to check. The best ways are to
use a hand-held ion chamber detector to survey the area while the scope
is operated in the most extreme conditions, such as putting a Pt
aperture in the stage and hitting the aperture with the most intense
beam you can produce, moving the shift and tilt controls through the
full extent of their range, etc. Another way is to place film badges
or thermoluminescent detectors around the room and measure the
background on a month-by-month schedule. You should decide where a
radiation leak is most likely by looking at the location of shielding
pieces and thin spots in the column wall, and you need to measure the
areas where a radiation leak, however unlikely, would do the most
damage--obviously where the operator sits, where specimens are loaded,
or anywhere that someone is expected to spend a fair amount of time.
Remember that x-rays can penetrate walls and floors, so check for
radiation that could harm someone in the lab above, below, across the
hall, or other possible locations. Thick concrete is a much better
shielding material than wood or sheet metal, so more care is required,
if your scope is surrounded by the latter. Take the time to make this
check, then you will be able to operate with greater peace of mind.
Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 16:43:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (donaldawbrey-at-texashealth.org) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, September 28, 2004 at 09:22:18
---------------------------------------------------------------------------

Email: donaldawbrey-at-texashealth.org
Name: Donald G. Awbrey HT(ASCP) QIHC

Organization: Harris Methodist Hospital

Title-Subject: [Microscopy] [Filtered] TEM Laser Printer

Question: Dear Micro netters,

We are looking for a high resolution printer for our TEM workstation.
I've seen monochrome lazer printers that have a 1200 X 1200 dpi
resolution. Our digital camera will be a 2K camera. Will this
printer print photos of diagnostic quality? Or would we have to go
with a dye sublimation printer? I've noticed that these sub printers
are very expensive, but have a "spatial" resolution of around 320
dpi. Is this the same as regular resolution? If so, then the laser
printer would have better resolution. This does not make sense. Is
1200 X 1200 dpi good enough for CAP inspection.

Any information on diagnostic quality printers for TEM will be
greatfully appreciated.

Thank you in advance.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 17:38:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Chuck;
Chuck;
When I was in grad school, we purchased a used JSM-U3 through JEOL that had been in previous use at the GM tech center. The stage door was EXTREMELY leaky under normal use conditions (it was different than our other JSM-U3). I eventually installed a lead lining in the door.

John Mardinly
Intel

-----Original Message-----
} From: Garber, Charles A. [mailto:cgarber-at-2spi.com]
Sent: Tuesday, September 28, 2004 8:12 AM
To: MICROSCOPY BB

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Kärt Padari wrote:
=====================================================
I´m worried about my health too.
My question: Is there any harmful radiation working with
JEOL 100-S electron microscope?
=====================================================
My first exposure to an EM was in 1963, the round screen "horizontal"
Philips 100 TEM. I was told (but don't know from my own knowledge that
this was true) that some of these earliest models were manufactured with
ordinary instead of lead glass. I also had contact with an early RCA TEM,
I think it was an EMU-1 (or something close to that). Those are the only two
EMs I have ever heard about that had inherent radiation problems and once
the problem was recognized, retrofits were installed, taking away the
problems. I have met operators of those early RCA instruments who
literally did their work wearing a lead apron. My sense if that there are
none of these old generation EMs in use any more.

Instruments manufactured after that era were designed such that the mass of
the column itself would be sufficiently massive and absorbing of x-rays,
that raditation just could not escape during operation. True, one could
envision that a column could be sufficiently misaligned that x-rays could
possibly get out, but the instruments seem to be designed in a way that if
they really were misaligned by that extent, there would be a vacuum leak and
the high voltage would automatically shut down. Some very many years ago,
we tried this with a JEOL 100CX and could not get the microscope
sufficiently misaligned to allow x-rays to get out. With a JSM-U3 SEM, at
that same time, the column would lose vacuum before it could be misaligned
sufficiently to allow x-rays to come through.

But there are at least several circumstances in which radiation can escape:

a) Someone breaks the lead glass viewing screen of a TEM and thinking they
are saving money, replaces the broken glass with ordinary glass. I have
heard of this very thing happening, on occasion over the years. Such a
replacement of the glass would be picked up instantly during any kind of a
radiation survey, however. Without such a survey, it is not possible to
differentiate, by appearance, lead vs. non-lead glass.

b) Adjustment knobs for the lenses seem to be slightly (x-ray) "leaky" in
some instruments, but the exposure is localized to the area of the knobs,
and therefore also to the fingers. With modern instruments where this is
done by the computer, this risk is much less and might no longer be present.
I have heard of people wrapping lead foil around their several fingers when
adjusting the knobs but I don't know if that is necessarily a "recommended"
procedure. But a general room survey would not necessarily reveal this
exposure risk.

c) Home made or radically altered commercial instruments which do not have
the "safety engineering" built into them that would otherwise be found in a
commerical instrument. I have always thought that this type of instrument
should be surveyed quite frequently because of the frequency that changes
seem to be made to the basic instrument.

Much of the motivation for those who do radiation surveys involving
commercially purchase instruments is to protect the organization from
lawsuits from former or present employees who make the claim that some
medical condition was either caused or aggrivated by their operation of
their TEM or SEM. Considering all the persons who have used both SEMs and
TEMs over the years, if there was some health issue, I would have thought
that it would have shown up clinically by now. When considering all the
risks in an EM loboratory, I have always thought that exposure to the
embedding resin chemicals would represent a far greater health risk than
operating a column instrument.

This is a very important topic and if there are other perspectives on this,
I would surely like to hear them.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 17:43:58 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Peter;
I'm not sure what good OSHA is. They require records of film
badges to be kept for 30 years but don't require film badges, so guess
what my employer did? They elimininated film badges!

John Mardinly
Intel

-----Original Message-----
} From: Tomic, Peter (Peter) [mailto:ptomic-at-agere.com]
Sent: Monday, September 27, 2004 12:06 PM
To: Pat Connelly; by way of MicroscopyListserver
Cc: microscopy-at-msa.microscopy.com

Pat;

Have you tried contacting OSHA [Occupational Safety and Health
Aministration]? OSHA is a US Gov't agency. http://www.osha.gov

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Pat Connelly [mailto:psconnel-at-sas.upenn.edu]
Sent: Monday, September 27, 2004 1:54 PM
To: by way of MicroscopyListserver
Cc: microscopy-at-msa.microscopy.com

} Name: John H. Cross, CIH
} Organization: Lockheed Martin Space Operations
} Title-Subject: [Microscopy] [Filtered] MListserver: Occupational
} Health Aspects of
} Microscope Usage
} Question: We have a group of technicians using microscopes to solder
} electronic
} components 10-12 hours per day 6-7 days a week.
}
} Does any professional, academic, or industry organization publish
} occupational health guidelines for the use of microscopes? A sample of

} questions I need to address are:
} How often must an individual take a break from looking through a
microscope.
} Is exposure to light coming through the eyepieces a problem?
} Has anyone described ergonomically-correct work stations for
microscopists?
}
} All comments will be welcome. I particularly need objective standards
} that I can present to management to justify work practice adjustments.
}
} John Cross
Email: John H. Cross-at-lmco.com
==============
John,
I am not aware of the reference that you requested. However now that
I am in my mid-50's ,
I recently have gotten several work related physical problems.

When I am using any scope for an extended period of time my eyes fail
to focus properly
for distance. This I first noticed after nearly a whole day on my
TEM, doing a lot of
scanning for a particular cell type in sections. When I left the
building for the night I
could not see properly anything that was more than a few yards in
front of me. I realized
that this had been happening over an extended period of time but it
was not so disturbing as
it had become. I consulted my eye doctor and he said that this was
not abnormal for people
my age. The eye muscles are not as elastic as they were a few years
ago hence they do not
snap back like they used to. I need to stop "scoping" every 15
minutes or so and give my
muscles a workout by focusing on a particular object in the distance
for a short while.
This has been working great for me after I got used to the short
interruptions and my concentration was improved because of the short
distraction from what can be very boring,
when what I am looking for is difficult to find.

A second problem is the nerve that goes through my elbow. Everyone
has heard of carpel
tunnel syndrome. There is a similar area in the elbow. The test for
this is to extend the
arms straight out to the front, at shoulder height with the backs of
the hands facing
upwards.
Make a fist, flex the wrist to raise just the fist upwards. If there
is no pain, it is OK,
but if you are truly having a problem the pain can be quite intense.
I would suggest that
one contact the doctor about this. My case was already very painful
when I went to the
doctor, thinking that it would get better itself - mistake! I
received several shots into the
area over an 8 week period because I can not take oral anti-inflammatory
drugs. I also had to do exercises several times a day to strengthen the
surrounding muscles.
In the mean time I took several older mouse-pads, cut them in half,
stacked them so that
my lower arm/elbow is at least as high as my hand when using the
controls. When using the hands to solder, one may just need more
cushioning
under the elbow.
I have seen advertised scopes that claim to be more ergonomical but
at the moment
I can not recall the make.

If this is not already being done, I should expect that the fumes
from the solder should be
sucked away from the scope and go through a suitable filter so that
they are not inhaled
by the tech.

Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Sep 28 21:56:08 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Chuck's mention of the horizontal Philips 100 TEM brought to mind a story
that very likely was true. At the beginning of my microscopy career I
worked in the lab of Humberto Fernandez-Moran (of pointed filament and
diamond knife fame). Moran started using TEMS in Europe in the late 40's
including working on the earliest versions of the Philips 100 TEM. He had a
a large scar on his nose from surgery to remove a skin cancer. He blamed
the cancer on long hours with his face pressed close to the unleaded window
of the TEM and the resultant exposure to x-rays. Being rather sensitive to
this problem, he was quite careful to have later instruments tested. When I
worked in his lab we had Siemens Elmiskop 1 and 1a TEMs that tested fine.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 9/28/04 5:39 PM, "Mardinly, John" {john.mardinly-at-intel.com} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} Chuck;
} Chuck;
} When I was in grad school, we purchased a used JSM-U3 through JEOL that had
} been in previous use at the GM tech center. The stage door was EXTREMELY leaky
} under normal use conditions (it was different than our other JSM-U3). I
} eventually installed a lead lining in the door.
}
} John Mardinly
} Intel
}
} -----Original Message-----
} } From: Garber, Charles A. [mailto:cgarber-at-2spi.com]
} Sent: Tuesday, September 28, 2004 8:12 AM
} To: MICROSCOPY BB
} Subject: [Microscopy] Safety around a column instrument
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
------------------------------------------------------------------------------}
-
}
} -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
}
} Kärt Padari wrote:
} =====================================================
} I´m worried about my health too.
} My question: Is there any harmful radiation working with
} JEOL 100-S electron microscope?
} =====================================================
} My first exposure to an EM was in 1963, the round screen "horizontal"
} Philips 100 TEM. I was told (but don't know from my own knowledge that
} this was true) that some of these earliest models were manufactured with
} ordinary instead of lead glass. I also had contact with an early RCA TEM,
} I think it was an EMU-1 (or something close to that). Those are the only two
} EMs I have ever heard about that had inherent radiation problems and once
} the problem was recognized, retrofits were installed, taking away the
} problems. I have met operators of those early RCA instruments who
} literally did their work wearing a lead apron. My sense if that there are
} none of these old generation EMs in use any more.
}
} Instruments manufactured after that era were designed such that the mass of
} the column itself would be sufficiently massive and absorbing of x-rays,
} that raditation just could not escape during operation. True, one could
} envision that a column could be sufficiently misaligned that x-rays could
} possibly get out, but the instruments seem to be designed in a way that if
} they really were misaligned by that extent, there would be a vacuum leak and
} the high voltage would automatically shut down. Some very many years ago,
} we tried this with a JEOL 100CX and could not get the microscope
} sufficiently misaligned to allow x-rays to get out. With a JSM-U3 SEM, at
} that same time, the column would lose vacuum before it could be misaligned
} sufficiently to allow x-rays to come through.
}
}
} But there are at least several circumstances in which radiation can escape:
}
} a) Someone breaks the lead glass viewing screen of a TEM and thinking they
} are saving money, replaces the broken glass with ordinary glass. I have
} heard of this very thing happening, on occasion over the years. Such a
} replacement of the glass would be picked up instantly during any kind of a
} radiation survey, however. Without such a survey, it is not possible to
} differentiate, by appearance, lead vs. non-lead glass.
}
} b) Adjustment knobs for the lenses seem to be slightly (x-ray) "leaky" in
} some instruments, but the exposure is localized to the area of the knobs,
} and therefore also to the fingers. With modern instruments where this is
} done by the computer, this risk is much less and might no longer be present.
} I have heard of people wrapping lead foil around their several fingers when
} adjusting the knobs but I don't know if that is necessarily a "recommended"
} procedure. But a general room survey would not necessarily reveal this
} exposure risk.
}
} c) Home made or radically altered commercial instruments which do not have
} the "safety engineering" built into them that would otherwise be found in a
} commerical instrument. I have always thought that this type of instrument
} should be surveyed quite frequently because of the frequency that changes
} seem to be made to the basic instrument.
}
}
} Much of the motivation for those who do radiation surveys involving
} commercially purchase instruments is to protect the organization from
} lawsuits from former or present employees who make the claim that some
} medical condition was either caused or aggrivated by their operation of
} their TEM or SEM. Considering all the persons who have used both SEMs and
} TEMs over the years, if there was some health issue, I would have thought
} that it would have shown up clinically by now. When considering all the
} risks in an EM loboratory, I have always thought that exposure to the
} embedding resin chemicals would represent a far greater health risk than
} operating a column instrument.
}
} This is a very important topic and if there are other perspectives on this,
} I would surely like to hear them.
}
} Chuck
}
} ===================================================
} Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
} President 1-(800)-2424-SPI
} SPI SUPPLIES FAX: 1-(610)-436-5755
} PO BOX 656 e-mail: cgarber-at-2spi.com
} West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com
}
}
} Look for us!
} ############################
} WWW: http://www.2spi.com
} ############################
} ==================================================
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 01:00:02 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

As has been mentioned previously on this listserver, at first nearly every
state, if not all of them, required regular surveys of EMs. This was
sparked by at least one manufacturer that released some TEMs with
non-leaded glass (problems mainly restricted to the facial area) and I
believe at least one other instance of TEM camera assemblies that leaked (a
number of early TEM operators took to clipping their film badges over their
genitals). Over the years, most states have dropped this requirement as
few surveys ever detect anything. However, a good knowledge of the
potential radiation and the detecting methods used is really required.

Any change in radiation leakage in an EM over time is probably an
indication that either something has been improperly changed in the EM or
the instruments being used to detect a problem have changed.

In the first case, the basic design of a modern EM (and by that I mean
anything produced in the last 30 years) makes them inherently safe in most
respects. The standard design of shrouding electromagnetic lenses in soft
iron (ferromagnetics) in order to use those shrouds to focus the fields in
narrow spaces means that the majority of the column is well shielded. In
areas where these lenses aren't used, the outer structures are very thick
metal just to support the electron gun or upper lenses and keep them in
alignment. Where these sections are mated, they normally have close
fitting, concentric overlaps for alignment. In other sealing areas, such
as vacuum manifolds, gauges, port covers and door seals, sufficient overlap
is provided to prevent a direct path for x-rays.

For example, a flat door with an o-ring sealing up against flat metal
chamber in an SEM generally has a half an inch to an inch of overlap. Yes,
x-rays will leak, but due to the repeated, zigzag path they would have to
take to get out, you won't see primary x-rays. Instead, you will get the
result of multiple fluorescence events, with each generation producing
x-rays of lower energy and fewer photons that can make it out. There
could, however, be structures within the chamber that are always, or
occasionally, in the right position to provide a fluorescence to the
primary sample x-rays with a portion going directly out between the door
and the chamber, through the o-ring.

That brings us to the equipment used to detect these leaks. Geiger tubes
of various shapes and sizes have been the standard over the years. There
are two general varieties - compensated and uncompensated. The
uncompensated tube is a bare tube. Because of the design, the
uncompensated Geiger tube is extremely sensitive to x-rays, the lower the
energy the more it reports. As long as some x-rays can penetrate the outer
glass tube, or cause a secondary fluorescence in it, the lower energy
x-rays stand a much better chance of ionizing the gas within.

Because a wide range of radiation detection is desired for most Geiger
counters, various means are used to 'compensate' them. This basically
means shielding them from lower energy x-rays so that they aren't swamped
by them and thus higher energy x-rays and gamma rays can be more
effectively detected. Other types of radiation detectors can have a
response similar to the uncompensated Geiger tube - they can be far more
sensitive to low energy x-rays than other radiation, but they are often
calibrated to high energy x-rays or gamma rays (the most interesting form
of radiation detection for many uses) and perhaps compensated in some way.

Leaving the technical behind, a change over time in the x-ray emissions of
an EM could also be the result of a change in instrumentation to detect it.
If the detector doesn't have a linear calibration that includes the low
x-ray energies, then it may produce results on an EM that don't represent
reality. Since most survey instruments can't differentiate radiation
sources by energy, appropriate adjustment has to be made to their readings.
An SEM running at 30KV won't leak 30KV x-rays, and if that assumption is
made the reading will be off. More than likely any emitted radiation would
be an order of magnitude or more lower in energy. At those energies, the
survey meter would likely have a much different sensitivity, perhaps
several orders of magnitude.

In regards to vacuum integrity, generally an instrument column misaligned
enough to allow x-ray leakage from the column would not be capable of
maintaining a vacuum and thus the instrument would itself prevent the
application of the electron beam. Avoiding the issue of properly operating
vacuum interlocks, I confess I can think of an instrument or two that could
have such misalignments and still operate. These would be visibly obvious
to anyone familiar with the instrument and extremely unlikely to occur even
from the most inexperienced service personnel. Yet, the possibility
exists.

User modification of an instrument is one I watch for carefully. I have
had customers who have done things like replace a sample chamber metal port
cover with a Plexiglas panel so they could peer in and see the sample
positioning. Of course, they would fashion a light tight cover to prevent
swamping of the secondary electron detector in operation, but it would
usually be of a thin aluminum construction. Great, we now have an aluminum
fluorescence source external to the chamber. Don't try this at home,
kiddies.

Localized, point sources such as lens adjustment knobs present little
problem. First, remember that radiation rates fall off as the inverse
square of the distance. If you measure a dose rate at 5mm from the
external exit, at 10mm it is 1/4 as strong, at 20mm 1/16 the strength and
at 40mm (just 1.6") 1/64 as strong.

You also have to consider the extent of the exposure. We probably all
agree that we'd like to minimize exposure to radiation as much as possible,
but what areas of the body are exposed have a large effect on any probable
future problems. While not fully understood, radiation effects are
generally agreed to affect different parts of the body to differing
extents. At the low end of things is exposure of peripheral areas - hands,
arms, feet and legs. These areas don't contain the essential organs that
the thorax does, don't have the faster regenerating cells or the high blood
supply that can support rapid cellular mutations. While there are always
exceptions, you rarely hear of cancers that originate in the fingers or
toes, arms or legs.

My own personal feeling is that Chuck is right, you stand a much greater
chance of long term damage from the various chemicals used in sample
preparation, not to mention common solvents and the samples themselves,
used in an EM lab than you do from possible radiation from an EM.

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174

phone (630) 513-7093 fax (630) 513-7092 http://www.sem.com

On Tuesday, September 28, 2004 10:12 AM, Garber, Charles A.
[SMTP:cgarber-at-2spi.com] wrote:
}
}
}
------------------------------------------------------------------------
------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
http://www.msa.microscopy.com/MicroscopyListserver
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-------
}
} -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
}
} Kart Padari wrote:
} =====================================================
} I?m worried about my health too.
} My question: Is there any harmful radiation working with
} JEOL 100-S electron microscope?
} =====================================================
} My first exposure to an EM was in 1963, the round screen "horizontal"
} Philips 100 TEM. I was told (but don't know from my own knowledge that
} this was true) that some of these earliest models were manufactured with
} ordinary instead of lead glass. I also had contact with an early RCA
TEM,
} I think it was an EMU-1 (or something close to that). Those are the only
two
} EMs I have ever heard about that had inherent radiation problems and once
} the problem was recognized, retrofits were installed, taking away the
} problems. I have met operators of those early RCA instruments who
} literally did their work wearing a lead apron. My sense if that there
are
} none of these old generation EMs in use any more.
}
} Instruments manufactured after that era were designed such that the mass
of
} the column itself would be sufficiently massive and absorbing of x-rays,
} that raditation just could not escape during operation. True, one could
} envision that a column could be sufficiently misaligned that x-rays could
} possibly get out, but the instruments seem to be designed in a way that
if
} they really were misaligned by that extent, there would be a vacuum leak
and
} the high voltage would automatically shut down. Some very many years
ago,
} we tried this with a JEOL 100CX and could not get the microscope
} sufficiently misaligned to allow x-rays to get out. With a JSM-U3 SEM,
at
} that same time, the column would lose vacuum before it could be
misaligned
} sufficiently to allow x-rays to come through.
}
}
} But there are at least several circumstances in which radiation can
escape:
}
} a) Someone breaks the lead glass viewing screen of a TEM and thinking
they
} are saving money, replaces the broken glass with ordinary glass. I have
} heard of this very thing happening, on occasion over the years. Such a
} replacement of the glass would be picked up instantly during any kind of
a
} radiation survey, however. Without such a survey, it is not possible to
} differentiate, by appearance, lead vs. non-lead glass.
}
} b) Adjustment knobs for the lenses seem to be slightly (x-ray) "leaky"
in
} some instruments, but the exposure is localized to the area of the knobs,
} and therefore also to the fingers. With modern instruments where this is
} done by the computer, this risk is much less and might no longer be
present.
} I have heard of people wrapping lead foil around their several fingers
when
} adjusting the knobs but I don't know if that is necessarily a
"recommended"
} procedure. But a general room survey would not necessarily reveal this
} exposure risk.
}
} c) Home made or radically altered commercial instruments which do not
have
} the "safety engineering" built into them that would otherwise be found in
a
} commerical instrument. I have always thought that this type of
instrument
} should be surveyed quite frequently because of the frequency that changes
} seem to be made to the basic instrument.
}
}
} Much of the motivation for those who do radiation surveys involving
} commercially purchase instruments is to protect the organization from
} lawsuits from former or present employees who make the claim that some
} medical condition was either caused or aggrivated by their operation of
} their TEM or SEM. Considering all the persons who have used both SEMs
and
} TEMs over the years, if there was some health issue, I would have thought
} that it would have shown up clinically by now. When considering all
the
} risks in an EM loboratory, I have always thought that exposure to the
} embedding resin chemicals would represent a far greater health risk than
} operating a column instrument.
}
} This is a very important topic and if there are other perspectives on
this,
} I would surely like to hear them.
}
} Chuck
}
} ===================================================
} Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
} President 1-(800)-2424-SPI
} SPI SUPPLIES FAX: 1-(610)-436-5755
} PO BOX 656 e-mail: cgarber-at-2spi.com
} West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com
}
}
} Look for us!
} ############################
} WWW: http://www.2spi.com
} ############################
} ==================================================
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 11:52:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Short Course and Workshop Announcement
University of Missouri - Columbia
(originally scheduled for August 16-18, 2004 was postponed due to Dr.
Russ' illness)

The Electron Microscopy Core Facility is hosting a 3-day Short Course
and Workshop on Computer-Assisted Image Analysis and Measurement
taught by Dr. John C. Russ on November 9=11, 2004. This popular
course is intended to familiarize users of image analysis equipment
with the fundamental principles and methods available to obtain
meaningful results, and to educate laboratory supervisors or research
professionals seeking to learn how to use such methods in their
applications. The techniques are applicable to fields ranging from
materials, geological and biological/medical research to food
technology and manufacturing quality control.

The course relies heavily on tightly coupled lectures and hands-on
experience with the various techniques. The laboratory includes a
wide variety of image analysis methods designed to cover the range of
approaches and tools, and a detailed set of practical instructions to
enable their use with a minimal learning curve. No specific
background is assumed, although users should already be familiar with
microscopy or other imaging technology, and the techniques required
to obtain the images to be measured. Many of the examples used in the
course involve light or electron microscope images, but students are
invited to bring their own most interesting images (TIFF files) for
discussion and analysis.

Image analysis and measurement methods are used in a broad range of
applications and are usually concerned with extracting a few
numerical values, such as the number, size, shape or location of
objects from the image. In other cases, global structural parameters
such as measures of the volume and surface of structures present are
of interest. These measurements may require image processing to
correct defects, feature enhancement, comparison of multiple images,
object recognition, or other steps. Ultimately, the image is reduced
to just the features of interest. Measurements on these individual
features, or on the image as a whole, must then be obtained and
interpreted in a proper stereological context to obtain useful data
about the objects. Statistical interpretation of the data allows
comparisons of different populations, understanding of distribution
plots, and other inferences about the original objects. Structural
modeling and geometric probability can be used to develop models for
this interpretation.

The course will have an enrollment limit of 20, and there are ~10
spots still open. More information including a registration form can
be found at http://www.emc.missouri.edu, or by contacting Lou Ross at
573.882.4777 or rosslm-at-missouri.edu.
--
Senior Electron Microscope Specialist
Electron Microscopy Core Facility
W136 Veterinary Medicine
University of Missouri
Columbia, MO 65211-5120
(573) 882-4777, fax 884=5414
email: rosslm-at-missouri.edu
http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 11:59:53 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi everyone,

Can you help my colleague, Milos Kalab, to solve his problem. His question is posted below. Thank you.

Ann Fook Yang
EM Unit/ Unite EM
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 613-759-1638
Facsimile/Télécopieur: 613-759-1701
960 Carling Ave/960 Boul Carling
Ottawa,Ontario/Ottawa, Ontario
Canada
K1A 0C6
yanga-at-agr.gc.ca

My objective is to obtain SEM images of stainless steel and other surfaces used in food processing. For this reason I wish to replicate small parts of the surfaces and examine the negative replicas. Advice on materials and procedures which would reproduce details down to 1 micrometer would be appreciated. (I am aware of Ted Pella and SPI cellulose acetate replication materials for coarser surfaces and I wonder why I have not been successful.)

Thank you.

Milos Kalab

Agriculture and Agri-Food Canada in Ottawa

kalabm-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 12:23:42 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Dear Listserver,

Is any one using or know of a consumer camera with full computer control
and live video preview mounted on an optical microscope?

Peggy Miller
UTHSCSA Ophthalmology
Lions Sight Research Center
7703 Floyd Curl Drive MC6230
San Antonio, Texas 78229-3900
PH: (210)567-8460
FAX:(210)567-8413

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 16:11:25 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We routinely use acetate replicas from machined metal surfaces that resolve
to the micron level.

Can you describe the procedure used by Milos? Perhaps it differs from what
we do.

Regards,
Woody

-----Original Message-----
} From: Yang, Ann-Fook [mailto:YANGA-at-agr.gc.ca]
Sent: Wednesday, September 29, 2004 1:01 PM
To: microscopy-at-microscopy.com

Hi everyone,

Can you help my colleague, Milos Kalab, to solve his problem. His question
is posted below. Thank you.

Ann Fook Yang
EM Unit/ Unite EM
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 613-759-1638
Facsimile/Télécopieur: 613-759-1701
960 Carling Ave/960 Boul Carling
Ottawa,Ontario/Ottawa, Ontario
Canada
K1A 0C6
yanga-at-agr.gc.ca

My objective is to obtain SEM images of stainless steel and other surfaces
used in food processing. For this reason I wish to replicate small parts of
the surfaces and examine the negative replicas. Advice on materials and
procedures which would reproduce details down to 1 micrometer would be
appreciated. (I am aware of Ted Pella and SPI cellulose acetate replication
materials for coarser surfaces and I wonder why I have not been successful.)

Thank you.

Milos Kalab

Agriculture and Agri-Food Canada in Ottawa

kalabm-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 17:10:08 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mark.evans-at-uvm.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, September 29, 2004 at 15:53:40
---------------------------------------------------------------------------

Email: mark.evans-at-uvm.edu
Name: Mark Evans

Organization: University of Vermont

Title-Subject: [Microscopy] [Filtered] MListserver: Isoamyl acetate and critical point drying

Question: Some protocols for sem indicate that following ethanol series dehydration samples should be soaked in isoamyl acetate and that this media should also be used for critical point drying. Can anyone tell me what the theory is behind using isoamyl acetate and what benefit, if any, there is over leaving samples in 100% ethanol prior to the critical point drying?
Thanks,
Mark

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Sep 29 21:34:39 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Milos Kalab asks:
====================================================
My objective is to obtain SEM images of stainless steel and other surfaces
used in food processing. For this reason I wish to replicate small parts of
the surfaces and examine the negative replicas. Advice on materials and
procedures which would reproduce details down to 1 micrometer would be
appreciated. (I am aware of Ted Pella and SPI cellulose acetate replication
materials for coarser surfaces and I wonder why I have not been successful.)
====================================================
If you are talking about pretty smooth surfaces, there is no reason that I
can see why either a) the cellulose acetate system should not "work" or b)
you could also try what we at SPI Supplies call the SPI Wet Replica Kit,
which is a very rapidly curing silicone system.

You did not say what your basis was for it "not working" but I will assume
that you just did not "see" anything when in fact you expected to be seeing
something. There could be several possible reasons for this:

a) there is some kind of organic contamination coating the surface, so if
you solvent washed the surface (or plasma etched it if it was not too large
to get into a plasma etcher) you might "uncover" what you wanted to be
seeing and/or

b) work with a more dilute solution of the cellulose acetate or

c) there is structure there but you might do better seeing it by Pt/C
shadowing the cellulose acetate (negative) replica, dissolving away the
plastic, picking up the replica on a TEM grid and viewing the replica in a
TEM instead of an SEM. It is possible that the topographical variation of
your structure is insufficient to give the level of contrast needed to be
seen by SEM.

The silicone system might be easier to work with, especially if you wanted
to return to the same identical area, if you wanted to be following the same
area as a function of time (e.g. as a function of use if you are doing wear
studies). But the same comments about making sure the surface is "clean"
and properly "prepared" would apply, otherwise you will just be replicating
the surface of the contamination or residues. The silicone system would
work only for SEM examination, not TEM.

Disclaimer: SPI Supplies offers both cellulose acetate replicating tapes
and sheets and also the SPI Wet Replica kit as described on the website
given below.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 02:28:47 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have not used amyl acetate for CPD since my first CPD run almost 30
years ago.
The head of department was incensed by the strong pear/banana smell
and banned it as antisocial.
In those days nobody seemed to worry about its toxicity. Amyl acetate
also damages
the rubber seals of the CPD faster than other solvents.

The objective is to fully replace the dehydrating solvent with liquid
CO2.
Amyl acetate is more soluble in liquid CO2 than the more polar
ethanol, but
many people nevertheless use ethanol routinely and obtain great
results, especially if the
specimens are small, thin, and unenclosed by cuticle (cultured cells
on coverslips, for example).
If the specimens are large chunks of plant material it would be better
to work with acetone (propanone)
as both dehydrating and intermediate solvent.

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "by way of MicroscopyListserver" {mark.evans-at-uvm.edu}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, September 29, 2004 11:12 PM

Peggy

most of the recent Canon Powershot range allow for control and previewing of the camera from a computer via the USB port. The A80 (recently superseded by the A95) and the A95 also have a screen which can be rotated to a useful angle for viewing when the camera is on the top of a microscope. One disadvantage is that they only produce JPEG images (not RAW or TIFF).
You could check some of the specifications at:
http://consumer.usa.canon.com/ir/controller?act=ProductCatIndexAct&fcategoryid=113

A more upmarket Canon would be the Powershot G6 (this does JPEG and RAW format I believe) - see website below for a review which includes detail of the computer control facilities:
http://www.dcresource.com/reviews/canon/powershot_g6-review/index.shtml

I would assume that some Nikons may have the facilities that you want but I have no personal experience of them - just my trusty little A80.

Certainly there are are microscope and camera adaptors to enable attachment to light microscopes for Nikon and Canon digital cameras - just do a web search.

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: "Miller, Margaret M" {MILLERMM-at-uthscsa.edu}

Hi, Peggy!

We do quite a lot of LM digital imaging these days. Through Nikon we had
purchased the Photometrics Cool Snap cf camera to place atop an Olympus BH-2
light microscope. The software program we're using is called Metavue; it
allows you to view live and make changes to lighting and such before saving.
The best part is being able to make much smaller files by making duplicate
images and saving into TIFF. It also allows you to put in micron bars after
calibrating your scope and camera system together. Afterwards, the
duplicated images are able to be used in Photoshop or Power Point.

Good luck in your search!

*Disclaimer--I do not work for, or receive any compensation from, Nikon or
the makers of Metavue. We are just satisfied with the setup.

Donna R. Clarkson, HT (ASCP)
Northrop Grumman Information Technology
for U S Army Medical Research Detachment
at Brooks City-Base
Phone (210) 536-1416
FAX (210) 536-1449
e-mail donna.clarkson-at-brooks.af.mil
"Our Army at War--Relevant and Ready"

-----Original Message-----
} From: Miller, Margaret M [mailto:MILLERMM-at-uthscsa.edu]
Sent: Wednesday, September 29, 2004 12:25 PM
To: Microscopy-at-microscopy.com

Dear Listserver,

Is any one using or know of a consumer camera with full computer control
and live video preview mounted on an optical microscope?

Peggy Miller
UTHSCSA Ophthalmology
Lions Sight Research Center
7703 Floyd Curl Drive MC6230
San Antonio, Texas 78229-3900
PH: (210)567-8460
FAX:(210)567-8413

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 09:04:36 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Amyl acetate is supposed to be more miscible in lqCO2 than is EtOH. I
have also heard that it's supposed to be a suspected carcinogen, but
I don't have any references on that. One reason I was given for using
Amyl acetate when I was learning EM Back When was that it smells of
bananas, and therefore it can be easily known when it's all been
flushed out.
I've never used A. acetate, just EtOH, and I get fine results. I may
have to purge more than I would if I used A. acetate, but not much.
And the EtOH has plenty of odor, so it's also easy to tell when the
bulk is gone by smell.
But it's the Aac or EtOH *in* the samples that has to be gotten rid
of, not the bulk fluid, and that's too small a volume to smell anyway.
Phil

} Email: mark.evans-at-uvm.edu
} Name: Mark Evans
}
} Organization: University of Vermont
}
} Title-Subject: [Microscopy] [Filtered] MListserver: Isoamyl acetate
} and critical point drying
}
} Question: Some protocols for sem indicate that following ethanol
} series dehydration samples should be soaked in isoamyl acetate and
} that this media should also be used for critical point drying. Can
} anyone tell me what the theory is behind using isoamyl acetate and
} what benefit, if any, there is over leaving samples in 100% ethanol
} prior to the critical point drying?
} Thanks,
} Mark
}
} ---------------------------------------------------------------------------

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 09:07:27 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Greetings Margaret,
I don't know of any "consumer grade" cameras (the kind you can get at
BestBuy) with real time focusing and robust computer control. We had an
older Kodak DC210 "micro-imaging package" and it was, and still is,
quite possibly the worst ccd solution marketed for microscopy that I
have ever seen. The little Pixellink cameras for microscopy are fine
for routine brightfield work but they cost about $2k (the Kodak system
was about the same amount several years ago). A favorite among amateur
microscopists is the Nikon CoolPix (google nikon coolpix microscopy),
but I don't know of a real time computer control interface for it. In
order to use such a camera on a microscope you either have to dimantle
the camera to expose the bare ccd, then make some sort of c-mount
adapter, or you will have to get a hold of a special optical coupler
with a lens system to project the image on the ccd correctly through the
camera lens. Actually I've heard that you can take a snapshot directly
through the eyepiece if you hold the camera just right. I highly
recommend a camera designed for microscopy if you don't want to look
through the eyepieces or don't like judging image quality from a 2 inch
low-res lcd.
-Karl

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 10:08:14 2004

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The following is the agenda for the Fall MATCSEM and Midwest Society meeting. For those planning on attending, please email me for parking permits:

wcarmichael-at-matcmadison.edu

Annual Fall MATCEM / MMMS Microscopy Meeting

Friday, October 15 at Madison Area Technical College, Truax campus

8:45 - 9:30 Meeting registration (Coffee, tea, juice, donuts and bagels will be provided)

9:30 - 9:45 Welcome, Introductions and Business information

9:45 - 10:30 Food Microstructure: Industry Perspectives
By Randy Brandsma of Schreiber Foods, Inc.
Randy is currently a research scientist with Schreiber Foods Inc. of Green Bay WI.
After receiving his MS in Dairy Science and working as a QA manager for Davisco International he earned his PhD from Cornell University with focus on membrane filtration for cheese manufacturing. He is currently using Confocal and SEM in his work to understand the microstructure of cheese and its effects on performance.

10:30 - 12:00 Forensic Microscopical Analysis of Food, Beverages and Containers from Top to Bottom.
By Richard E. Bisbing and Elaine F. Schumacher of McCrone Associates, Inc.

Richard is the Executive Vice President, managing the technical operations group and overseeing all services at McCrone Associates. Prior to joining McCrone Richard was involved in trace evidence work for the Michigan state police and Dept. of public health. He continues to consult on analytical light microscopy and forensic sciences.

Elaine is a Senior Research Scientist and utilizes TEM techniques such as high resolution imaging, electron diffraction, x-ray microanalysis and EELS to characterize a wide variety of industrial materials and problems. Prior to McCrone Elaine worked at UOP Research Center developing catalysts and process technology for the refining industry.

Lunch - A box lunch will be provided courtesy of the MATC vendors

1:15 - 2:30 How Measurements in the nm to µm Size Range Help in Polymer Product Development by Bodan Ma and Sunil Jayasuriya of SC Johnson Polymer

Sunil is the Technical Manager for Polymer Characterization and Applications Research group. He earned his PhD in Physical Chemistry from the Univ. of Bristol, UK. Sunil has worked on applications of surface chemistry and colloid science for printing, personal care, and package coating industries.

Bodan is the Technical Manager for Coatings and has extensive experience in the structure-property relationship of polymeric materials, such as adhesives and coatings. He holds a PhD in Polymer Sciences from Univ. of Massachusetts, Amherst and holds 8 US patents in formulation of new materials.

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 11:10:47 2004

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The very old Sorvall Critical Point Dryer came with a spare parts box
that had special
O-Rings that needed to be used if amyl acetate was to be used. The
directions did not
give any reason for using it. I have usually used Acetone for
dehydrations and a freshly
opened bottle of Mallinckrodt #2440 acetone for the final exchange
before the drying.

Many years ago an investigator insisted on using amyl acetate with
his sample and he
ran the operation himself. He later admitted that similar samples
that I ran in acetone
looked better.

If one uses amyl acetate in the critical point dryer it is extremely
necessary for the
amyl acetate to be properly vented into a hood (acetone also). If
the amyl acetate of
this volume gets into the room it can make one behave strangely.
My co-workers thought that I was drunk! I did not make that mistake again.
Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu
===========================
} I have not used amyl acetate for CPD since my first CPD run almost
} 30 years ago.
} The head of department was incensed by the strong pear/banana smell
} and banned it as
} antisocial.In those days nobody seemed to worry about its toxicity.
} Amyl acetate also
} damages the rubber seals of the CPD faster than other solvents.
}
} The objective is to fully replace the dehydrating solvent with liquid CO2.
} Amyl acetate is more soluble in liquid CO2 than the more polar ethanol, but
} many people nevertheless use ethanol routinely and obtain great
} results, especially if
} the specimens are small, thin, and unenclosed by cuticle (cultured
} cells on coverslips,
} for example). If the specimens are large chunks of plant material it
} would be better to
} work with acetone (propanone) as both dehydrating and intermediate solvent.
}
} Dr. Chris Jeffree {c.jeffree-at-ed.ac.uk}
} University of Edinburgh
============================
} } Email: mark.evans-at-uvm.edu
} } Name: Mark Evans
} } Organization: University of Vermont
} } Title-Subject: [Microscopy] Isoamyl acetate and critical point drying
} }
} } Question: Some protocols for sem indicate that following ethanol
} } series dehydration samples should be soaked in isoamyl acetate and
} } that this media should also be used for critical point drying. Can
} } anyone tell me what the theory is behind using isoamyl acetate and
} } what benefit, if any, there is over leaving samples in 100% ethanol
} } prior to the critical point drying?
} } Thanks,
} } Mark
} } ---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 12:36:11 2004

Contents Retrieved from Microscopy Listserver Archives
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We have been doing replicating products since the 1950s, so if you wish to
discuss replication please call Mike Bouchard at 1-800-451-3406 and he'll be
glad to provide assistance on replicating. Mike has many years of
experience in this area.

Thanks,
Deb Sicard

Disclaimer: Ladd has been a supplier of EM products, including replicating
materials, for more than 50 years

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: ladres-at-att.net

----- Original Message -----
} From: "White, Woody N." {nwwhite-at-bwxt.com}
To: "'Yang, Ann-Fook'" {YANGA-at-agr.gc.ca} ; {microscopy-at-microscopy.com}
Sent: Wednesday, September 29, 2004 5:06 PM

We routinely use acetate replicas from machined metal surfaces that resolve
to the micron level.

Can you describe the procedure used by Milos? Perhaps it differs from what
we do.

Regards,
Woody

-----Original Message-----
} From: Yang, Ann-Fook [mailto:YANGA-at-agr.gc.ca]
Sent: Wednesday, September 29, 2004 1:01 PM
To: microscopy-at-microscopy.com

Hi everyone,

Can you help my colleague, Milos Kalab, to solve his problem. His question
is posted below. Thank you.

Ann Fook Yang
EM Unit/ Unite EM
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 613-759-1638
Facsimile/Télécopieur: 613-759-1701
960 Carling Ave/960 Boul Carling
Ottawa,Ontario/Ottawa, Ontario
Canada
K1A 0C6
yanga-at-agr.gc.ca

My objective is to obtain SEM images of stainless steel and other surfaces
used in food processing. For this reason I wish to replicate small parts of
the surfaces and examine the negative replicas. Advice on materials and
procedures which would reproduce details down to 1 micrometer would be
appreciated. (I am aware of Ted Pella and SPI cellulose acetate replication
materials for coarser surfaces and I wonder why I have not been successful.)

Thank you.

Milos Kalab

Agriculture and Agri-Food Canada in Ottawa

kalabm-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 15:02:08 2004

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I can offer only the comments of an experimenting amateur, with a Nikon Coolpix 990. I am using GNU/Linux as an operating system, and have had a modicum of success with setting up several programs to manipulate the camera's controls. It's exciting enough to encourage me to do further experiments with a newer model of Coolpix.

I take photos through the eyepiece, using a relatively inexpensive coupler that is merely a clamp to hold the camera onto the eyepiece. Several companies manufacture these, as well as optical couplers (so-called relay lenses) which take the place of an eyepiece. (I don't understand the difference between relay lenses and the projection lenses of the past).

I really like that the coolpix can be monitored in real time through the TV, which works wonders for me, as a teacher, in teaching about microscopical realms without having student microscopes at our school. Using some tips for setting up this camera for microscopy (more than one set of which I found on the Inet) I find it relatively easy to take at least snapshots. With a cable release, and a bright enough light---perhaps I will finally get around to setting up a strobe---the results promise to be able to freeze motion even of cilia.

A promising suggestion was to use a video capture card to move the video image to the computer screen while using software to remotely fire the camera. I don't know whether this is possible, but I hope to try it. I can see why the Coolpix 990 has received so much attention from the microscopical community. It is available relatively cheaply on ebay, too, so perhaps this could serve as the basis for some experiments for you, too.

I am doubly encouraged at how well the camera is supported by a GIMP (Gnu Image Manipulation Program---a photoshop like program) plugin. Better than any other software, so far, I have found it easy to even monitor the image in *pretty much* real time and snap on demand, at which point the image is immediately available for cropping and editing. The program is free (in terms of your being able to share copies---in terms, in other words, of freeDOM, as well as free BEER freedom). This, again, encourages my further experimentation. I am considering the upcoming Nikon Coolpix 8800 which has vibration reduction technology included!

Take my comments with the appropriate grain of salt.

Alan Davis
Kagman High School
Saipan, Northern Mariana Islands
aedavis-at-eccomm.com

On Thu, 30 Sep 2004 08:02:31 -0500
Clarkson Donna R Contr USAMRD/MCMR {donna.clarkson-at-brooks.af.mil} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi, Peggy!
}
} We do quite a lot of LM digital imaging these days. Through Nikon we had
} purchased the Photometrics Cool Snap cf camera to place atop an Olympus BH-2
} light microscope. The software program we're using is called Metavue; it
} allows you to view live and make changes to lighting and such before saving.
} The best part is being able to make much smaller files by making duplicate
} images and saving into TIFF. It also allows you to put in micron bars after
} calibrating your scope and camera system together. Afterwards, the
} duplicated images are able to be used in Photoshop or Power Point.
}
} Good luck in your search!
}
} *Disclaimer--I do not work for, or receive any compensation from, Nikon or
} the makers of Metavue. We are just satisfied with the setup.
}
} Donna R. Clarkson, HT (ASCP)
} Northrop Grumman Information Technology
} for U S Army Medical Research Detachment
} at Brooks City-Base
} Phone (210) 536-1416
} FAX (210) 536-1449
} e-mail donna.clarkson-at-brooks.af.mil
} "Our Army at War--Relevant and Ready"
}
}
}
} -----Original Message-----
} } From: Miller, Margaret M [mailto:MILLERMM-at-uthscsa.edu]
} Sent: Wednesday, September 29, 2004 12:25 PM
} To: Microscopy-at-microscopy.com
} Subject: [Microscopy] LM digital imaging
}
}
}
}
} ----------------------------------------------------------------------------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ----------------------------------------------------------------------------
} ---
}
} Dear Listserver,
}
} Is any one using or know of a consumer camera with full computer control
} and live video preview mounted on an optical microscope?
}
} Peggy Miller
} UTHSCSA Ophthalmology
} Lions Sight Research Center
} 7703 Floyd Curl Drive MC6230
} San Antonio, Texas 78229-3900
} PH: (210)567-8460
} FAX:(210)567-8413
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 16:51:56 2004

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Hello, All-

Last year a couple of students from BYU Hawaii were interested in looking
for copper in the mitochondria of yeast by EELS and/or ESI, using our LEO
912 EFTEM. The first (but by no means the only) stumbling block was
getting decent ultrastructure, or at least good enough that they could
identify the mitochondria, and good enough infiltration that 25-30 nm
sections could be obtained.

I do not have any experience with yeast and so I am open to any and all
hints, tips, and suggestions!

If this works out, I invite you all to come to see the results at M&M 2005
in Honolulu next August.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 17:57:15 2004

Contents Retrieved from Microscopy Listserver Archives
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After years of trying desperately to get one of our microtomes
working, I'm thinking of changing the company that provides
service on our instruments (2 Reichert Ultracut E and 2 Leica
UCT/FCS). Does anyone in the NorthEast know of someone
capable of providing service in Connecticut? I'm especially
interested in someone with good experience with the
Leica instruments.
Thank you

Marc
--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Thu Sep 30 21:23:11 2004

Contents Retrieved from Microscopy Listserver Archives
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John:

See http://http://www.math.ualberta.ca/imaging/
There, one might find these remarks:

"... newer cameras (Coolpix 995/775 and beyond) can only be controlled via a serial cable"

There's more to all this than I understand.

Alan

On Thu, 30 Sep 2004 20:58:25 -0400
John Twilley {jtwilley-at-sprynet.com} wrote:

} Dear Alan,
}
} Do I understand you correctly that the 990 has some input for control by a PC? Is this true of the 995 as well? Are you writing this control routine yourself?
}
} John Twilley
}
} Alan E. Davis wrote:
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } I can offer only the comments of an experimenting amateur, with a Nikon Coolpix 990. I am using GNU/Linux as an operating system, and have had a modicum of success with setting up several programs to manipulate the camera's controls. It's exciting enough to encourage me to do further experiments with a newer model of Coolpix.
} }
} } I take photos through the eyepiece, using a relatively inexpensive coupler that is merely a clamp to hold the camera onto the eyepiece. Several companies manufacture these, as well as optical couplers (so-called relay lenses) which take the place of an eyepiece. (I don't understand the difference between relay lenses and the projection lenses of the past).
} }
} } I really like that the coolpix can be monitored in real time through the TV, which works wonders for me, as a teacher, in teaching about microscopical realms without having student microscopes at our school. Using some tips for setting up this camera for microscopy (more than one set of which I found on the Inet) I find it relatively easy to take at least snapshots. With a cable release, and a bright enough light---perhaps I will finally get around to setting up a strobe---the results promise to be able to freeze motion even of cilia.
} }
} } A promising suggestion was to use a video capture card to move the video image to the computer screen while using software to remotely fire the camera. I don't know whether this is possible, but I hope to try it. I can see why the Coolpix 990 has received so much attention from the microscopical community. It is available relatively cheaply on ebay, too, so perhaps this could serve as the basis for some experiments for you, too.
} }
} } I am doubly encouraged at how well the camera is supported by a GIMP (Gnu Image Manipulation Program---a photoshop like program) plugin. Better than any other software, so far, I have found it easy to even monitor the image in *pretty much* real time and snap on demand, at which point the image is immediately available for cropping and editing. The program is free (in terms of your being able to share copies---in terms, in other words, of freeDOM, as well as free BEER freedom). This, again, encourages my further experimentation. I am considering the upcoming Nikon Coolpix 8800 which has vibration reduction technology included!
} }
} } Take my comments with the appropriate grain of salt.
} }
} } Alan Davis
} } Kagman High School
} } Saipan, Northern Mariana Islands
} } aedavis-at-eccomm.com
} }
} } On Thu, 30 Sep 2004 08:02:31 -0500
} } Clarkson Donna R Contr USAMRD/MCMR {donna.clarkson-at-brooks.af.mil} wrote:
} }
} } }
} } }
} } } ------------------------------------------------------------------------------
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } -------------------------------------------------------------------------------
} } }
} } } Hi, Peggy!
} } }
} } } We do quite a lot of LM digital imaging these days. Through Nikon we had
} } } purchased the Photometrics Cool Snap cf camera to place atop an Olympus BH-2
} } } light microscope. The software program we're using is called Metavue; it
} } } allows you to view live and make changes to lighting and such before saving.
} } } The best part is being able to make much smaller files by making duplicate
} } } images and saving into TIFF. It also allows you to put in micron bars after
} } } calibrating your scope and camera system together. Afterwards, the
} } } duplicated images are able to be used in Photoshop or Power Point.
} } }
} } } Good luck in your search!
} } }
} } } *Disclaimer--I do not work for, or receive any compensation from, Nikon or
} } } the makers of Metavue. We are just satisfied with the setup.
} } }
} } } Donna R. Clarkson, HT (ASCP)
} } } Northrop Grumman Information Technology
} } } for U S Army Medical Research Detachment
} } } at Brooks City-Base
} } } Phone (210) 536-1416
} } } FAX (210) 536-1449
} } } e-mail donna.clarkson-at-brooks.af.mil
} } } "Our Army at War--Relevant and Ready"
} } }
} } }
} } }
} } } -----Original Message-----
} } } } From: Miller, Margaret M [mailto:MILLERMM-at-uthscsa.edu]
} } } Sent: Wednesday, September 29, 2004 12:25 PM
} } } To: Microscopy-at-microscopy.com
} } } Subject: [Microscopy] LM digital imaging
} } }
} } }
} } }
} } }
} } } ----------------------------------------------------------------------------
} } } --
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } ----------------------------------------------------------------------------
} } } ---
} } }
} } } Dear Listserver,
} } }
} } } Is any one using or know of a consumer camera with full computer control
} } } and live video preview mounted on an optical microscope?
} } }
} } } Peggy Miller
} } } UTHSCSA Ophthalmology
} } } Lions Sight Research Center
} } } 7703 Floyd Curl Drive MC6230
} } } San Antonio, Texas 78229-3900
} } } PH: (210)567-8460
} } } FAX:(210)567-8413
} } }
} } }
} } }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 07:37:03 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Tek-Net in Lakewood, NJ
732-905-5530

Geoff

Marc Pypaert wrote:

} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} After years of trying desperately to get one of our microtomes
} working, I'm thinking of changing the company that provides
} service on our instruments (2 Reichert Ultracut E and 2 Leica
} UCT/FCS). Does anyone in the NorthEast know of someone
} capable of providing service in Connecticut? I'm especially
} interested in someone with good experience with the
} Leica instruments.
} Thank you
}
} Marc
} --
} Marc Pypaert
} Department of Cell Biology
} Center for Cell and Molecular Imaging
} Ludwig Institute for Cancer Research
} Yale University School of Medicine
} 333 Cedar Street, PO Box 208002
} New Haven, CT 06520-8002
} TEL 203-785 3681
} FAX 203-785 7446
}
}

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 08:52:21 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Marc, et al,

I am also interested in getting a repairperson for my Ultracut E. It really
needs an overhaul.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Marc Pypaert [mailto:marc.pypaert-at-yale.edu]
Sent: Thursday, September 30, 2004 6:58 PM
To: 'Microscopy-at-MSA.Microscopy.Com'

After years of trying desperately to get one of our microtomes
working, I'm thinking of changing the company that provides
service on our instruments (2 Reichert Ultracut E and 2 Leica
UCT/FCS). Does anyone in the NorthEast know of someone
capable of providing service in Connecticut? I'm especially
interested in someone with good experience with the
Leica instruments.
Thank you

Marc
--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 09:03:25 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi, everyone:

I have some questions regarding DNA stains:

What are the advantages of using DAPI instead of Hoescht? In which
conditions should we use one or the other?

What are the main differences between the 2 Hoescht dyes?

I read about a new DNA stain, DRAQ5, has anyone used it? Can it be applied
to study apoptosis?

Thank you in advance,

Vera Santos

Instituto de Tecnologia Biomédica

Faculdade Medicina Dentária

Universidade de Lisboa

Portugal

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 12:07:41 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Peggy,

I use Microscopical Optical Consulting, out of Valley Cottage NY. You
can reach them at 845-268-6450.

Ann Lehman
Electron Microscopy Facility
Mailstop: LSC314
Trinity College
300 Summit Street
Hartford, CT 06106
v. 860-297-4289
f. 860-297-2538
e. ann.lehman-at-trincoll.edu
w. http://www.trincoll.edu/~alehman

-----Original Message-----
} From: Sherwood, Margaret [mailto:MSHERWOOD-at-PARTNERS.ORG]
Sent: Friday, October 01, 2004 9:47 AM
To: 'Marc Pypaert'; 'Microscopy-at-MSA.Microscopy.Com'

Marc, et al,

I am also interested in getting a repairperson for my Ultracut E. It
really
needs an overhaul.

Peggy

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Marc Pypaert [mailto:marc.pypaert-at-yale.edu]
Sent: Thursday, September 30, 2004 6:58 PM
To: 'Microscopy-at-MSA.Microscopy.Com'

After years of trying desperately to get one of our microtomes
working, I'm thinking of changing the company that provides
service on our instruments (2 Reichert Ultracut E and 2 Leica
UCT/FCS). Does anyone in the NorthEast know of someone
capable of providing service in Connecticut? I'm especially
interested in someone with good experience with the
Leica instruments.
Thank you

Marc
--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 15:02:20 2004

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Hi:

We just installed a new TEM and it was suggested that we use a 'demand
regulator' to control the flow of nitrogen during specimen exchange and/or
venting the column etc. The installing engineer didn't have the details for
ordering etc.

Ok, so tell me about demand regulators and where to get one.

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 18:15:35 2004

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Colleagues,

Our Mini-Workshop Series on "Cryoultramicrotomy for Materials Science" is
coming to Akron, Ohio!

**When**:
Thursday, October 14 - Friday, October 15, 2004, 9:00am-4:00pm

**Where**:
University of Akron
Department of Polymer Engineering
Polymer Engineering Academic Center (PEAC)
Room 307
250 South Forge Street
Akron, OH 44325

**What**:
A two-day mini-workshop with presentations, demonstrations and hands-on
sessions for cryoultramicrotomy, including toolmaking (wire loops and hair probes),
glass knife making, evaluation of glass knives, care and cleaning of diamond
knives and operation of the cryoultramicrotome.

Lectures, demonstrations and an introduction to the cryoultramicrotome will
be given on the first day; open lab sessions and hands-on use of the
instrumentation in small groups will be the focus of the second day.

Demonstrations will be given using well-characterized specimens which are
provided by the instructors. There is a limited amount of time to work with
specimens provided by attendees. If you would like to bring your own specimens,
please provide details on the materials when you RSVP and reserve a place in
the workshop.

**Background**:
These techniques are of special interest to anyone working with polymers or
other materials which could benefit from sectioning or surface "polishing"at
low temperatures (no embedding required). The sections may be used for TEM,
optical microscopy, IR spectroscopy and FTIR. The polished surface of the bulk
material is suitable for AFM, SEM, X-ray microanalysis and elemental mapping.

**Important Info**:

1. There is no charge for this workshop.

2. Meals and refreshments will be served!

3. Attendance is open to everyone for the presentations and demonstrations
on the first day. However, attendance is limited for the cryoultramicrotomy
hands-on sessions on the second day.

**RSVPs and Reservations**:
To RSVP and to reserve a spot for the hands-on sessions, please contact Kim
Megaw at Boeckeler Instruments, Inc. ( {kim-at-boeckeler.com} , 800.552.2262).

**Sponsors and Organizers**:
University of Akron
Department of Polymer Engineering
RMC Products Group, Boeckeler Instruments, Inc.

See you in Akron!

Bob Chiovetti
Senior Product Specialist
Boeckeler Instruments, Inc.

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 1 20:41:20 2004

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Jon,

Check your local scuba shop. I used some PVC (Tygon) tubing, a few hose
clamps, and a few copper plumbing fittings to adapt a scuba regulator for
my dry nitrogen backfill.

I hose-clamped a piece of large diameter Tygon over the mouthpiece then
downsized with the Cu fittings to a 1/4" hose barb which hooked to the hose
to the scope. On the supply side, I cut the original fitting off the high
pressure hose and used a brass hose barb to connect it to my nitrogen gas
regulator.

Have fun explaining to your financial people why you needed to buy a scuba
regulator!

Cheers,
Henk

At 04:03 PM 10/1/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hendrik O. Colijn colijn.1-at-osu.edu
OSU Campus Electron Optics Facility www.ceof.ohio-state.edu
040 Fontana Labs, 116 W. 19th Ave

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 2 03:31:27 2004

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Why is this stuff not being supplied by the vendor, I wonder.

Chris Jeffree
University of Edinburgh

----- Original Message -----
From: "Jon Krupp" {jmkrupp-at-cats.ucsc.edu}
To: {Microscopy-at-microscopy.com}
Sent: Friday, October 01, 2004 9:03 PM
Subject: [Microscopy] Demand regulator

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi:
}
} We just installed a new TEM and it was suggested that we use a
} 'demand
} regulator' to control the flow of nitrogen during specimen exchange
} and/or
} venting the column etc. The installing engineer didn't have the
} details for
} ordering etc.
}
} Ok, so tell me about demand regulators and where to get one.
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 3 09:40:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ghina_24-at-yahoo.com) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Sunday, October 3, 2004 at 00:06:00
---------------------------------------------------------------------------

Email: ghina_24-at-yahoo.com
Name: ghina husnulnisa

Organization: university of andalas

Education: Undergraduate College

Location: padang,west sumatra,indonesia

Question: Do you know about composition of may-gruenwald's eosin methylene blue solution ?
thank's for your answer.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 3 17:51:38 2004

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__________________________________________________
Do You Yahoo!?
Tired of spam? Yahoo! Mail has the best spam protection around
http://mail.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 07:04:34 2004

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Tina,
I recently fixed yeast cells for the first time and also found that it is hard to see the membranes. I followed a protocol suggested by Mark Winey which referenced a paper by Byers (Byers, B. and Goetsch, L. (1991) Preparation of yeast cells for thin section electron microscopy. Methods Enzymol. 194: 602-608.) This procedure involves spheroplasting which removes the cell wall, thus allowing good infiltration. The cells turned out looking great but the people I did the work for wanted to see more membranes.

Another good reference for fixing yeast is a paper by Robin Wright (Wright,R. (2000) Transmission Electron Microscopy of Yeast. Microsc. Res. Tech. 51:496-510). She gives alot of helpful hints for fixing yeast. She gives a detailed procedure in the paper using potassium permanganate as a post fixative. If you use potassium permanganate as a post fixative you don't have to spheroplast the cells (according to the paper, I have not tried it yet). Of course we all know that potassium permanganate extracts much of the cytoplasm, which is perfect for viewing membranes. I hope this will be helpful.

Janice Pennington
Senior Electron Microscopist
Nephrology/Anatomy and Cell Biology
Indiana University School of Medicine
635 Barnhill Drive, MS 5065
Indianapolis, IN 46202
Phone (317) 274-8730
Fax (317) 278-2040

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 09:10:21 2004

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Dear Listers,

I would like to open a discussion about the use of Biosafety Level 2
regulated cells, tissues and organisms in a multi-user microscopy
facility not designed to house BSL2 regulated agents (no once-through
air or biosafety cabinet).

Is it customary to have researchers use the microscopy facility if BSL2
regulated agents are alive but completely contained in unbreakable and
well-sealed containers? While such conditions are easily accomplished
for transport of materials, they are less so for the actual viewing.
How is this commonly resolved?

Is it customary for users to write a protocol for microscope use,
spelling out what to do in an emergency situation?

Is expected from microscopy facility personnel to know exactly what to
do in case of an emergency situation (e.g. if somebody works on BSL2
regulated bacteria in a flow cell and one of the connections breaks
during microscope operation, spilling the content over microscope
equipment), or is this the responsibility of the investigator?

In case of spillage, a broken slide, etc., how does one deal with the
resulting contaminated equipment?

Is it customary to have every user fill out and sign a form explaining
what organisms they plan to use, how it is regulated and how they plan
to use those organisms in the microscopy facility?

Thank you for your input.

All the best,
Judith.

Judith Wopereis
Microscopy Facility Manager and
Instructor of Laboratories in Biological Sciences
Smith College
Northampton, MA 01063
(413) 585 3829 (voice mail)
(413) 585 3786 (fax)
jwoperei-at-email.smith.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 09:12:36 2004

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We purchased ours through our local compressed gas vendor.

Hendrik O. Colijn wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Jon,
}
} Check your local scuba shop. I used some PVC (Tygon) tubing, a few
} hose clamps, and a few copper plumbing fittings to adapt a scuba
} regulator for my dry nitrogen backfill.
}
} I hose-clamped a piece of large diameter Tygon over the mouthpiece
} then downsized with the Cu fittings to a 1/4" hose barb which hooked
} to the hose to the scope. On the supply side, I cut the original
} fitting off the high pressure hose and used a brass hose barb to
} connect it to my nitrogen gas regulator.
}
} Have fun explaining to your financial people why you needed to buy a
} scuba regulator!
}
} Cheers,
} Henk
}
}
} At 04:03 PM 10/1/2004, you wrote:
}
}
} } ------------------------------------------------------------------------------
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} }
} } Hi:
} }
} } We just installed a new TEM and it was suggested that we use a 'demand
} } regulator' to control the flow of nitrogen during specimen exchange
} } and/or
} } venting the column etc. The installing engineer didn't have the
} } details for
} } ordering etc.
} }
} } Ok, so tell me about demand regulators and where to get one.
} }
} } Thanks
} }
} } Jonathan Krupp
} } Microscopy & Imaging Lab
} } University of California
} } Santa Cruz, CA 95064
} } (831) 459-2477
} } jmkrupp-at-cats.ucsc.edu
}
}
} Hendrik O. Colijn colijn.1-at-osu.edu
} OSU Campus Electron Optics Facility www.ceof.ohio-state.edu
} 040 Fontana Labs, 116 W. 19th Ave
}
}
}

--
--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 10:14:05 2004

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I would like to know if there is a mixture of epoxy and carbon powders for ion-
thinning in market. A researcher from Hungary made a low angle ion-thinner
(IV3?), and also he confirmed that if you use C powder with epoxy, you can ion-
thin fine grain materials like powder. I do not remember the reference now,
but you can get a lower thinning rate of the C and epoxy mixture, according to
the paper.
I used a kit for ion-thinning in Japan. Probably, it was imported from
Hungary.
If you use similar technique, please advise where I can get the powdered epoxy
and C.

Thank you,
Hiromi Konishi, Ph.D.
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 10:29:26 2004

Contents Retrieved from Microscopy Listserver Archives
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We have also used these on several instruments at our facility. Alex Greene
set them up. The only difference was he filled the mouthpiece with RTV
sealant and used a secondary output on the regulator to connect to the
scope. I am not sure if all SCUBA regulators have this output, or if the
ones he found were special.

One problem you might find is if the demand is too high or the supply too
low, the small silicone diaphragm used for exhaling can invert allowing room
air into the system. I have also always worried (however with no proof)
that the line between the regulator and the instrument, being at zero
pressure WRT the room, can become contaminated with room air.

On our latest TEM and SEM installs, we have not used these since the
manufactures have included doors or popup valves that open when the pressure
difference becomes zero WRT the room.

-Ray

Ray D. Twesten, PhD.
Center for Microanalysis of Materials
Seitz Materials Research Laboratory
104 S. Goodwin Ave., Urbana, IL 61801
+1 217 244-6177 (Fax -2278)

-----Original Message-----
} From: colijn-at-er6s1.ecr6.ohio-state.edu
[mailto:colijn-at-er6s1.ecr6.ohio-state.edu]On Behalf Of Hendrik O. Colijn
Sent: Friday, October 01, 2004 8:47 PM
To: Microscopy-at-microscopy.com

Jon,

Check your local scuba shop. I used some PVC (Tygon) tubing, a few hose
clamps, and a few copper plumbing fittings to adapt a scuba regulator for
my dry nitrogen backfill.

I hose-clamped a piece of large diameter Tygon over the mouthpiece then
downsized with the Cu fittings to a 1/4" hose barb which hooked to the hose
to the scope. On the supply side, I cut the original fitting off the high
pressure hose and used a brass hose barb to connect it to my nitrogen gas
regulator.

Have fun explaining to your financial people why you needed to buy a scuba
regulator!

Cheers,
Henk

At 04:03 PM 10/1/2004, you wrote:

} ---------------------------------------------------------------------------
---
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hendrik O. Colijn colijn.1-at-osu.edu
OSU Campus Electron Optics Facility www.ceof.ohio-state.edu
040 Fontana Labs, 116 W. 19th Ave

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 11:44:37 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Tina,

First of all, I can vouch for the Wright protocol for preparing yeast for
TEM mentioned by Janice (1. below). Works great! Membranes stand right out
there, resins infiltrate through wall completely into cell (I used
Embed812).

In your query (2. below) you mention that the ultimate goal of your study is
to look for copper in mitochondria in yeast, using EELS or whatever
analytical technique. For elemental analysis in sections, given all the prep
they usually go through, there is always the danger of leaching out the
element you are interested in looking for. Any elements/compounds that are
water soluble - they're gone! So even if you succeed in getting good
membrane and mitochondrial fixation, may not be any copper left. Do you know
for sure if the copper is bound in the mitochondria?

I have heard that freeze-substitution does a better job of preserving
elements in place for elemental analysis - you'd just have to try it and
see. Or try freeze-drying small masses of sample, then vacuum infiltrate
with resin.

Good luck! Gib
--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra
-------------

1. ---------
Tina,
I recently fixed yeast cells for the first time and also found that it is
hard to see the membranes. I followed a protocol suggested by Mark Winey
which referenced a paper by Byers (Byers, B. and Goetsch, L. (1991)
Preparation of yeast cells for thin section electron microscopy. Methods
Enzymol. 194: 602-608.) This procedure involves spheroplasting which
removes the cell wall, thus allowing good infiltration. The cells turned
out looking great but the people I did the work for wanted to see more
membranes.

Another good reference for fixing yeast is a paper by Robin Wright
(Wright,R. (2000) Transmission Electron Microscopy of Yeast. Microsc. Res.
Tech. 51:496-510). She gives alot of helpful hints for fixing yeast. She
gives a detailed procedure in the paper using potassium permanganate as a
post fixative. If you use potassium permanganate as a post fixative you
don't have to spheroplast the cells (according to the paper, I have not
tried it yet). Of course we all know that potassium permanganate extracts
much of the cytoplasm, which is perfect for viewing membranes. I hope this
will be helpful.

Janice Pennington
Senior Electron Microscopist
Nephrology/Anatomy and Cell Biology
Indiana University School of Medicine
635 Barnhill Drive, MS 5065
Indianapolis, IN 46202
Phone (317) 274-8730
Fax (317) 278-2040

2. -----------------
Hello, All-

Last year a couple of students from BYU Hawaii were interested in looking
for copper in the mitochondria of yeast by EELS and/or ESI, using our LEO
912 EFTEM. The first (but by no means the only) stumbling block was
getting decent ultrastructure, or at least good enough that they could
identify the mitochondria, and good enough infiltration that 25-30 nm
sections could be obtained.

I do not have any experience with yeast and so I am open to any and all
hints, tips, and suggestions!

If this works out, I invite you all to come to see the results at M&M 2005
in Honolulu next August.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 12:28:39 2004

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Dear Hiromi:

The Low Angle Ion Thinner you are referring to is the IV3 from
Technoorg-Linda in Budapest. Actually, they make the IV3 with high
energy guns, low energy guns as well as a focussed ion gun. They also
produce the Gentle Mill which is a dedicated low energy ion polisher.

As the distributor for Technoorg-Linda products in North America, we do
offer the carbon/epoxy product that you reference. I will contact you
offline with the part number and pricing.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

hkonishi-at-indiana.edu wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 13:25:49 2004

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Hi Tina,
Yeast cells freeze quite nicely. I think the closest high pressure
freezer to you is located in Kent McDonald's lab at Berkeley .

Beth

On Thursday, September 30, 2004, at 05:53 PM, Tina Carvalho wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Hello, All-
}
} Last year a couple of students from BYU Hawaii were interested in
} looking
} for copper in the mitochondria of yeast by EELS and/or ESI, using our
} LEO
} 912 EFTEM. The first (but by no means the only) stumbling block was
} getting decent ultrastructure, or at least good enough that they could
} identify the mitochondria, and good enough infiltration that 25-30 nm
} sections could be obtained.
}
} I do not have any experience with yeast and so I am open to any and all
} hints, tips, and suggestions!
}
} If this works out, I invite you all to come to see the results at M&M
} 2005
} in Honolulu next August.
}
} Aloha,
} Tina
}
} ***********************************************************************
} *****
} * Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu
} *
} * Biological Electron Microscope Facility * (808) 956-6251
} *
} * University of Hawaii at Manoa *
} http://www.pbrc.hawaii.edu/bemf*
} ***********************************************************************
} *****
}
}
}
**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 16:03:18 2004

Contents Retrieved from Microscopy Listserver Archives
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But how does one know which marker pens are OK and which are not?

cheers

rtch

}
} One thing of note....
}
} DO NOT use sharpie markers or any other acid base pen to label cd's or
} dvd's. The acid in these pens etches through the top of the disk
} destroying your data.
}
} Dave Crone B.E. (Mechanical)
} Engineer-in-Training
} Department Assistant
} Metallurgical Lab
} Mechanical Engineering
} College of Engineering
} University of Saskatchewan
} 57 Campus Drive
} Saskatoon, SK
} S7N 5A9
} Phone: (306) 966-5461
} Fax: (306) 966-5427

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 18:24:47 2004

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It is a safe bet that if they are sold on the premise that they are cd safe
they should be good

Dave Crone B.E. (Mechanical)
Engineer-in-Training
Department Assistant
Metallurgical Lab
Mechanical Engineering
College of Engineering
University of Saskatchewan
57 Campus Drive
Saskatoon, SK
S7N 5A9
Phone: (306) 966-5461
Fax: (306) 966-5427
E-mail: dgc132-at-mail.usask.ca
dgc132-at-gmail.com
-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Monday, October 04, 2004 3:06 PM
To: Dave Crone; 'MICROSCOPY'

But how does one know which marker pens are OK and which are not?

cheers

rtch

}
} One thing of note....
}
} DO NOT use sharpie markers or any other acid base pen to label cd's or
} dvd's. The acid in these pens etches through the top of the disk
} destroying your data.
}
} Dave Crone B.E. (Mechanical)
} Engineer-in-Training
} Department Assistant
} Metallurgical Lab
} Mechanical Engineering
} College of Engineering
} University of Saskatchewan
} 57 Campus Drive
} Saskatoon, SK
} S7N 5A9
} Phone: (306) 966-5461
} Fax: (306) 966-5427

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext
87713
Microanalyst Fax : 64 9 3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 19:10:31 2004

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I have used Sharpies many times to mark disks, and have never seen a
problem yet. I should add that I always use top-coated disks.

John Mardinly
Intel

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Monday, October 04, 2004 2:06 PM
To: Dave Crone; 'MICROSCOPY'

But how does one know which marker pens are OK and which are not?

cheers

rtch

}
} One thing of note....
}
} DO NOT use sharpie markers or any other acid base pen to label cd's or
} dvd's. The acid in these pens etches through the top of the disk
} destroying your data.
}
} Dave Crone B.E. (Mechanical)
} Engineer-in-Training
} Department Assistant
} Metallurgical Lab
} Mechanical Engineering
} College of Engineering
} University of Saskatchewan
} 57 Campus Drive
} Saskatoon, SK
} S7N 5A9
} Phone: (306) 966-5461
} Fax: (306) 966-5427

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext
87713
Microanalyst Fax : 64 9
3737435
Department of Geology email :
r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 19:36:57 2004

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Hi,

I agree with Henk and Mike. I believe CDRs ARE archival grade if handled
properly. Even those thousand year old clay tablets, suggested in jest,
are almost useless if broken or turned to dust from improper handling.

I did not read the whole article but I what to address the Sharpie® acidic
ink problem. In the interest of having all this CDR stuff in one posting,
I offer this web information:

I used Sharpie pens for years on CDRs without a problem.
The acidic pen posting raised these questions:
Were my Sharpie® pens the acidic types?
Was my first official US flag research CD going to disintegrate?
So, I looked to SandfordCorp.com to see what they said about acidic pens.

http://www.sanfordcorp.com/sanford/consumer/jhtml/help/sanford_help_922.jhtml

Quoting:
"There are two criteria, which identify "Acid Free" Products:
1. The product must contain no added acid
2. The product must contain an ink with a pH specification of 7 or above,
or the product has no measurable pH because it contains a solvent - based
ink or it is a solid. (The pH cannot be measured if the ink does not
contain water)

Product Color
(snip other types of markers that are not permanent)

Permanent Markers
7000 Marker All Colors
7007 Marker All Colors
Deluxe Marker - All Colors Not Black
King Size Marker - All Colors Not Black
Liquid Tip Marker All Colors
Magnum 44 - All Colors Not Black
Mean Streak All Colors
Rub-A-Dub Black
Sharpie Autograph Black
Label Pen Black
Penguin Freezer Wrap Marker Black
T.E.C. Markers Black (Trace Element free pens)
Sharpie Industrial Black "
End quote.

It should be obvious what to use.
I used black Industrial and Label pens without any problems, IMO.

Disclaimer: I don't work for Sanford Corp but I like Sharpie® pens.

My thanks to Hendrik O. Colijn at The Ohio State University for providing
the original reference.

Paul Beauregard
Senior Research Associate

-----------------------------------------------------------------------
} Original Sharpie Pen post:
} One thing of note....
} DO NOT use sharpie markers or any other acid base pen to label cd's or
} dvd's. The acid in these pens etches through the top of the disk destroying
} your data.
}
} Dave Crone B.E. (Mechanical)
}
End Beauregard postings.
-------------------------------------------
At 10:28 AM 9/27/04 -0700, Michael O'Keefe wrote:
}
} Henk,
}
} That's an extremely informative and useful article. Thank you!
}
} It was interesting to learn that CD RW and DVD RW (bits encoded in metal
structure
} by a phase change from crystalline to amorphous) are less stable over time
than CD
} R and DVD R (bits encoded in degradable organic dyes). And that RW discs
that are
} "cycled" a lot (many re-writes) will degrade faster.
}
} The best advice seems to be to use R (write once) discs (CD or DVD) and
store them
} vertically in a cool, low-light environment. Of course, transferring to
fresh
} media every year or so couldn't hurt...
}
} Mike
}
} "Hendrik O. Colijn" wrote:
}
} }
------------------------------------------------------------------------------
} }
} } Hi all,
} }
} } I just ran across this reference in our local newspaper about the care and
} } storage of CDs and DVDs. It is copublished by CLIR (Council on Library and
} } Information Resources) and NIST, so it should be reliable info.
} }
} } http://www.clir.org/pubs/reports/pub121/contents.html
} }
} } From my quick run through of the article, it appears that DVDs may be
} } inherently more stable than CDs.
} }
} } Cheers,
} } Henk
} }
} } Hendrik O. Colijn colijn.1-at-osu.edu
} } Campus Electron Optics Facility Ohio State University
} } (614) 292-0674 http://www.ceof.ohio-state.edu
} } Time is that quality of nature which keeps events from happening all at
} } once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 19:58:26 2004

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Ritchie,

According to the article I read, the issue seems to be damage to the
lacquer on the top surface of the CD. The author of the article recommends
water based markers or perhaps alcohol based, but not other solvent
based. For example, I've got a marker which appears to be xylene-based
(sniff test!) and probably damaging to the protective lacquer. I certainly
found it interesting that the top-surface is more delicate than the bottom!

For details, see below...
http://www.clir.org/pubs/reports/pub121/contents.html

Cheers,
Henk

At 05:06 PM 10/4/2004, Ritchie Sims wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hendrik O. Colijn colijn.1-at-osu.edu
OSU Campus Electron Optics Facility www.ceof.ohio-state.edu
040 Fontana Labs, 116 W. 19th Ave

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 4 21:07:25 2004

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Greetings,

Optical Elements Corporation (OPELCO) has current openings for an Image
Analysis Sales Specialist and a Confocal Microscopy Sales Specialist in
the Mid-Atlantic region. If interested, please click on the following
link or contact me directly.

http://www.opelco.com/employmentcontact.htm

Best Regards,

Cliff Glier
COO
OPELCO
105 Executive Drive Suite 100
Dulles, VA 20166
703.471.0080 x230
703.904.9432 (fax)
cglier-at-opelco.com
www.opelco.com

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 10:29:47 2004

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Paul,

Thanks for your info. I went to the Sanford site and noticed that they
provide MSDS sheets for their markers. Interestingly, Sharpies do not all
use the same solvents. I'm not an organic chemist, so I would appreciate
if someone would correct me... If I remember correctly, n-propanol and
n-butanol are alcohols and should not affect the lacquer. I don't know
about diacetone alcohol or about the ethers. Based on my uneducated guess,
I would probably avoid the naptha solvents in the "Sharpie Professional"
series.

Can anyone provide additional info about lacquers and solvents?

Sharpie Fine Point Permanent, Sharpie Twin-tip, Super Sharpie, Super
Sharpie Twin-tip
n-propanol, n-butanol, diacetone alcohol

Sharpie Ultra Fine Point
n-propanol, n-butanol, diacetone alcohol, isopropyl alcohol, ethyl alcohol

Sharpie Industrial Fine Point
ethylene glycol monobutyl ether, ethylene glycol monoethyl ether, ethyl alcohol

Sharpie Professional
nitroparaffin solvent, solvent naptha

Cheers,
Henk Colijn

At 08:41 PM 10/04/04, Beauregard wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hendrik O. Colijn colijn.1-at-osu.edu
Campus Electron Optics Facility Ohio State University
(614) 292-0674 http://www.ceof.ohio-state.edu
Time is that quality of nature which keeps events from happening all at
once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 12:41:49 2004

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Dear All,

I've recently started taking birefringence photographs of Congo Red stained
tissue. I've noticed that over time, the very same field doesn't appear the
same, and that the labeled surface varies up to 25%.

Everything being very stable (all screws firmly screwed, polarizer glued to
its base), I'm wondering if anyone has performed a test to check the warm-up
period of a halogen 6 volt lamp. The company who sells the lamp says 5 to 10
minutes, but could it be longer?

Thank you!

Marie-Claude Belanger

_________________________________________________________________
Des mécanismes de contrôle parental puissants permettent ŕ votre enfant de
découvrir tout ce qu’Internet a ŕ offrir.
http://join.msn.com/?pgmarket=fr-ca&page=features/parental&ST=1&xAPID=1983&DI=2043
Commencez dčs maintenant ŕ profiter de tous les avantages de MSN Premium et
obtenez les deux premiers mois GRATUITS*.

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 12:57:22 2004

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Dear Listserver,

Does anyone have a good reciepe for TEM
fixation of ebryonic cell cultures? (ie 293
kidney). Are these cell's osmolarities generally
higher or lower than other cell types. Thanks.

Mike Delannoy

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 16:38:06 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (monica.iliescu-at-polymtl.ca) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 5, 2004 at 10:47:16
---------------------------------------------------------------------------

Email: monica.iliescu-at-polymtl.ca
Name: Monica ILIESCU

Organization: Ecole Polytechnique

Title-Subject: [Microscopy] [Filtered] Sample preparation

Question:
Does some know how prepare the biological samples for ESEM observations? We have an Quanta FEG 200, FEI Company, and we want to prepare for observation a sample from chitosan solution, to see the chitosan nanoparticles.
Thank you!

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 16:38:57 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (aiqbal-at-email.arizona.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 5, 2004 at 13:21:33
---------------------------------------------------------------------------

Email: aiqbal-at-email.arizona.edu
Name: Asad Iqbal

Organization: University of Arizona

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Please if some one could help me with this.
I would like to know if there is any software available to measure thickness and composition of the sample using SEM/EDS. Where can I get it from?

Thank You,

Regards,
Asad

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 16:43:13 2004

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I am looking for help imaging active drug particles in an aqueous pharmaceutical suspension. I am trying to locate someone who can view frozen sections of this material in the 100 angstrom size range. I believe this will require an environmental SEM with a cryogenic stage. I would appreciate any help. Thank you.

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 17:05:09 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi all,
I have not used NIH Image or Scion Image and a student in my department
has the following question:

} I'm looking at leaf morphology in a number of tree species, and I've
} got 100's of flatbed leaf scans that I'm trying to analyze using Scion
} Image (a PC spin-off of NIH Image) and ImageJ. The problem I'm having
} is that the program is recognizing (and measuring) the background as
} well as the leaf in its area calculations. Do you have any advice or
} could you help in any way in dealing with this problem?

Any help would be greatly appreciated!
thanks in advance,
Beth

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 17:19:46 2004

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}
} I believe CDRs ARE archival grade if handled
} properly.

That (handled properly) is indeed the problem with this class of media.

As was mentioned in the report referenced by an earlier post, (if you
read between the lines), this media CAN be very easily damaged.

As an IT Manager, I would suggest you think about what you mean by
"Archive" class media.

If you mean something that you can hide away in a controlled
environment, and carefully access at some point in the future, then
maybe this class of media is appropriate.

If you mean something that you can use for routine "archive" access (as
opposed to "on-line" access) I would strongly suggest that the media CAN
be too sensitive to physical damage (more so on the label side than the
"bottom" side).

If you mean something that will absolutely, positively be there when you
need it for "disaster recovery", I would suggest that this isn't the
media you want for that.

I don't mean to say the media isn't durable, or won't last. Just that
there is a chance that a single disk may be easily damaged, either by
natural causes (thermal cycling, humidity, etc.) or accidentally by
routine handling. My friend Murphy says that this will happen on the
most important area of the most important disk at the most inopportune
time.

I have lived the nightmare of backup systems not working for a number of
reasons. You don't want to go there.

John W. Raffensperger, Jr.
IT Manager
Apache Stainless Equipment

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 17:35:18 2004

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I would like to know the best way to prepare ion-thinning samples of small
particles. The size is several 10 um. I know that FIB or microtome might work
better, but I want to try ion thinning. The material is mineral like SiO2.

If you embed small grains in epoxy, the grains drop during milling in many
cases because thinning rates of sample and epoxy are different. Also, rough
surface that are produced by preferential etching is another problem. It is
hard to make good ion-thinning sample of small grains in general.

Using Araldite (AT1) containing C or M-bond 610 can reduces the problem of
preferential etching of glue (Barna 1992, Westman et at 1999, McCaffrey and
Barna 1997). (SBT sells "Carbon powder & Araldite-Type AT1" for low angle ion
milling). Photo-resist is "hard" in ion milling (Yoshioka at al 1995).

I do not have any other idea that may reduce the problem in preferential
etching. If you have any suggetions, please advise. Also, if someone used AT1
with Gatan Dual Mill or PIPS, I would like to know if you got better result or
not.

Thank you,

Hiromi Konishi, Ph.D.
Indiana University
www.unm.edu/~hkonishi

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 5 19:22:37 2004

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It is probably trivial but ...

.. does the student threshold and binarize the picture before to do
the analysis ?

1) Threshold and choose the level he wants

2) Binarize (black & white picture, 0 or 256)

3) Analyse (and if the program take everything & not only the
particles, try invert picture. I don't remember if NIH or Scion Image
consider the white or the black spots as particles...).

Hope it helps

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
Christian Wuethrich, PhD
Harvard Medical School
Division of Viral Pathogenesis
Beth Israel Deaconess Medical Center
Research East. Room 217
41 Av. Louis Pasteur
Boston, MA 02115
United States

Phone: 001-617-667-2143
Fax: 001-617-667-8210

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 00:37:19 2004

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Friends
on Darwin, a new italian journal on science and science policy, there
is an article on Multiphoton microscopy "Il radioso futuro della
microscopia ottica" and also the cover has been dedicated to
multiphoton microscopy. I'd like to thank Kenneth Dunn for providing
one of the images of the article collected and rendered by Ruben
Sandoval at the Indiana Center for Biological Microscopy. Website is
www.darwinweb.it.
All my best
ALby

------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 03:05:53 2004

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Dear Asad,

layer thickness measurement within the Electron Microscope and with the
EDX-spectrometer with electron excitation is possible, but is faced to a
lot of limits. The penetration-range of electrons in specimen is
strongly limited. If the layer is going to become thicker (depends from
primary electron energy, typically 1 micron or less), saturation is
reached, no reliable results are possible. The calculation of all
interactions are complex. If there are multi-layers, the electrons have
to travel through the top layers... Therefore layer-measurements are
only possible with very thin layers.

With an X-ray excitation the entire situation is more friendly and
therefore more reliable. Thicknesses of 1 nm up to 50 microns are
possible to deal with. Because of the larger range of X-ray penetration
in specimen, multi-layers are not a problem. An X-ray excitation in SEM
is available now and proper software for calculation thickness and
concentrations with X-ray excitation, as well: see:
http://www.ifg-adlershof.de/sem.htm

Best regards

Frank Eggert

====================
http://www.microanalyst.net
====================

by way of MicroscopyListserver wrote:

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (aiqbal-at-email.arizona.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 5, 2004 at 13:21:33
---------------------------------------------------------------------------

Email: aiqbal-at-email.arizona.edu
Name: Asad Iqbal

Organization: University of Arizona

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Please if some one could help me with this.
I would like to know if there is any software available to measure thickness and composition of the sample using SEM/EDS. Where can I get it from?

Thank You,

Regards,
Asad

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 07:31:41 2004

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John,
Then what would a "good" method of data archive? Hardware RAID and tape?

---
Robb Westby
Senior SEM/FIB Technician
Maxim Integrated Products

On Tue, 2004-10-05 at 15:23, Chiphead wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} }
} } I believe CDRs ARE archival grade if handled
} } properly.
}
} That (handled properly) is indeed the problem with this class of media.
}
} As was mentioned in the report referenced by an earlier post, (if you
} read between the lines), this media CAN be very easily damaged.
}
} As an IT Manager, I would suggest you think about what you mean by
} "Archive" class media.
}
} If you mean something that you can hide away in a controlled
} environment, and carefully access at some point in the future, then
} maybe this class of media is appropriate.
}
} If you mean something that you can use for routine "archive" access (as
} opposed to "on-line" access) I would strongly suggest that the media CAN
} be too sensitive to physical damage (more so on the label side than the
} "bottom" side).
}
} If you mean something that will absolutely, positively be there when you
} need it for "disaster recovery", I would suggest that this isn't the
} media you want for that.
}
} I don't mean to say the media isn't durable, or won't last. Just that
} there is a chance that a single disk may be easily damaged, either by
} natural causes (thermal cycling, humidity, etc.) or accidentally by
} routine handling. My friend Murphy says that this will happen on the
} most important area of the most important disk at the most inopportune
} time.
}
} I have lived the nightmare of backup systems not working for a number of
} reasons. You don't want to go there.
}
} John W. Raffensperger, Jr.
} IT Manager
} Apache Stainless Equipment
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 08:43:55 2004

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Hi,

Already a couple of years ago, former colleagues did automated
calcium-ratio measurements with CCD-camera's on individual
(cardio)myocytes in cell cultures. They used a modified CCD-camera which
allowed them to capture an image of an individual (cardio)myocyte every
10 milliseconds to monitor intracellular calcium.

I am wondering which type of camera could now be used to give the same
time-resolution (10 msec. frame time) for individual cells (the hardware
they used is now no longer available) ?

Reference:

Cornelissen, F., Wouters, L., Ver Donck, L., Verellen, G., Geerts, H.
Automatic quantification of the effect of cardioprotective drugs in
isolated myocytes.
Bioimaging, 1993, 1, pp. 197-206.

Regards,

Peter Van Osta

----------------------------------------------
Peter Van Osta

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 10:08:41 2004

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In my opinion (for what it may be worth) tape has
proven to be, and remains, the best "archival" media.
It has proven to be the most durable, and most likely
to be available when needed.

Raid would come into play not so much for archive, but
for "availability". If you can live with the data
being unavailable for a period of time while a new
disk drive is put in place (if required) and the
backup restored, then raid is not necessarily
required. If you NEED to have the data available NOW,
then raid provides some fault tolerance, and the
ability to keep the data available while the recovery
is in process.

Tape is not perfect, it can be destroyed, but it is
less likely to have the types of single use failure
that CD/DVD media are susceptible to. They can take
an awful lot of environmental and physical abuse, and
still be readable.

Don't get me wrong, CD/DVD have their place. I use
them all the time. Just not for archive, and I never
use them to hold the only copy of something (even on
multiple disks) that needs to be kept. For cases
where the data could not be kept on the hard drives, I
would make a tape backup, then a set of CD/DVDs for
the users.

John Raffensperger

--- Robb Westby {robbw-at-mxim.com} wrote:

}
}
}
------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
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}
-------------------------------------------------------------------------------
}
} John,
} Then what would a "good" method of data archive?
} Hardware RAID and tape?
}
} ---
} Robb Westby
} Senior SEM/FIB Technician
} Maxim Integrated Products
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 15:14:26 2004

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Hello,
Would using hepes as a buffer for reducing glutaraldehyde
with Nh4Cl be a problem? I know hepes isn't compatible with
osmium, but what about other IEM chemicals say tannic acid?
thanks
Mike D.

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 17:35:15 2004

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We use HEPES for paraformaldehyde/glutaraldehyde in the primary fix, with
50 mM glycine in the blocking step, and with 1% osmium. why do you think
it is incompatible with osmium?

At 03:18 PM 10/06/04, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 18:17:59 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwareham-at-utah.gov) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, October 6, 2004 at 16:06:52
---------------------------------------------------------------------------

Email: bwareham-at-utah.gov
Name: Beverly Wareham

Organization: Utah Veterinary Diagnostic Laboratory

Title-Subject: [Microscopy] [Filtered] hydrogels/organogels

Question: Hi all,
I'm looking for a protocol to prepare some gel samples for SEM. They are referred to in papers as hydrogels or organogels. Any help with this is greatly appreciated.

Thanks,
Beverly Wareham
Utah Veterinary Diagnostic Laboratory
Logan, Utah

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 18:18:51 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (njt3-at-u.washington.edu) from http://msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Wednesday, October 6, 2004 at 15:14:41
---------------------------------------------------------------------------

Email: njt3-at-u.washington.edu
Name: Jeanie Taylor

Organization: Univ of Wash

Education: Graduate College

Location: Seattle, Wa

Question: I am trying to calibrate the scale on an Olympus BH-2 compound scope. How do I check the measurement of the sacle in the eyepiece?

Thanks!

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 18:19:13 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mahtab977-at-yahoo.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Wednesday, October 6, 2004 at 16:48:16
---------------------------------------------------------------------------

Email: mahtab977-at-yahoo.com
Name: Mahtab Shahkarami

Organization: San Jose State University

Education: Graduate College

Location: San Jose, CA USA

Question: I was wondering if anyone has had any experience using Si-chips (from Ted Pella) for growing cells. My purpose is to visualize attachment appendages of gram-negative bacteria, so a smooth surface is key. I'm not sure how much better Si-chips are than glass coverslips, and I also don't know how how to sterilize them (autoclave or ethanol?).

Furthermore, I want to thank you all for your responses to a past question of mine about HMDS drying- the procedure/tips I recieved were very useful.

-Mahtab Shahkarami

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 20:13:40 2004

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On Oct 6, 2004, at 4:22 PM, by way of MicroscopyListserver wrote:

} I'm looking for a protocol to prepare some gel samples for SEM. They
} are referred to in papers as hydrogels or organogels. Any help with
} this is greatly appreciated.
}
Dear Beverly,
Robert Apkarian has worked with these substances a lot, so check his
recent papers (if you have not already done so).
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 21:14:30 2004

Contents Retrieved from Microscopy Listserver Archives
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Another media which may be considered "archival quality" is magneto-optical
(MO) disks. They are mounted in the case and have a shelf life expectation
of 100+ years. As far as I know most of the government agencies used this
media to store our records at FBI and INS. MOs may be destroyed by
physical force (hammer?) or extreme temperature (fire). Tapes are great
too and more practical than MOs. The greatest disadvantage of MOs is that
they are slow and capacity is not very impressive (a couple of Gigs, which
is nothing nowadays). Modern CD/DVDs may not be considered as a good
storage solution. Meantime, we are using them in everyday life (with some
risk). The best known to me storage media is ceramic tablets. Sergey

At 08:12 AM 10/6/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 6 21:52:34 2004

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Pardon this commercial announcement.

Bioptechs does not make a habit of this type of announcement in this forum.
However, in this case I, think it is appropriate.

For the past 12 years we have been asked , by many users of this
list, for a micro-environmental cell culture chamber system for
upright microscopes. I am pleased to announce that we have finally
completed it! It is called the FCS3. It is based on the popular FCS2
technology. This system will enable any upright microscope equipped
with a digital camera to acquire long term ,live-cell , time-lapse
images of living organisms including mammalian specimens. Now, those
of you without an inverted microscope can easily accommodate
live-cell experiments with the same ease as inverted scope users.
Ideal for multi user facilities! Additional information is
available at: http://www.bioptechs.com/Products/FCS3/fcs3.html (This
link will take you directly to the appropriate page)

If you are offended by this posting please respond directly to me
with your admonishment.

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 00:30:19 2004

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I have been following the tread since we also store data. (as do all EM units!) I did not see the mentioning of hardisks as a option. I have thrown away (beginning of last year) my vintage 20meg hard disk that was purchased in 1989. My Pentium 1 was scrapped. It was still working perfectly with all the data intact. Hot-swapping allows fast and reliable backup easy. The cost of HD has dropped dramatically. Re installing is fast (hot swapping)
Just a thought.

-----Original Message-----
} From: Sergey Ryazantsev [mailto:sryazant-at-ucla.edu]
Sent: Thursday, October 07, 2004 4:19 AM
To: Microscopy-at-microscopy.com

Another media which may be considered "archival quality" is magneto-optical
(MO) disks. They are mounted in the case and have a shelf life expectation
of 100+ years. As far as I know most of the government agencies used this
media to store our records at FBI and INS. MOs may be destroyed by
physical force (hammer?) or extreme temperature (fire). Tapes are great
too and more practical than MOs. The greatest disadvantage of MOs is that
they are slow and capacity is not very impressive (a couple of Gigs, which
is nothing nowadays). Modern CD/DVDs may not be considered as a good
storage solution. Meantime, we are using them in everyday life (with some
risk). The best known to me storage media is ceramic tablets. Sergey

At 08:12 AM 10/6/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 06:22:49 2004

Contents Retrieved from Microscopy Listserver Archives
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We had a quick look at hydogels by putting them wet in an
ESEM.

Dave

On Wed, 06 Oct 2004 18:22:35 -0500 by way of
MicroscopyListserver {bwareham-at-utah.gov} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwareham-at-utah.gov) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, October 6, 2004 at 16:06:52
} ---------------------------------------------------------------------------
}
} Email: bwareham-at-utah.gov
} Name: Beverly Wareham
}
} Organization: Utah Veterinary Diagnostic Laboratory
}
} Title-Subject: [Microscopy] [Filtered] hydrogels/organogels
}
} Question: Hi all,
} I'm looking for a protocol to prepare some gel samples for SEM. They are referred to in papers as hydrogels or organogels. Any help with this is greatly appreciated.
}
} Thanks,
} Beverly Wareham
} Utah Veterinary Diagnostic Laboratory
} Logan, Utah
}
} ---------------------------------------------------------------------------
}
}
}
} This incoming email to UWE has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
}

----------------------------------------
Patton, David
Email: David.Patton-at-uwe.ac.uk
"University of the West of England"

This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 08:00:02 2004

Contents Retrieved from Microscopy Listserver Archives
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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Mahtab Shahkarami wrote:
============================================================================
=
Question: I was wondering if anyone has had any experience using Si-chips
(from Ted Pella) for growing cells. My purpose is to visualize attachment
appendages of gram-negative bacteria, so a smooth surface is key. I'm not
sure how much better Si-chips are than glass coverslips, and I also don't
know how how to sterilize them (autoclave or ethanol?).
============================================================================
I have been lead to believe that at least some are using our own gold coated
Si-Chips for the growing of cells, see URL
http://www.2spi.com/catalog/submat/gold-coated-silicon-chips.shtml

The description of the uncoated silicon chips, also used for cell growth, is
given on URL
http://www.2spi.com/catalog/standards/silicon-chip-sample.shtml
The smoothness of the silicon surface is comparable to that of a glass cover
slip. The silicon used for their production is standard electronics
industry grade silicon wafers.

The uncoated silicon chips can certainly be autoclaved, however, we don't
have information on the survivability of the gold coated substrates under
autoclave conditions. We would appreciate knowing if anyone has such
information since we are asked that question from time to time.

Disclaimer: SPI Supplies manufactures both uncoated and gold coated silicon
chip substrates for cell growth applications.

Chuck
===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 08:51:01 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

My company is considering obtaining an Hitachi 806 cold field emitter
SEM. The organization that if offering it has not been pleased with its
performance, but is offering a really good deal. I was wondering if
anyone has experience with this tool? If so I would appreciate your
comments.

Thanks,

Gerhard
--
Gerhard S. Schoenthal, PhD
Director of Laboratories
Virginia Diodes, Inc.
321 West Main Street
Charlottesville, VA 22903

W: 434.297.3257
M: 434.409.7760
F: 530.884.5710

W: Schoenthal-at-vadiodes.com

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 08:59:21 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

My company is considering obtaining an Hitachi 806 cold field emitter
SEM. The organization that if offering it has not been pleased with its
performance, but is offering a really good deal. I was wondering if
anyone has experience with this tool? If so I would appreciate your
comments.

Thanks,

Gerhard
--
Gerhard S. Schoenthal, PhD
Director of Laboratories
Virginia Diodes, Inc.
321 West Main Street
Charlottesville, VA 22903

W: 434.297.3257
M: 434.409.7760
F: 530.884.5710

W: Schoenthal-at-vadiodes.com

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 09:10:02 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Tom,
I once read on this listserver that organic
buffers shouldn't be used with osmium because they
could react (oxidized?). Although I will admit that
I have used reduced osmium with hepes with no noticeable artifacts (maybe due to the lower oxidation
state). I want to know if Hepes can be used as the
only buffer in a post-embed IEM protocol up to
uranyl acetate.

thanks
Mike Delannoy

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 09:39:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Charles;

To answer your question about gold surviving autoclave on Si substrate,
you must state what the base metal is, e.g. Ti, Ti-Pt? I don't think you
put Au directly on the wafer without a base metal.

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Garber, Charles A. [mailto:cgarber-at-2spi.com]
Sent: Thursday, October 07, 2004 10:04 AM
To: MICROSCOPY BB

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Mahtab Shahkarami wrote:
========================================================================
====
=
Question: I was wondering if anyone has had any experience using
Si-chips
(from Ted Pella) for growing cells. My purpose is to visualize
attachment appendages of gram-negative bacteria, so a smooth surface is
key. I'm not sure how much better Si-chips are than glass coverslips,
and I also don't know how how to sterilize them (autoclave or ethanol?).

========================================================================
====
I have been lead to believe that at least some are using our own gold
coated Si-Chips for the growing of cells, see URL
http://www.2spi.com/catalog/submat/gold-coated-silicon-chips.shtml

The description of the uncoated silicon chips, also used for cell
growth, is given on URL
http://www.2spi.com/catalog/standards/silicon-chip-sample.shtml
The smoothness of the silicon surface is comparable to that of a glass
cover
slip. The silicon used for their production is standard electronics
industry grade silicon wafers.

The uncoated silicon chips can certainly be autoclaved, however, we
don't have information on the survivability of the gold coated
substrates under
autoclave conditions. We would appreciate knowing if anyone has such
information since we are asked that question from time to time.

Disclaimer: SPI Supplies manufactures both uncoated and gold coated
silicon chip substrates for cell growth applications.

Chuck
===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 09:44:27 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (schoenthal-at-vadiodes.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, October 7, 2004 at 09:03:40
---------------------------------------------------------------------------

Email: schoenthal-at-vadiodes.com
Name: Gerhard Schoenthal

Organization: Virginia Diodes, Inc.

Title-Subject: [Microscopy] [Filtered] Opinions on Hitachi 806 SEM

Question: Hi,

My company is considering obtaining an Hitachi 806 cold field emitter SEM. The organization that if offering it has not been pleased with its performance, but is offering a really good deal. I was wondering if anyone has experience with this tool? If so I would appreciate your comments.

Thanks,

Gerhard
--
Gerhard S. Schoenthal, PhD
Director of Laboratories
Virginia Diodes, Inc.
321 West Main Street
Charlottesville, VA 22903

W: 434.297.3257
M: 434.409.7760
F: 530.884.5710

W: Schoenthal-at-vadiodes.com

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 09:55:13 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have seen HEPES react with KMnO4 (it literally turns the mix into a gel
that then breaks down into time into a precipitate). Never had a problem
with either 1% osmium or 1% reduced osmium. After osmium, we usually rinse
with dH2O before ethanol dehydration since by this time the tissue is no
longer osmotically sensitive. We have done uranyl acetate in ethanol, or
sodium acetate buffer, or water at this stage. I haven't seen a lot of
difference but I think others are strong advocates of uranyl in the ethanol
or sodium acetate. If by post-embedding IEM you mean doing immunostaining
of osmicated, embedded tissues, you have a low probability of success with
most antigens in my experience. I have had a few antigens survive
osmication but generally only ones in high abundance to start. Most immuno
EM work using staining of sections would use aldehyde fixation
(formaldehyde only, or with low glutaraldehyde ~0.2% or sometimes a
standard 2% PF + 2.5% glut) followed by buffer rinses and then maybe a
uranyl acetate en bloc staining and dehydration before embedding in an
immuno friendly plastic like K4M, HM20, LRW, or LRG. LR Gold is my current
favorite but we find the choice is dependent on the antigen and we need to
re-invent the wheel each time and try them all. During our immunostaining
of sections, we use a HEPES buffer (70 mM NaCl, 30 mM HEPES, 2 mM CaCl2, pH
7.4) for the antibodies (usually with 0.1% BSA). good luck.

At 09:12 AM 10/07/04, you wrote:
} Tom,
} I once read on this listserver that organic
} buffers shouldn't be used with osmium because they
} could react (oxidized?). Although I will admit that
} I have used reduced osmium with hepes with no noticeable artifacts (maybe
} due to the lower oxidation
} state). I want to know if Hepes can be used as the
} only buffer in a post-embed IEM protocol up to
} uranyl acetate.
}
} thanks
} Mike Delannoy

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 09:58:22 2004

Contents Retrieved from Microscopy Listserver Archives
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} Date: Thu, 07 Oct 2004 09:58:33 -0500
} To: MICHAEL J DELANNOY {delannoy-at-jhmi.edu}
} From: Tom Phillips {phillipst-at-missouri.edu}
} Subject: [Microscopy] Re: Re: re: Hepes and reduction
} Cc: microscopy
}
} I have seen HEPES react with KMnO4 (it literally turns the mix into a gel
} that then breaks down into time into a precipitate). Never had a problem
} with either 1% osmium or 1% reduced osmium. After osmium, we usually
} rinse with dH2O before ethanol dehydration since by this time the tissue
} is no longer osmotically sensitive. We have done uranyl acetate in
} ethanol, or sodium acetate buffer, or water at this stage. I haven't seen
} a lot of difference but I think others are strong advocates of uranyl in
} the ethanol or sodium acetate. If by post-embedding IEM you mean doing
} immunostaining of osmicated, embedded tissues, you have a low probability
} of success with most antigens in my experience. I have had a few antigens
} survive osmication but generally only ones in high abundance to
} start. Most immuno EM work using staining of sections would use aldehyde
} fixation (formaldehyde only, or with low glutaraldehyde ~0.2% or sometimes
} a standard 2% PF + 2.5% glut) followed by buffer rinses and then maybe a
} uranyl acetate en bloc staining and dehydration before embedding in an
} immuno friendly plastic like K4M, HM20, LRW, or LRG. LR Gold is my
} current favorite but we find the choice is dependent on the antigen and we
} need to re-invent the wheel each time and try them all. During our
} immunostaining of sections, we use a HEPES buffer (70 mM NaCl, 30 mM
} HEPES, 2 mM CaCl2, pH 7.4) for the antibodies (usually with 0.1%
} BSA). good luck.
}
}
}
} At 09:12 AM 10/07/04, you wrote:
} } Tom,
} } I once read on this listserver that organic
} } buffers shouldn't be used with osmium because they
} } could react (oxidized?). Although I will admit that
} } I have used reduced osmium with hepes with no noticeable artifacts (maybe
} } due to the lower oxidation
} } state). I want to know if Hepes can be used as the
} } only buffer in a post-embed IEM protocol up to
} } uranyl acetate.
} }
} } thanks
} } Mike Delannoy
}
} Thomas E. Phillips, PhD
} Professor of Biological Sciences
} Director, Molecular Cytology Core
} 3 Tucker Hall
} University of Missouri
} Columbia, MO 65211-7400
}
} 573-882-4712 (office)
} 573-882-0123 (fax)
} PhillipsT-at-missouri.edu

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 10:17:53 2004

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Silicon wafers behave pretty much like glass. They are ultra-smooth, cells
can be grown on them
without prior coating with gold, and they are rsistant to most reagents you
are likely to use.
An advantage of silicon as a substrate for SEM of cell monlayers is that the
substrate has some conductivity,
the silicon background charges rather less than glass for a given
accelerating voltage and beam current,
and therefore thinner sputtered coatings of gold/palladium, platinum or
chromium can be employed.
A disadvantage is they are more expensive than coverslips, and thicker.
Chris

----- Original Message -----
} From: "Garber, Charles A." {cgarber-at-2spi.com}
To: "MICROSCOPY BB" {Microscopy-at-MSA.Microscopy.com}
Sent: Thursday, October 07, 2004 3:04 PM

Continuing the thread, Some have cited acid-based markers as a potential
problem. Paul Beauregard offered a site at Sanford listing their acid-free
markers. It was not clear whether Sharpie Fine Point markers were included
or not, so I posed the question to their customer service department asking
for clarification. I received the following two responses.

First, they stated that their markers are not acid-free. Next, they stated
that their markers have been tested on CDs without problems.

I guess that simply means that no problem has been observed yet. Since it
is a case of trying to prove a negative, I will go ahead and continue to
use them unless someone can definitely show that the Fine Point markers
have caused a problem. But I suppose I will still pick up a 'certified' CD
marker the next time I go to the store.

Warren

} From: {consumer.service-at-sanfordcorp.com}
} To: {wesaia-at-iastate.edu}
} Subject: [Microscopy] Re: 000356732A, reply from Sanford, Paper Mate, Sharpie,
} uni-ball, Eldon Office Solutions or Foohy.com web-site.
} Date: Tue, 5 Oct 2004 19:00:25 -0400
}
} Hello Warren,
}
} We received your recent inquiry regarding Sharpie® Fine Point Markers.
}
} The Sharpie® Fine Point Markers are not acid free.
}
} Thank you for e-mailing us and for your support of Sanford products.
}
} Sanford Consumer Affairs
}
} 000356732A

} From: {consumer.service-at-sanfordcorp.com}
} To: {wesaia-at-iastate.edu}
} Subject: [Microscopy] Re: 000356732B, reply from Sanford, Paper Mate, Sharpie,
} uni-ball, Eldon Office Solutions or Foohy.com web-site.
} Date: Thu, 7 Oct 2004 11:00:05 -0400
}
} Hello Warren,
}
} Although the Sharpie Markers are not acid free, they have been found safe
} for use on CD's and DVD’s by our lab. Our lab has conducted extensive
} testing on these markers, and found since they are alcohol based, they are
} safe for that application.
}
} Thank you for e-mailing us and for your support of Sanford products.
}
} Sanford Consumer Affairs
}
} 000356732B
-------------
} Date: Mon, 04 Oct 2004 20:41:11 -0400
} To: Microscopy-at-microscopy.com
} From: Beauregard {beaurega-at-westol.com}
} Subject: [Microscopy] Re: Re: CD/DVD as archival media revisited
}
} Hi,
}
} I agree with Henk and Mike. I believe CDRs ARE archival grade if handled
} properly. Even those thousand year old clay tablets, suggested in jest,
} are almost useless if broken or turned to dust from improper handling.
}
} I did not read the whole article but I what to address the Sharpie® acidic
} ink problem. In the interest of having all this CDR stuff in one posting,
} I offer this web information:
}
} I used Sharpie pens for years on CDRs without a problem.
} The acidic pen posting raised these questions:
} Were my Sharpie® pens the acidic types?
} Was my first official US flag research CD going to disintegrate?
} So, I looked to SandfordCorp.com to see what they said about acidic pens.
}
} http://www.sanfordcorp.com/sanford/consumer/jhtml/help/sanford_help_922.jhtml
}
} Paul Beauregard
} Senior Research Associate

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 12:24:33 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

A colleague is interested in using a centrifuge to spin cells down on to
glass slides. We would like the cells to be in multiple discrete spots on
the slide. Anybody have tips on using this approach or places to buy such
a device. Thanks, Tom

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 12:47:33 2004

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Hi Listers:

I have a question regarding the ultrastructural differences between
Aspergillus and a gram positive bacteria. Does anyone out there know any
differences that could be documented by the electron microscope? We have
done all the special stains on this pathology specimen, but we are hoping
the EM will help to further identify the organism we have in question.

Thanks for any help!

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 13:33:44 2004

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ThermoElectron Cytospin:
http://www.thermo.com/com/cda/product/detail/1,,16469,00.html

Up to two 6-mm diameter cell spots per cytofunnel. I authored the user's'
manual in 1982 or so.

Gary Gill

-----Original Message-----
} From: Tom Phillips [mailto:phillipst-at-missouri.edu]
Sent: Thursday, October 07, 2004 12:29 PM
To: Microscopy-at-msa.microscopy.com

NESM Fall 2004 Meeting and Workshop on Cryo Techniques

The 2004/2005 meetings of the New England Society for Microscopy kick off this
Fall with a pair of events on Cryo Techniques for specimen preparation. These
techniques are useful for processing soft, high-volatile specimens for both SEM
and TEM investigations. Soft, wet specimens are common in biological and human
medical investigations. Perhaps less-appreciated are the relatively dry, soft
polymers investigated by materials scientists and food technologists. The
introductory event consists of three lectures on Cryo Techniques in Microscopy.
It will be held on October 19th in the JEOL conference room in Peabody,
Massachusetts. Registration starts at 5:30 PM, then a buffet dinner, and then
the presentations. Those especially interested in learning Cryo skills should
also plan to attend the two-day Workshop on Cryo-Ultramicrotomy on November 3-4.
This workshop, sponsored or supported by NESM, RMC/Boeckeler, Harvard, and MIT,
will be held at Harvard's Center for Imaging and Mesoscale Structures. The
details of the meeting and workshop, including registration information, can be
found on NESM's website http://prism.mit.edu:8083 under "current newsletter".

Registration forms/information for both events can be sent to: NESM Treasurer,
Paul Bain c/o NESM, Harvard Medical School, Countway 212, 10 Shattuck Street,
Boston, MA 02115 email: Paul_bain-at-hms.harvard.edu. The October 19th meeting
costs $5 for members and $20 for non-members (you receive a one-year NESM
membership) and the registration deadline is Friday, October 15th. The November
3-4 Workshop has a $50 professional registration and a $25 student registration.
The registration deadline for the Workshop is Friday, October 22nd. (Register
early for the workshop--space is limited!)

Peggy Sherwood
Corresponding Secretary/Newsletter Editor-NESM

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 7 16:40:44 2004

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karen

while you are aware of this, we should all remind ourselves that EM
diagnostics of micro-organisms can be quite inexact. while negative
stain of viruses will usually give good information concerning the
family, even there we cannot go beyond the fact that the virus is a
herpes, not a poxvirus, not that it is cytomegalovirus, or herpes
zoster, or any other herpes, for that matter. we need the information
of the infectious diseases and/or microbiology staff to be able to go
from EM to specific diagnosis.

having said that, there are clear differences between the bacterial and
fungal cells. most significant is the presence of internal membrane
organelles with the eukaryotic cell, such as aspergillis, and the
presence of the nucleoid in the prokaryotic cell. a second difference
is that the fungal cell is significantly larger than the bacterial
cell. by this, i mean 15-30microns as opposed to 1-5 microns. thirdly,
the yeast and fungal cell walls and external structures are thicker (up
to 500nm) than those seen with the gram positive bacteria. fourthly,
with yeast, and some fungi, you will see budding scars. their
orientation may give some idea as to the specific nature of the
micro-organism you are seeing.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 8 01:12:32 2004

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Hi

We are looking at upgrading our facility here for photographing resected
organs etc at the histopathology department. The new system will be based
on digital cameras so that we can link the photos to the patient
information and diagnosis in our database.

What I would like to know is what people are using these days in terms of
macro lenses, ring flashes (if they exist for the newer cameras) and
lighting systems, lamps, multiple swan-neck lighting.

Any tips would be appreciated from users and from manufacturers etc.

Thanks

Med vänliga hälsningar/With best regards

Gareth

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 8 03:25:57 2004

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Hi,

Thank you all for sending information and suggestions about calcium
ratio mesurements. The main issue was/is to find a camera-solution to
achieve at least the the same framerate as was possible with the old
hardware (now obsolete). Commonly used PAL video-cameras, have a
framerate of about 25 frames per second (FPS, or 33 in NTSC countries)
or lower. Popular digital cameras have advantages over "traditional"
video-standard cameras, but not always achieve a framerate of 25/33 FPS.

What was done in the old system, was to put a "temporal" framesplitter
on the camera, so it allowed to capture quarter frames at 1/4 of the
frametime, which lead to a temporal sampling of 10 msec instead of 40 msec.

Chosing a modern camera which surpasses the old days solution is not a
simple exercise. FireWire interfaces (800 Mbits/sec.) do not deliver the
high bandwidth of CameraLink interfaces (base 2380 Mbit/sec. up to 7140
Mbit/sec.) and their performance goes down when using full-frame
transfer. FireWire cameras are widely available, while the faster
CameraLink cameras are not so popular. Every computer nowadays comes
with a FireWire interface, but a CameraLink is not standard.

http://vsd.pennnet.com/Articles/Article_Display.cfm?Section=Articles&Subsection=Display&ARTICLE_ID=187955

Regards,

Peter

----------------------------------------------
Peter Van Osta

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------

=========================================================
Hi,

Already a couple of years ago, former colleagues did automated
calcium-ratio measurements with CCD-camera's on individual
(cardio)myocytes in cell cultures. They used a modified CCD-camera which
allowed them to capture an image of an individual (cardio)myocyte every
10 milliseconds to monitor intracellular calcium.

I am wondering which type of camera could now be used to give the same
time-resolution (10 msec. frame time) for individual cells (the hardware
they used is now no longer available) ?

Reference:

Cornelissen, F., Wouters, L., Ver Donck, L., Verellen, G., Geerts, H.
Automatic quantification of the effect of cardioprotective drugs in
isolated myocytes.
Bioimaging, 1993, 1, pp. 197-206.

Regards,

Peter Van Osta

----------------------------------------------
Peter Van Osta

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 8 06:04:17 2004

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Both Nikon and Olympus manufacture professional digital SLRs with
top-quality macro lenses and flash systems.
I always used to rate Olympus 35mm systems (based on OM2n, OM4ti) highly for
their macro lenses, and TTL ringflash and macro-flash capability, and had
always dreamed of the day when they would issue their updated system. Alas
that was not to be, but an interesting new digital system has been launched
by Olympus called E1 which uses the four thirds system. Macro lenses and a
ringflash are available for this camera, I see, so this may turn into the
digital equivalent of the OM system if it is equally well received in the
market place.

Depending on how critical you are of issues like camera versatility,
performance etc. you might get a long way towards a solution with a simpler
camera like the Nikon Coolpix 4500. It has remarkable macro capability for
the price, focussing to about 1 inch from front of lens, and there is a
so-called ringflash accessory for it too, actually a ring of high-intensity
white LEDs. I use one of these myself, and know many other scientists who
swear by them for field-recording of specimens ranging from fluorescent gels
to plants and fungi, even aurora borealis displays are within its
capabilities.

I have nothing to gain commercially from these comments
Hope this helps
Chris

----- Original Message -----
} From: "Gareth Morgan" {Gareth.Morgan-at-labmed.ki.se}
To: {Microscopy-at-msa.microscopy.com}
Sent: Friday, October 08, 2004 7:17 AM

For macrophotography of wet biological samples, you must use a
cross-polarization setup to eliminate unsightly lighting "glints"
(highlights). For the past 3 years, we have used both a copystand and
handheld configurations using:

Fujifilm S1 Pro DSLR (ISO 320, 3Kx2K pixels, JPG FINE setting)
Nikon 105mm MACRO with circular polarizing filter
Nikon Speedlight SB-29 Ring light with Polarizing filter
Nikon 24-140mm Zoom (general photography)
Bencher Copymate II with polarizing filters
IBM 1GB Microdrive
~1 ft. cable release (for use with copy stand configuration--don't get a
camera without cable release connector!)
Microdrive/Compact Flash USB Card Reader (forget about transferring directly
from camera to computer).

1. This older Fujifilm camera (current model is S3) is 3.3M sensor creating
6M image via interpolation. I've read and heard all the arguments regarding
interpolation, but the proof is in the image. Awesome. Camera will save in
TIF (18MB file) but it takes nearly 1 minute to transfer captured image to
microdrive so we opted for JPG format in FINE mode, so that the resulting
~2.5MB JPG format saves quicker, but still opens to 6Mpixel, 18MB image.
RAW format is way to go now, but the logistics of easily viewing RAW are not
available to most, and probably not handled by your database.

2. With copystand configuration and 105mm macro, adjust the circular
polarizer to minimize glints. Our current exposures are approximately 1/4 -
1/2 second, and really depend on tissue coloration.

3. For handheld configuration, one needs to determine the correct rotational
placement of the ringlight/polarizer relative to the polarizing filter on
the lens and make a series of test shots (this is because you can't see a
live preview of glint minimization as you do with the copystand setup). The
polarizing filter was custom cut to the shape of the ringlight and mounted
to the front.

Finally, the quality is primarily the lens and the sensor. Have some vendors
let you demo their DSLR models, if possible.

Best regards,

Walter F. Bobrowski
Investigative Pathology
Safety Sciences
Pfizer Global Research & Development
Ann Arbor, MI 48105

TEL: 734-622-7814
FAX: 734-622-3478
Mobile: 734-646-0502

-----Original Message-----
} From: Gareth Morgan [mailto:Gareth.Morgan-at-labmed.ki.se]
Sent: Friday, October 08, 2004 2:17 AM
To: Microscopy-at-msa.microscopy.com

Hi

We are looking at upgrading our facility here for photographing resected
organs etc at the histopathology department. The new system will be basedo
n digital cameras so that we can link the photos to the patient
information and diagnosis in our database.

What I would like to know is what people are using these days in terms ofm
acro lenses, ring flashes (if they exist for the newer cameras) and
lighting systems, lamps, multiple swan-neck lighting.

Any tips would be appreciated from users and from manufacturers etc.

Thanks

Med vänliga hälsningar/With best regards

Gareth

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratorietf
ör klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

LEGAL NOTICE
Unless expressly stated otherwise, this message is confidential and may be privileged. It is intended for the addressee(s) only. Access to this E-mail by anyone else is unauthorized. If you are not an addressee, any disclosure or copying of the contents of this E-mail or any action taken (or not taken) in reliance on it is unauthorized and may be unlawful. If you are not an addressee, please inform the sender immediately.

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 8 09:19:38 2004

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Hi Gareth,

We use a Nikon D1 with a 60mm Micro Nikkor lens and a Speed Light SB-21 lens-mounted dual
flash. We are extremely pleased with the results. We typically use a polarizer and polarizing
material over the flash to get rid of specular highlights.

Robert Underwood
Sr. Research Scientist
U of Washington

On Fri, 8 Oct 2004, Gareth Morgan wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hi
}
} We are looking at upgrading our facility here for photographing resected organs
} etc at the histopathology department. The new system will be based on digital
} cameras so that we can link the photos to the patient information and diagnosis
} in our database.
}
} What I would like to know is what people are using these days in terms of macro
} lenses, ring flashes (if they exist for the newer cameras) and lighting
} systems, lamps, multiple swan-neck lighting.
}
} Any tips would be appreciated from users and from manufacturers etc.
}
} Thanks
}
} Med vĂ¤nliga hĂ¤lsningar/With best regards
}
} Gareth
}
} http://www.ki.se/biomedlab
} e-mail Gareth.Morgan-at-labmed.ki.se
}
} Tel +46 8 5858 1038
} Fax +46 8 5858 7730
}
} Gareth Morgan MPhil MSc FIBMS,
} Department of Laboratory Medicine (Labmed),
} Karolinska Institute,
} Karolinska University Hospital at Huddinge, F46
} SE 141 86 Stockholm
} Sweden
}
} OBS! BesĂ¶ksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet fĂ¶r
} klinisk patologi och cytologi.
}
} NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10. Clinical
} Histo- and Cytopathology Laboratory.
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 9 12:21:52 2004

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I don't know about gold coating, but titanium-coated silicon wafers are OK
in the autoclave. Another way to sterilise them is to glow-discharge them.

Lesley Weston.

on 07/10/2004 7:04 AM, Garber, Charles A. at cgarber-at-2spi.com wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
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}
----------------------------------------------------------------------------
--} -
}
} -- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --
}
} Mahtab Shahkarami wrote:
} ============================================================================
} =
} Question: I was wondering if anyone has had any experience using Si-chips
} (from Ted Pella) for growing cells. My purpose is to visualize attachment
} appendages of gram-negative bacteria, so a smooth surface is key. I'm not
} sure how much better Si-chips are than glass coverslips, and I also don't
} know how how to sterilize them (autoclave or ethanol?).
} ============================================================================
} I have been lead to believe that at least some are using our own gold coated
} Si-Chips for the growing of cells, see URL
} http://www.2spi.com/catalog/submat/gold-coated-silicon-chips.shtml
}
} The description of the uncoated silicon chips, also used for cell growth, is
} given on URL
} http://www.2spi.com/catalog/standards/silicon-chip-sample.shtml
} The smoothness of the silicon surface is comparable to that of a glass cover
} slip. The silicon used for their production is standard electronics
} industry grade silicon wafers.
}
} The uncoated silicon chips can certainly be autoclaved, however, we don't
} have information on the survivability of the gold coated substrates under
} autoclave conditions. We would appreciate knowing if anyone has such
} information since we are asked that question from time to time.
}
} Disclaimer: SPI Supplies manufactures both uncoated and gold coated silicon
} chip substrates for cell growth applications.
}
} Chuck
} ===================================================
} Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
} President 1-(800)-2424-SPI
} SPI SUPPLIES FAX: 1-(610)-436-5755
} PO BOX 656 e-mail: cgarber-at-2spi.com
} West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com
}
}
} Look for us!
} ############################
} WWW: http://www.2spi.com
} ############################
} ==================================================
}
}

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 10 15:42:36 2004

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}
} Depending on how critical you are of issues like camera versatility,
} performance etc. you might get a long way towards a solution with a
} simpler camera like the Nikon Coolpix 4500. It has remarkable macro
} capability for the price, focussing to about 1 inch from front of
} lens, and there is a so-called ringflash accessory for it too,
} actually a ring of high-intensity white LEDs. I use one of these
} myself, and know many other scientists who swear by them for
} field-recording of specimens ranging from fluorescent gels to plants
} and fungi, even aurora borealis displays are within its capabilities.
}

I endorse the comments about the 4500. I have one, and it's great.

Unfortunately, the Coolpix 4500 seems to have been discontinued, at least in this
country.

Does anyone know why, or whether Nikon is planning to launch a successor?

Anyone from Nikon care to reply?

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 10 16:18:07 2004

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Curious! It is still listed on the Nikon Europe site.
http://www.europe-nikon.com/details.aspx?countryid=20&languageid=22&prodId=117&catId=76
I presume any replacement would be introduced into US first. With
8megapixels perhaps.
Chris

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
To: "Chris Jeffree" {c.jeffree-at-ed.ac.uk} ;
{microscopy-at-msa.microscopy.com}
Sent: Sunday, October 10, 2004 9:45 PM

Hello everyone,

I am currently involved in a research project that is using many different
imaging modalities to look at objects of a variety of sizes. I am interested
in using texture parameters to try to classify this material and was
wondering if there was any existing computer programs or relevant papers
written that could help my with my project.

Please feel free to email me if you think you can help. Thank you all for
your time.

Thomas Sadowski
Southern Connecticut State University

_________________________________________________________________
Don’t just search. Find. Check out the new MSN Search!
http://search.msn.click-url.com/go/onm00200636ave/direct/01/

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 10 18:00:56 2004

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In response to my posting about an hour ago regarding the unavailability of the Coolpix
4500, I have so far received Out of Office Autoreplies from Ian Kitajama, Robert Hull,
Jonathon Dunlap, Tim Maitland, Pei Zou, and John Czernawski, plus an interesting one
apparently generated by antispam software at the office of videbula-at-uol.com.br, which
invited me to respond so that it would not classify my posting as spam!

Guys, can't you understand that by using auto reply you are threatening the continued
existence of this forum?

If everyone who makes a posting knows that their inboxes are going to fill up with
autoreplies, people are going to think twice before posting.

Please have the courtesy to either unsubscribe for the duration of your absences, or to
susbscribe to the list using an alternative email address.

thanks

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 10 19:06:32 2004

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My local Nikon agent says that production of this great model has now ceased, so when
stocks run out, that's it.

So if you're contemplating buying one and if they're still available in your country, buy it
now.

cheers

rtch

} From: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
To: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
Copies to: {microscopy-at-msa.microscopy.com}

A solution might be the Nikon CoolPix 8700. It has the
following technical data:

NIKON COOLPIX 8700 DIGITAL CAMERA
with 8.0 effective megapixels and an 8x Zoom-Nikkor ED lens
Large vari-angle 270° highly transmissible advanced TFT-LCD monitor
for greater visibility - even in daylight

We are offering high quality adapters for digital cameras,
also for the Nikon 8700, so that you can connect it to a
microscope (eyepiece or phototube). If you would like to
know more about the adapters or if you wish to receive a list
of adapters we offer, please contact me.

with best regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

RS} ------------------------------------------------------------------------------
RS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
RS} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
RS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
RS} -------------------------------------------------------------------------------

} }
} } Depending on how critical you are of issues like camera versatility,
} } performance etc. you might get a long way towards a solution with a
} } simpler camera like the Nikon Coolpix 4500. It has remarkable macro
} } capability for the price, focussing to about 1 inch from front of
} } lens, and there is a so-called ringflash accessory for it too,
} } actually a ring of high-intensity white LEDs. I use one of these
} } myself, and know many other scientists who swear by them for
} } field-recording of specimens ranging from fluorescent gels to plants
} } and fungi, even aurora borealis displays are within its capabilities.
} }

RS} I endorse the comments about the 4500. I have one, and it's great.

RS} Unfortunately, the Coolpix 4500 seems to have been discontinued, at least in this
RS} country.

RS} Does anyone know why, or whether Nikon is planning to launch a successor?

RS} Anyone from Nikon care to reply?

RS} cheers

RS} rtch

RS} --
RS} Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
RS} Microanalyst Fax : 64 9 3737435
RS} Department of Geology email : r.sims-at-auckland.ac.nz
RS} The University of Auckland
RS} Private Bag 92019
RS} Auckland
RS} New Zealand

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 11 07:45:26 2004

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A post-doctoral position is available January 2005. This position
requires extensive hands-on experience in transmission/analytical
electron microscopy, scanning electron microscopy, x-ray diffraction,
and other analytical characterization techniques. Additional
experience in materials synthesis and/or devices is highly desirable.
Please contact: Prof. Nitin Padture {nitin.padture-at-uconn.edu} .

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Nitin P. Padture, Ph.D.
Professor
Department of Materials Science and Engineering
Institute of Materials Science
97 N. Eagleville Road
University of Connecticut, Storrs, CT 06269-3136, USA
Phone: (860)486-4206; FAX: (860)486-4745
Email: nitin.padture-at-uconn.edu
Website: http://www.ims.uconn.edu/metal/faculty/padture.htm
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 11 13:35:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (dmwilliams-at-dow.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, October 11, 2004 at 13:25:07
---------------------------------------------------------------------------

Email: dmwilliams-at-dow.com
Name: David M. Williams

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone have a fixation procedure for the whole body perfusion of rabbits? (adult New Zealand White).
(We only have experience with rats).

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 11 16:06:48 2004

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I would like to hear from anyone who has bought a diamond knife in the past
couple of years. I would like to know your experiences with the knife's
quality. I would like feedback about the following brands; Microstar,
Diatome, and Delaware Diamond. Please reply to me privately.

Tom Bargar
Univ. Nebraska Medical Center
Core Electron Microscopy Research Facility
tbargar-at-unmc.edu
402-559-7347

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 12 08:33:49 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jwyffel-at-mindspring.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 12, 2004 at 08:31:03
---------------------------------------------------------------------------

Email: jwyffel-at-mindspring.com
Name: Jennifer

Organization: Clemson University

Title-Subject: [Microscopy] [Filtered] MListserver:carbohydrate

Question: I am searching for a stain/technique to use on shark eggs. There is a carbohydrate jelly found within the egg case and surrounding the ovum much like albumen in chicken eggs. It varies in density or viscosity with location. I would like to image the differences using a carbohydrate stain that would hopefully stain the regions differentially. I will bisect the egg case before staining. Any ideas or suggestions are welcome. Thanks Jennifer

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From MicroscopyL-request-at-ns.microscopy.com Tue Oct 12 10:02:27 2004

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Does anyone out there know what kinds of microscopy are used in evaluating
animal feed for contaminants or pathogens? It seems to me that optical
microscopy would be as valuable a tool as TEM/SEM but I am unsure what role
EDX plays in analysis of animal feed.

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 12 14:44:43 2004

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Listers,

Does anyone have contact information for Consolidated Vacuum Corp.,
or know that they no longer exist? I cannot find contact information
for them, although searching the web did provide a spring 2000
dividend statement and lots of used CVC equipment.
I have an ancient CVC diffusion pump for which I need information.
The odd thing about this pump is that the heater is internal and sits
within the bottom of the tree, in direct contact with the oil. No
normal external pancake heater.
If anyone has information about such a diff pump, I would appreciate
hearing about it.
Thanks.
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 12 21:09:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mburnham-at-kentdenver.org) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, October 12, 2004 at 14:28:01
---------------------------------------------------------------------------

Email: mburnham-at-kentdenver.org
Name: Michael Burnham

Organization: Kent Denver School

Education: 9-12th Grade High School

Location: Denver, Colorado

Question: We have an old but fully functional Zeiss EM9 transmission electron microscope, which has developed a "flicker" or pulse in the beam. This intermittent pulse momentarily increases the intensity of the beam which ruptures the specimen. I've tried various remedies---replace the filament, checking contacts and tubes, etc. but to no avail. I am about to replace the gun with an old-stock spare; however, I'd truly appreciate suggestions (including if anyone knows of a technician in the Denver area who still might work on old teaching TEM's).

Thank you,
Michael Burnahm
Science Chair
Kent Denver School
Englewood, CO 80113
303-770-7660 ex. 203

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 13 02:13:45 2004

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Hi,

In the past few years I have used this mailing lists to discuss numerous
microscopy issues and I have learned a lot from the people who are a
member of this community.

This mailing list is mostly used by people who work in microscopy and
who have a background in using a microscope in a "traditional" way. Most
people know about Koehler illumination, the meaning of N.A. for
resolution when doing microscopy with the naked eye. For digital
microscopy, most people have a basic understanding of Nyquist sampling
and the spatial requirements for image quantification. Young scientist
always get help from the community on these issues.

Traditional people using a microscope in biology had a background in
biology, medicine, etc. and some basic understanding of morphology and
shape. Microscopy and morphology were a bit out of focus due to the
emphasis on genomics and proteomics, but HCS brought it back. However
with the advent of High Content Screening (HCS), biochemists started
using devices based on optical microscopes without any basic training in
(digital) optical microscopy or morphology. Studying a cell or tissue
requires some basic knowledge of morphology and the interaction of light
with matter and the optics of a microscope.

Modern software design sort of "uncouples" the HCS world from the
optical reality of the optical instrument, but basicaly these machines
are optical microscopes and adhere to the same optical principles as a
"traditional" microscope. In my opinion using such an instrument without
any basic understanding op digital optical microscopy makes no sense.

My question is, how do microscopists who are trained in "classical"
microscopy explain the basics of microscopy to biochemists ? Are there
textbooks or educational books written on biological optical microscopy
with the non-morphologist in mind ?

Regards,

Peter

P.S I do not want to offend anyone, but it is something I experienced
personally and I am at a loss how to deal with it.

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 13 07:32:42 2004

Contents Retrieved from Microscopy Listserver Archives
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Michael,

I have a Zeiss EM900 and have/had a similar problem. To eliminate the
flicker I changed the objective aperture to the next larger one (50um
?). Our Zeiss repair person thinks the smaller aperture was being
contaminated too quickly and causing a charge build up. The high
voltage was checked and no variations were noted. Since the larger
aperture, the flicker has not reappeared.

Best of luck,

Ed

Edward Calomeni
Director EM Lab
Ohio State University - Pathology
M018 Starling Loving Hall
320 W. 10th Ave.
Columbus, OH 43210-1240
614-293-5580 (office)
614-293-8806 (lab)
calomeni-1-at-medctr.osu.edu

} } } by way of Ask-A-Microscopist {mburnham-at-kentdenver.org} 10/12/2004
10:13:13 PM } } }

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The Microscopy ListServer -- Sponsor: The Microscopy Society of
America

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mburnham-at-kentdenver.org) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Tuesday, October 12, 2004 at 14:28:01
---------------------------------------------------------------------------

Email: mburnham-at-kentdenver.org
Name: Michael Burnham

Organization: Kent Denver School

Education: 9-12th Grade High School

Location: Denver, Colorado

Question: We have an old but fully functional Zeiss EM9 transmission
electron microscope, which has developed a "flicker" or pulse in the
beam. This intermittent pulse momentarily increases the intensity of the
beam which ruptures the specimen. I've tried various remedies---replace
the filament, checking contacts and tubes, etc. but to no avail. I am
about to replace the gun with an old-stock spare; however, I'd truly
appreciate suggestions (including if anyone knows of a technician in the
Denver area who still might work on old teaching TEM's).

Thank you,
Michael Burnahm
Science Chair
Kent Denver School
Englewood, CO 80113
303-770-7660 ex. 203

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 13 08:39:58 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rangari0-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 12, 2004 at 22:51:23
---------------------------------------------------------------------------

Email: rangari0-at-yahoo.com
Name: vk

Organization: tuskegee university

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi all
Can any one tell me how to thin the diamond film or cross section the diamond film for HRTEM
Thank you for your kind help

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 13 13:32:32 2004

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You should use diamond abrasive paper to ground the sample to about
40microns, then ion-mill the sample to electron transparent!

Changhui

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 13 16:06:43 2004

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You don't mention your substrate. I assume that this is a diamond film on a substrate such as silicon.

If your film is on a Si substrate, then I highly recommend the small angle cleavage technique or Microcleave technique. Check the South Bay Technology website for their microcleave kit and associated PDF files by John McCaffrey and myself.

If you must do ion milling, then you should be aware that carbon films do not ion mill very well with Ar beams. However, if you have a low angle mill, then things are alleviated quite a lot. One of the things that people have done to overcome the low milling rate of carbon is to add a little O2 into the Ar. Try 20%.) This is essentially a reactive etch for you. I have a paper in the MRS number four series on TEM sample prep that shows the relative differences of ion milling rates with Ar, Ne, Ar+O2, and Ne+O2 gases in a Gatan Duomill at 10 degrees. We used AFM to measure the relative heights of a DLC film on a TiC film on a silicon substrate. The idea was to try to match the mass of both the C and Si with the gas as close as possible. The best results were obtained using Ne+O2. Ne did a good job also.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: rangari0-at-yahoo.com [mailto:rangari0-at-yahoo.com]
Sent: Wednesday, October 13, 2004 9:44 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rangari0-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 12, 2004 at 22:51:23
---------------------------------------------------------------------------

Email: rangari0-at-yahoo.com
Name: vk

Organization: tuskegee university

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hi all
Can any one tell me how to thin the diamond film or cross section the diamond film for HRTEM
Thank you for your kind help

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 13 16:12:23 2004

Contents Retrieved from Microscopy Listserver Archives
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Is there anyone that can point me in the direction of some papers that show the modeling of EELS spectral lines from the density of states calculations for crystalline oxides. I am particularly interested in TiO2. If you know of any programs that are available, I would also be interested in that.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 09:21:47 2004

Contents Retrieved from Microscopy Listserver Archives
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Well, here I am pulling my hair out again, trying to get things to work as I
would like.. I am currently trying to get TEM images in 16-bit Digital
Micrograph 3 format into 8-bit tiff format - which I need to do since the
images are held centrally on a server, and need to be read by lots of
internal customers using their own PCs. I have at my disposal PhotoShop 4.0
and 5.0 with the Reindeer Games image processing toolkit, Thumbs Plus 4.5,
as well as ImageJ and Irfan view.

The problem - only a small amount of the 16-bit dynamic range is present
in the image, and the levels used vary from image to image. 'Auto levels'
in PhotoShop doesn't work as well as I thought it would, since it goes too
far and saturates the bright and dark pixels. I can adjust things as I
would like manually using PhotoShop(minimum used level = 0, maximum used
value = 65535, then convert to 8-bit), but this is pretty tedious to do for
every image. Nothing else seems to be able to do what I want. I can't be
the first person to have this problem - so does anyone know of a solution
(preferably a free one, of course)?

Many thanks in advance

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Inc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

=======================================================================
This e-mail is intended for the person it is addressed to only. The
information contained in it may be confidential and/or protected by
law. If you are not the intended recipient of this message, you must
not make any use of this information, or copy or show it to any
person. Please contact us immediately to tell us that you have
received this e-mail, and return the original to us. Any use,
forwarding, printing or copying of this message is strictly prohibited.
No part of this message can be considered a request for goods or
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From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 10:31:09 2004

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Richard

In more recent versions of Photoshop, and in the Reindeer Graphics Optipix
plugins, you can set the amount of "tail clipping" that occurs - the fraction of
the pixels that are set to black and white by adjusting the limits on your
image. That feature was not present in Photoshop 4 or 5. Probably the best
(fast, relatively cheap) approach would be to upgrade to the latest Photoshop, and
then create a simple action that opens an image, auto-adjusts the levels with
a small tail clip (e.g., 0.01% at each end), converts to 8 bits, and saves the
image into a new folder. That can be run as a batch while you do something
else, and will produce a new set of images for your server without replacing the
originals,just in case someone needs the full 16 bit dynamic range or the
actual original grey scale values later on.

John Russ
======
In a message dated 10/14/04 11:22:52 AM, richard.beanland-at-bookham.com writes:

} ... {snip} I am currently trying to get TEM images in 16-bit Digital
}
} Micrograph 3 format into 8-bit tiff format - which I need to do since the
}
} images are held centrally on a server, and need to be read by lots of
}
} internal customers using their own PCs. I have at my disposal PhotoShop
} 4.0
}
} and 5.0 with the Reindeer Games image processing toolkit, Thumbs Plus 4.5,
}
} as well as ImageJ and Irfan view.
}

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 10:52:26 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I think I might have the record for a problem solved by the ListServer - 7
minutes from posting to solution! Many thanks indeed John, and unabashed
adoration for Nestor for running this great resource..

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: 14 October 2004 16:35
To: richard.beanland-at-bookham.com; microscopy-at-msa.microscopy.com

I would like to know if anyone has experience in getting a Digital Single Lens
Reflex camera (DSLR) to provide a "live" preview for display on a Computer.

We purchased a Nikon D-70 and Nikon Image Capture 4.1 software which allows
remote control of the camera through a PC. After initial tests it seems that
it is impossible to acquire even a low resolution "live" preview with this
camera.

Capturing an image through the computer interface of Nikon Capture 4.0 is
simple but the lack of a preview (even low-res) is quite inconvenient.

In theory it should be possible for the camera to be controlled such that the
mirror is held in the open position and the CCD continuously dumps the data to
the PC. This method doesn't seem like something that is supported by standard
OEM provided solutions or is as easy as we'd first hoped.

Our intermediate solution is to place a crosshair occular on the scope which
will be used to make the image and camera parfocal before simply taking a
picture. While it works we'd really like to get a live preview and make it
ridiculously simple to use (which was the reason for picking this camera
initially.)

If anyone has any suggestions or has experienced this problem I'd greatly
appreciate your help.

Thanks,
Dustin Grzesik

Research Technician
Analytical Imaging Facility
Albert Einstein College of Medicine

--
"Strong, light, cheap. pick two." Keith Bontrager

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 14:22:02 2004

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Richard
Auto-level function in the Photoshop works fine to me for most DM
images. I also use macros (action) function to convert many files
altogether as Jon Russ suggested. Auto-level function does not work well
if you have very bright or dark area on your picture, then you have to
adjust levels manually (and I don't think you could use automatization
there). I also find that DM did good job choosing B&W balance when convert
images into 8-bit using export-} tiff option. So, I usually create two sets
of images (16 and 8-bit) at the level of DM, not Photoshop. The problem
with DM is that I have difficulties to automate the process. DM has quite
extended macros language and it supposed to be quite easy to write macros
for automatic conversion 16 into 8-bit and save into another
directory. But, perhaps, I am too lazy to do it well, so it does not work
in my hands. If somebody already crossed that border and has functioning
macros and willing to share, I would be grateful to have it. Have a good
day, Sergey.

At 03:22 PM 10/14/2004 +0100, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 16:05:01 2004

Contents Retrieved from Microscopy Listserver Archives
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Although it may not be too helpful for PC users, the incredibly
low-cost "Graphics Converter" program which I run on my mac does a good
job reading the DM files for me. It also has a batch function for
converting them all at once.

Stuart

On Oct 14, 2004, at 2:27 PM, Sergey Ryazantsev wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Richard
} Auto-level function in the Photoshop works fine to me for most DM
} images. I also use macros (action) function to convert many files
} altogether as Jon Russ suggested. Auto-level function does not work
} well if you have very bright or dark area on your picture, then you
} have to adjust levels manually (and I don't think you could use
} automatization there). I also find that DM did good job choosing B&W
} balance when convert images into 8-bit using export-} tiff option. So,
} I usually create two sets of images (16 and 8-bit) at the level of DM,
} not Photoshop. The problem with DM is that I have difficulties to
} automate the process. DM has quite extended macros language and it
} supposed to be quite easy to write macros for automatic conversion 16
} into 8-bit and save into another directory. But, perhaps, I am too
} lazy to do it well, so it does not work in my hands. If somebody
} already crossed that border and has functioning macros and willing to
} share, I would be grateful to have it. Have a good day, Sergey.
}
} At 03:22 PM 10/14/2004 +0100, you wrote:
}
}
} } ----------------------------------------------------------------------
} } --------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------
} } ---------
} }
} } Well, here I am pulling my hair out again, trying to get things to
} } work as I
} } would like.. I am currently trying to get TEM images in 16-bit
} } Digital
} } Micrograph 3 format into 8-bit tiff format - which I need to do since
} } the
} } images are held centrally on a server, and need to be read by lots of
} } internal customers using their own PCs. I have at my disposal
} } PhotoShop 4.0
} } and 5.0 with the Reindeer Games image processing toolkit, Thumbs Plus
} } 4.5,
} } as well as ImageJ and Irfan view.
} }
} } The problem - only a small amount of the 16-bit dynamic range is
} } present
} } in the image, and the levels used vary from image to image. 'Auto
} } levels'
} } in PhotoShop doesn't work as well as I thought it would, since it
} } goes too
} } far and saturates the bright and dark pixels. I can adjust things as
} } I
} } would like manually using PhotoShop(minimum used level = 0, maximum
} } used
} } value = 65535, then convert to 8-bit), but this is pretty tedious to
} } do for
} } every image. Nothing else seems to be able to do what I want. I
} } can't be
} } the first person to have this problem - so does anyone know of a
} } solution
} } (preferably a free one, of course)?
} }
} } Many thanks in advance
} }
} } Richard
} }
} } _______________________________
} } Richard Beanland
} } Analytical Services
} } Bookham Inc
} } Caswell,
} } Towcester,
} } Northamptonshire NN12 8EQ
} } UK
} } Tel: +44 (0) 1327 356362
} } Fax: +44 (0) 1327 356775
} } http://www.bookham.com
} }
} }
} } ======================================================================
} } =
} } This e-mail is intended for the person it is addressed to only. The
} } information contained in it may be confidential and/or protected by
} } law. If you are not the intended recipient of this message, you must
} } not make any use of this information, or copy or show it to any
} } person. Please contact us immediately to tell us that you have
} } received this e-mail, and return the original to us. Any use,
} } forwarding, printing or copying of this message is strictly
} } prohibited.
} } No part of this message can be considered a request for goods or
} } services.
} } ======================================================================
} } =
}
}

Prof. Stuart McKernan
IT Characterization Facility, University of Minnesota
E-mail : stuartm-at-umn.edu
12 Shepherd Labs,
         Office: (612) 624-6009
100 Union Street S. E., Minneapolis, MN 55455             Lab:
(612) 626-7594

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 16:34:48 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (monica.iliescu-at-polymtl.ca) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, October 14, 2004 at 16:30:39
---------------------------------------------------------------------------

Email: monica.iliescu-at-polymtl.ca
Name: Monica ILIESCU

Organization: Ecole Polytechnique

Title-Subject: [Microscopy] [Filtered] QX-102 capsules for ESEM

Question: Dear colleagues,

I would like to learn if someone of you use QX-102 capsules for ESEM imaging of wet samples (namely, biological) at atmospheric pressure. QuantomiX Inc manufactured like capsules in disposable package. My question is if these capsules can be used again after one experiment, i.e. if they can be used subsequently for many samples when sterile conditions are not imposed.

Thank you,
Monica Iiescu, PhD

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From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 16:35:31 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (breath999-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, October 13, 2004 at 14:47:24
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Email: breath999-at-yahoo.com
Name: Peter Bradley

Organization: UCLA

Title-Subject: [Microscopy] [Filtered] MListserver: Formaldehyde/PBS - old works better?

Question: I'm hoping someone here can help me out with storage of formaldehyde in PBS. I found out a person here was using fixative (3.7% formaldehyde in PBS) stored in the fridge for about 2-3 weeks. I told him to toss it out and only use fresh. It turns out that staining (IFA) with one antibody is beautiful in 2 week old but destroyed in fresh fix. We have recently tried various titrations of % formald, time, etc. but none give the nice staining seen in 2 week old formald (1 week is not long enough). I have seen a bit about polymerization, etc, but I am concerned that an artifact could be created by the old fix.

Any help would be greatly appreciated.
Thanks in advance,
Peter

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From MicroscopyL-request-at-ns.microscopy.com Thu Oct 14 16:38:10 2004

Contents Retrieved from Microscopy Listserver Archives
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} From: Day, Jeff
Sent: Wednesday, October 13, 2004 10:29 AM
To: 'Microscopy-at-MSA.Microscopy.Com'

Monica,
They are single use items at about $40 a capsule. You don't need ESEM to
use them, just a good backscatter detector.
Gianni Torraca
Analytical Sciences
AMGEN

-----Original Message-----
} From: monica.iliescu-at-polymtl.ca [mailto:monica.iliescu-at-polymtl.ca]
Sent: Thursday, October 14, 2004 2:39 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (monica.iliescu-at-polymtl.ca) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday,
October 14, 2004 at 16:30:39
---------------------------------------------------------------------------

Email: monica.iliescu-at-polymtl.ca
Name: Monica ILIESCU

Organization: Ecole Polytechnique

Title-Subject: [Microscopy] [Filtered] QX-102 capsules for ESEM

Question: Dear colleagues,

I would like to learn if someone of you use QX-102 capsules for ESEM imaging
of wet samples (namely, biological) at atmospheric pressure. QuantomiX Inc
manufactured like capsules in disposable package. My question is if these
capsules can be used again after one experiment, i.e. if they can be used
subsequently for many samples when sterile conditions are not imposed.

Thank you,
Monica Iiescu, PhD

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From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 10:08:19 2004

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Hello Marie-Claude,
I have some chemists doing spectroscopy using an inverted microscope
base in our facility. Ours is a 12V halogen lamp, but thier tests
indicate a 4 hour warm up period for maximum stability. Having the lamp
power supply rheostat adjusted to provide nearly highest output (highest
color temperture) aids in warm up. Also, a new (high-quality) bulb might
help in your case.
Regards,
Karl

Marie-Claude Bélanger wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Dear All,
}
} I've recently started taking birefringence photographs of Congo Red
} stained tissue. I've noticed that over time, the very same field
} doesn't appear the same, and that the labeled surface varies up to 25%.
}
} Everything being very stable (all screws firmly screwed, polarizer
} glued to its base), I'm wondering if anyone has performed a test to
} check the warm-up period of a halogen 6 volt lamp. The company who
} sells the lamp says 5 to 10 minutes, but could it be longer?
}
} Thank you!
}
} Marie-Claude Belanger
}
} _________________________________________________________________
} Des mécanismes de contrôle parental puissants permettent ŕ votre
} enfant de découvrir tout ce qu’Internet a ŕ offrir.
} http://join.msn.com/?pgmarket=fr-ca&page=features/parental&ST=1&xAPID=1983&DI=2043
} Commencez dčs maintenant ŕ profiter de tous les avantages de MSN
} Premium et obtenez les deux premiers mois GRATUITS*.
}

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 12:03:59 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi,

I am one of those stubborn Mac users and I need an advise in dealing with
Gatan DigitalMicrograph images.

We use DigitalMicrograph v.3.7 on a Windows PC to acquire TEM images.
I have DigitalMicrograph v.3.4 on a Mac and I want to use my Mac to work
with the image files.

The problem is that the Mac DM3.4 does not recognize the .dm3 file format
from the PC. Usually I save two versions of each file one in .dm3 format and
one in TIF, which I can use on the Mac. The problem is that this is a time
consuming procedure when dealing with a large number of files.

I have other software such as ImageJ and Graphic Converter on my Mac and I
can open the .dm3 files with them. The problem is that the annotation is
lost during the transfer.

The question: Is there a way to convert multiple files as batch process from
dm3 into TIF format without opening and saving each file individually,
where the original annotation in the files and the file names will remain
unchanged?

Thanks,

Krassimir.

P.S. Switch to PC is not regarded as a valid answer.

---------------------------------------------------------
Krassimir N. Bozhilov, PhD
EM Scientist and Manager
Central Facility for Advanced Microscopy and Microanalysis
University of California
Riverside, CA 92521

Tel 951 827 2998
Fax 951 827 2489
--------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 13:32:39 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi Peter:

I don't think formalin in PBS would 'go bad' or lose much activity
in 2 weeks in the 'frig. Even formaldehyde made fresh from
paraformaldehyde -which I was always taught must be made fresh- lasts
for several weeks in the cold. That was published in the last few years
but I can't find the reference, if anyone has it please send it to me.
There are several variables we need to know before we can make an
informed decision. How long was the tissue fixed (formalin works
slowly)? How old was the formaldehyde used to make the fix-PBS mixture?
Was the stock bottle already weakened by polymerization of formalin?
Fixed in the cold or room temp? What kind of tissue? Hoiw about the rest
of the processing? What antibody and detection system? How many trials
did you do with each fix? It sounds like your sample size for the 'old,
cold' fix is one, hardly sufficient to draw a valid conclusion.

Geoff

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 13:53:51 2004

Contents Retrieved from Microscopy Listserver Archives
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On Oct 15, 2004, at 10:08 AM, K.N. Bozhilov wrote:

} I am one of those stubborn Mac users and I need an advise in dealing
} with
} Gatan DigitalMicrograph images.
}
} We use DigitalMicrograph v.3.7 on a Windows PC to acquire TEM images.
} I have DigitalMicrograph v.3.4 on a Mac and I want to use my Mac to
} work
} with the image files.
}
} The problem is that the Mac DM3.4 does not recognize the .dm3 file
} format
} from the PC. Usually I save two versions of each file one in .dm3
} format and
} one in TIF, which I can use on the Mac. The problem is that this is a
} time
} consuming procedure when dealing with a large number of files.
}
} I have other software such as ImageJ and Graphic Converter on my Mac
} and I
} can open the .dm3 files with them. The problem is that the annotation
} is
} lost during the transfer.
}
} The question: Is there a way to convert multiple files as batch
} process from
} dm3 into TIF format without opening and saving each file individually,
} where the original annotation in the files and the file names will
} remain
} unchanged?
}
Dear Krassimir,
Could you please post the responses you get so us other stubborn Mac
users can convert our files? If this is done using a GATAN script in
DM, could it also be used to convert the data type to unsigned, 2-byte?
TIA.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 15:37:09 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

We have found that many of the standard power supplies provided by the
microscope manufacturers are noticeably unstable as measured with tube or
CCD camera time lapse imaging of cells by phase contrast, at least with
the power supply from the wall of 102 to 118 VAC here in NYC.

On the microscope stations where we have needed to rectify this, we have
purchased special stable power sources (AC to 12V DC conversions) instead
of using the ones supplied in the bases of the microscopes.

-Michael

On Fri, 15 Oct 2004, Karl Garsha wrote:

} Hello Marie-Claude,
} I have some chemists doing spectroscopy using an inverted microscope
} base in our facility. Ours is a 12V halogen lamp, but thier tests
} indicate a 4 hour warm up period for maximum stability. Having the lamp
} power supply rheostat adjusted to provide nearly highest output (highest
} color temperture) aids in warm up. Also, a new (high-quality) bulb might
} help in your case.
} Regards,
} Karl
}
} Marie-Claude Bélanger wrote:
}
} } Dear All,
} }
} } I've recently started taking birefringence photographs of Congo Red
} } stained tissue. I've noticed that over time, the very same field
} } doesn't appear the same, and that the labeled surface varies up to 25%.
} }
} } Everything being very stable (all screws firmly screwed, polarizer
} } glued to its base), I'm wondering if anyone has performed a test to
} } check the warm-up period of a halogen 6 volt lamp. The company who
} } sells the lamp says 5 to 10 minutes, but could it be longer?
} }
} } Thank you!
} }
} } Marie-Claude Belanger
} }
} } _________________________________________________________________
} } Des mécanismes de contrôle parental puissants permettent ŕ votre
} } enfant de découvrir tout ce qu’Internet a ŕ offrir.
} } http://join.msn.com/?pgmarket=fr-ca&page=features/parental&ST=1&xAPID=1983&DI=2043
} } Commencez dčs maintenant ŕ profiter de tous les avantages de MSN
} } Premium et obtenez les deux premiers mois GRATUITS*.
} }
}
} --
} Karl Garsha
} Light Microscopy Specialist
} Imaging Technology Group
} Beckman Institute for Advanced Science and Technology
} University of Illinois at Urbana-Champaign
} 405 North Mathews Avenue
} Urbana, IL 61801
} Office: B650J
} Phone: 217.244.6292
} Fax: 217.244.6219
} Mobile: 217.390.1874
} www.itg.uiuc.edu
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 18:31:32 2004

Contents Retrieved from Microscopy Listserver Archives
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Greetings:

We just got a spiffy new inverted light microscope. It is in a multiple
user lab and most will want to use a 63X oil objective.

Most of my experience is with standard upright scopes where adding the oil
is pretty up front and easy, slide stays on the stage, swing objective out,
add oil, swing objective back in. This inverted thing is a little more
complicated.

Some users get the objective in position, remove their slide, add oil, then
replace the slide. Works OK, but seems like slide might not land back in
exactly the same spot and a once in a lifetime location might be lost.

So, any advice or clever techniques. I have thought of a long probe to
reach under the slide, but could be a mess. Have read some advice about
rotating objective to the side, adding oil, then rotating back quickly
before oil slips off.

Not a big deal, but seems like there should be a better way.

Thanks

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 18:35:50 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Krassimir and scripters,
I have the same problem with the DM for Mac. I have found that converting
to DM2 format will allow me to open my DM3-PC files on the Mac. Also, for
full 16-bit data, I have found the gfx format to be quite portable. Gatan
is constantly changing how it saves 16-bit TIF files that you never know
what you are going to get. The Gatan script below will convert a directory
full of DM3 files to DM2 format. It does so by using the
"ImageDisplayExportToFile" command. By changing a few variables (see
script) it will save in any format Gatan supports.

I have found that these script files do not cut and paste well from email.
You may need to clean up the line breaks a bit to get it to work correctly.
If necessary, I can send you the script as an attachment.

Hope this helps, Ray

/*
BatchDirFileConvert.s

The basic idea is to scan through a directory for DM files and convert them
to a new format
The script uses the "void ImageDisplayExportToFile( ImageDisplay imgDisp,
String format, String file_name ) "
script command. Here you give the export format in the string "format".
Gatan changes how this works from version to version so use at your own
risk.

Copyright 10/15/2004 Ray D. Twesten - University of Illinois

*/

//******************************
//Modify these strings to change format.
// See SaveAs or Export menu item for correct strings
//******************************
string format = "Gatan 2.5 Format" // Good for sending to Mac version of
DM
string extension = ".dm2"
string saveDir = "DM2"

//
// string format = "Fixed Format" // Good all around 16-bit format
// string extension = ".gfx"
// string saveDir = "GFX"

//
// Get image path and create tag group to hold file names:
//
string fileName = ""
if(!OkCancelDialog("Choose Any file in Dir to Open")) exit(0)
if(!OpenDialog(fileName))
exit(0)
string dirName = PathExtractDirectory( fileName, 0 )

Taggroup dir = GetFilesInDirectory( dirName, 1 )
number numfiles = TagGroupCountTags( dir )

string newPath = PathConcatenate( dirName, saveDir)
if( !DoesDirectoryExist( newPath ))
CreateDirectory( newPath )

//
// Record keeping
//
OpenResultsWindow()
Result("\n\n" + DateStamp() + "\n")

//
// Save image loop:
//
number savedImageCounter = 0
string curImg
number i
string extn

image front

for(i = 0; i { numfiles; i++)
{
if(!TagGroupGetTagAsString( dir, "[" + i + "]:Name", curImg ))
throw("Does Not Exist "+ i)
curImg = PathConcatenate( dirName, curImg)
extn = PathExtractExtension(curImg, 0)
Result("\nTrying: " + curImg + "\n")

if( extn == "dm3" || extn == "DM3")
{
front:= OpenImage(curImg)
ShowImage(front) // Needed to have valid image display

curImg = PathConcatenate( newPath, PathExtractBaseName(curImg, 0) +
extension)
Result("image: " + curImg )
try
ImageDisplayExportToFile( front.ImageGetImageDisplay(0) , format,
curImg )
catch
{
Result("\nfile conversion was interrupted\n" + \
"possible reason: complex or RGB image
encountered\n" + \
Datestamp() + "\n")
throw("Ouch !")
}
Result(" (saved)\n")
deleteImage(front)
savedImageCounter = savedImageCounter + 1
OpenAndSetProgressWindow( "image: " +savedImageCounter,"saved
as",extension +" file")
} //End of OpenSave if loop

} //End of loop trough tags

Result("end " + DateStamp() + "\n")

// End BatchDirFileConv.s
//**********************************************************8

Ray D. Twesten, PhD.
Center for Microanalysis of Materials
Seitz Materials Research Laboratory
104 S. Goodwin Ave., Urbana, IL 61801
+1 217 244-6177 (Fax -2278)

-----Original Message-----
} From: K.N. Bozhilov [mailto:bozhilov-at-ucr.edu]
Sent: Friday, October 15, 2004 12:08 PM
To: microscopy-at-msa.microscopy.com

Hi,

I am one of those stubborn Mac users and I need an advise in dealing with
Gatan DigitalMicrograph images.

We use DigitalMicrograph v.3.7 on a Windows PC to acquire TEM images.
I have DigitalMicrograph v.3.4 on a Mac and I want to use my Mac to work
with the image files.

The problem is that the Mac DM3.4 does not recognize the .dm3 file format
from the PC. Usually I save two versions of each file one in .dm3 format and
one in TIF, which I can use on the Mac. The problem is that this is a time
consuming procedure when dealing with a large number of files.

I have other software such as ImageJ and Graphic Converter on my Mac and I
can open the .dm3 files with them. The problem is that the annotation is
lost during the transfer.

The question: Is there a way to convert multiple files as batch process from
dm3 into TIF format without opening and saving each file individually,
where the original annotation in the files and the file names will remain
unchanged?

Thanks,

Krassimir.

P.S. Switch to PC is not regarded as a valid answer.

---------------------------------------------------------
Krassimir N. Bozhilov, PhD
EM Scientist and Manager
Central Facility for Advanced Microscopy and Microanalysis
University of California
Riverside, CA 92521

Tel 951 827 2998
Fax 951 827 2489
--------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 15 19:51:17 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

I am using an inverted fluorescent microscope and I do not seem to have
this kind of problems...
I usually put the oil before I place the slide.

I however have enough space around the objective to swing it out just a
little bit, add the oil with no risk of slipping off and than swing it
back in.
To make my life easier, I also have a sort of opening on the stage that is
made to add the oil.

I can send pictures of my stage if you want.

Hope that helps,

Anne-Laure

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Le Ny Anne-Laure
Grad Student Chemical engineering
University of Southern California
PCE 310
Tel: 213-740-1320
Cell: 626-840-5456
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

On Fri, 15 Oct 2004, Jon Krupp wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Greetings:
}
} We just got a spiffy new inverted light microscope. It is in a multiple
} user lab and most will want to use a 63X oil objective.
}
} Most of my experience is with standard upright scopes where adding the oil
} is pretty up front and easy, slide stays on the stage, swing objective out,
} add oil, swing objective back in. This inverted thing is a little more
} complicated.
}
} Some users get the objective in position, remove their slide, add oil, then
} replace the slide. Works OK, but seems like slide might not land back in
} exactly the same spot and a once in a lifetime location might be lost.
}
} So, any advice or clever techniques. I have thought of a long probe to
} reach under the slide, but could be a mess. Have read some advice about
} rotating objective to the side, adding oil, then rotating back quickly
} before oil slips off.
}
} Not a big deal, but seems like there should be a better way.
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 16 02:32:45 2004

Contents Retrieved from Microscopy Listserver Archives
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:
: We have found that many of the standard power supplies provided by
the
: microscope manufacturers are noticeably unstable as measured with
tube or
: CCD camera time lapse imaging of cells by phase contrast, at least
with
: the power supply from the wall of 102 to 118 VAC here in NYC.
:
: On the microscope stations where we have needed to rectify this,
we have
: purchased special stable power sources (AC to 12V DC conversions)
instead
: of using the ones supplied in the bases of the microscopes.
:
: -Michael
:
: On Fri, 15 Oct 2004, Karl Garsha wrote:
:
: } Hello Marie-Claude,
: } I have some chemists doing spectroscopy using an inverted
microscope
: } base in our facility. Ours is a 12V halogen lamp, but thier
tests
: } indicate a 4 hour warm up period for maximum stability. Having
the lamp
: } power supply rheostat adjusted to provide nearly highest output
(highest
: } color temperture) aids in warm up. Also, a new (high-quality)
bulb might
: } help in your case.
: } Regards,
: } Karl
: }
For low voltage bulbs I have solved this problem in the past with a
lead acid auto battery on a trickle charger with a resistor to
reduce the voltage to what ever I need on the lamp. Then you only
have to wait until the resistor heats up until the light is stable.
It also gets rid of the very slight 120 Hz flicker on the bulb if
you are using AC.

The flicker is not normally a problem as no camera will pick it up
and your eyes will never see it but it can be in some imaging if the
capture is fast enough.

For 110 VAC I have generaly found the unconditioned power better
than that going thourgh so called power conditioners. Put some surge
protectors accorss the line and try it as is.

Gordon
Gordon Couger

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 16 12:51:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Jonathan,

I've found the "move the objective" to be the best way to oil lens on
an inverted 'scope.
But, something else you might want to do: go to someplace like
WalMart or the like and buy a bag of little hair scrunchies. They
just fit the lenses, and even come color-coded. This will keep the
oil from running down the lenses into threads, the turret, and so
forth.

Phil

} Greetings:
}
} We just got a spiffy new inverted light microscope. It is in a multiple
} user lab and most will want to use a 63X oil objective.
}
} Most of my experience is with standard upright scopes where adding the oil
} is pretty up front and easy, slide stays on the stage, swing objective out,
} add oil, swing objective back in. This inverted thing is a little more
} complicated.
}
} Some users get the objective in position, remove their slide, add oil, then
} replace the slide. Works OK, but seems like slide might not land back in
} exactly the same spot and a once in a lifetime location might be lost.
}
} So, any advice or clever techniques. I have thought of a long probe to
} reach under the slide, but could be a mess. Have read some advice about
} rotating objective to the side, adding oil, then rotating back quickly
} before oil slips off.
}
} Not a big deal, but seems like there should be a better way.
}
} Thanks
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu

--
Philip Oshel
Supervisor, AMFSC and BBPIC microscopy facilities
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706 - 1284
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 17 11:42:41 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (diller-at-stefan-diller.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, October 17, 2004 at 07:48:38
---------------------------------------------------------------------------

Email: diller-at-stefan-diller.com
Name: Stefan Diller

Organization: Photography

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Is there anyone out there who can give me advice in using an EDAX 9100 system on a Philips EM 420?
Especially I am looking for tips how to do linescans or element mapping... My manual is not so clear in this point.

The system has a digital ratemeter 9201 which - I understand - es necessary to aquire linescans and element-maps.

Does anybody know what the latest available software version for this system is and if there is any possibility to use "modern" printers for printing spectra and other data?

Any advice is greatly appreciated.

Stefan Diller

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 17 11:43:13 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (innap-at-savion.huji.ac.il) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Sunday, October 17, 2004 at 11:23:10
---------------------------------------------------------------------------

Email: innap-at-savion.huji.ac.il
Name: Inna Popov

Organization: The Hebrew University of Jerusalem

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear All,
I would appreciate any help and recommendations in preparation of metallographic sample from the extruded polymer wire of 0.3-0.5 mm dia. The polymer wire is a composite material: polyethylene matrix strenghthened by ultra high molecular weight polyethylene fibers. The purpose of the study is to see the interface between the fibers and the matrix.
Do you have any idea of how to polish cross sectional sample (I need them in two orthogonal directions) from this kind of material?
Thank you in advance,
Inna

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From MicroscopyL-request-at-ns.microscopy.com Mon Oct 18 14:26:59 2004

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Here is a summary of all responses so far.

The new version of Digital Micrograph 3.9 (GMS1.4) can do batch conversion
to tif, jpg, and bmp formats.

There is also a plug-in for older versions of DM which can be used to
convert to the above formats and also to dm2 format.

Problems still remaining:

Batch conversion to dm2 deletes all annotations. Scale bar is not the issue
since the information about the pixel size is still preserved.

Conversion to non-Gatan format burns the annotations in the image data and
annotations cannot be separated or moved if desired. Also such conversions
result in certain loss of data in general.

Saving directly to dm2 is similar to converting to tif or jpeg, with the
advantage that no data loss occurs, but magnification information is lost
and all annotations become permanent part of the image data.

Conclusion: there is no perfect alternative to using Digital Micrograph on a
Windows PC and working with dm3 files.

Thank you for all inputs.

Krassimir.

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 18 16:17:01 2004

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Our lab has routinely processed samples according to the methods
posted at http://www.micro.wisc.edu/smith in the past without
artifacts, but recently we have encountered an unknown contaminant
seen as an electron dense (opaque) amorphic precipitate. Please visit
the web-site listed above for examples of the artifact and detailed
processing methods. We would like your opinions as to the source of
this contamination so we might avoid it in future experiments. Your
comments are much appreciated.

Ben August
U.W. Electron Microscopy Facility
Medical School
University of Wisconsin - Madison
bkaugust-at-facstaff.wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 18 16:19:22 2004

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Could someone provide the digital equivalency (in terms of
resolution) of 3.25 x 4 inch TEM film.

I have read that a 6 megapixel digital file has the resolution
capability of a 35 mm grayscale negative. If this is true, then an 18
megapixel digital file would be equivalent to a TEM grayscale
negative in terms of resolution capability.

I was thinking (based on darkroom enlargement capabilities of TEM
films) that a 180 MP digital file would be more likely to exhibit the
resolution one would see in a TEM negative.

Thanks for the information.

JB
--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 18 18:20:41 2004

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Film with a fine grain size and lots of silver (e.g., TEM film) can resolve
the equivalent of about 4000 points per inch ("pixels" if you like). Good film
scanners can digitize film with that resolution. That means your 3.25x4 inch
film would represent 13000 x 16000 pixels or about 2 x 10^8 pixels. But it
would take twice that many bytes to hold the data because the dynamic range of
film greatly exceeds 8 bits. Film with a lot of silver in it can easily produce
12 bits (1 part in 4000) and even a bit more. A MaxD of 4.2, which is possible
with X-ray film, corresponds to about 14 bits. So you would have to store the
data as two bytes per pixel. Pay no attention to the myth that a 6 megapixel
camera delivers the performance of film - it isn't close in either dynamic
range or spatial resolution.

John Russ
======
In a message dated 10/18/04 6:21:15 PM, bozzola-at-siu.edu writes:

} Could someone provide the digital equivalency (in terms of
} resolution) of 3.25 x 4 inch TEM film.
}
} I have read that a 6 megapixel digital file has the resolution
} capability of a 35 mm grayscale negative. If this is true, then an 18
} megapixel digital file would be equivalent to a TEM grayscale
} negative in terms of resolution capability.
}
} I was thinking (based on darkroom enlargement capabilities of TEM
} films) that a 180 MP digital file would be more likely to exhibit the
} resolution one would see in a TEM negative.
}
} Thanks for the information.
}
} JB

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 18 19:17:48 2004

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John - Assuming 7um silver grains that's about right - but, of course,
it assumes that the point spread in the film is less than that and that
each electron makes a single developable grain - neither of which is likely
tom be achieved in reality.
CCD and CMOS Cameras and imaging plates have ~15um pixels with higher QE
than film. Optically coupled, as opposed to fiber optically coupled, CCDs
offer very good MTF over a wide field of view. However, FO coupled CCDs
have higher sensitivity - as low as single electrons. Imaging plates, on
the other hand, provide extremely high dynamic range - far exceeding film
or CCDs - while providing a wide field of view.

Bill Miller

At 05:26 PM 10/18/2004, John J. Bozzola wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Oct 18 19:55:33 2004

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On Oct 18, 2004, at 2:26 PM, John J. Bozzola wrote:

} Could someone provide the digital equivalency (in terms of resolution)
} of 3.25 x 4 inch TEM film.
}
} I have read that a 6 megapixel digital file has the resolution
} capability of a 35 mm grayscale negative. If this is true, then an 18
} megapixel digital file would be equivalent to a TEM grayscale negative
} in terms of resolution capability.
}
} I was thinking (based on darkroom enlargement capabilities of TEM
} films) that a 180 MP digital file would be more likely to exhibit the
} resolution one would see in a TEM negative.
}
} Thanks for the information.
}
Dear John,
Digital equivalency depends on, first, the grain size, and, second,
the scanner pixel size. For most film, the grain size is small
compared to the pixel size; however, for pixel size less than ~5 um,
grain size may be important, and, as pixel size decreases below 5 um,
grain size becomes increasingly important. A 3.25 x 4 inch film is
roughly 16,000 x 20,000 5 um x 5 um pixels for a size of ~335 Mpixel,
so, if you have a good scanner, 18 Mpixel does not contain nearly as
much info as there is on a scan of a negative, and, furthermore, the
negative itself has about 1.5 orders of magnitude more information than
is retrieved by a good scanner (and even more, if you take into account
that the ODs in the film may not be scanned quantitatively).
High-resolution film, such as 4489, has even better resolution than
these figures would indicate due to its extremely fine grain and
relatively good OD range; SO163 is pretty much in line with these
figures; LoDose X-ray film is somewhat poorer. The drawback to 4489 is
that it takes more beam to get an image, and LoDose requires much less
beam, so, since radiation damage is often limiting, it is sometimes
best to try for less information with less damage--there is no free
lunch.
The equivalence of 6 Mpixel with 35 mm film may have been derived from
assuming a certain print size and using the highest spatial frequency
seen by the human eye. In other words, comparing a print from a 6
Mpixel file with one made from film, one would see no difference.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 00:46:53 2004

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John
If my arithmetic is correct, 3.25x4" EM negative contains approximately 3
Gb equivalent of digital information: standard film has 100-200 lines/mm
resolution; technical films: 350-600 lines/mm. 600 lines/mm gives us
600*25=15000 dpi.
1 in^2=225*10^6 *3.25*4~3 Gb right? Not bad. Human eye produced 120 Mb gray
(rods only) image and resolution is about 6000 dpi.

Color 35 mm film (24x36 mm) has resolution about 150 lines/mm, so:
24x36mm=864mm^2*150^2=19440000 ~19 Mpix

When you are trying to compare "analog" and digital photography one need
to remember that we still don't have much instrumentation to handle that
giant amount of information. I am not talking about computer
recourses. See, for instance human eye may recognize only 200 shades of
gray, so we actually could not see a difference between 8 and 16-bit gray
images. Our monitors has normally 72 dpi resolution and this is what you
are analyzing on the screen. Similarly, the published images has 72 dpi as
well and barely reproduces 10-15 shades of gray... Sergey

At 02:26 PM 10/18/2004, you wrote:

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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 03:53:02 2004

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John
Your estimate of 180mpixels is close to mine.
Fine-grained b&w film can resolve ~80 lines per mm. Actually line
pairs per mm, since
a line is not a line unless seen against a background of different
intensity.
to resolve 80 lines you need 2 pixels per line: With 80 pixels per mm,
80 lines per mm
merge into solid grey, so *a minimum* 160 pixels per mm required,
assuming the
spacing and position of the lines exactly corresponds with the pitch
of the pixels.
If not, again all you see is solid grey.

for 3.25x4" film = 13208 x 16256 pixels = 214.7 mega pixels
for 35mm film = 5760x3840 = 22.1 mega pixels

Some high-performance films like Kodak Technical Pan can resolve
better than 80 line pairs per mm

Note that for TEM film in particular you may need more than 8 bits to
record the dynamic range of the film.
Which is paradoxical, because at limiting resolution, film is a binary
medium. A silver grain is there, or it isn't.

Chris

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "John J. Bozzola" {bozzola-at-siu.edu}
To: {Microscopy-at-msa.microscopy.com}
Sent: Monday, October 18, 2004 10:26 PM

The other issue to consider is the resolution of your microscope. It may
be no worth scanning a negative to see individual silver grains, if your
electron beam is printing at 100 grains wide.

Martin

At 05:58 AM 10/19/2004, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 08:18:45 2004

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Dear Colleagues...

We are planning to buy a tissue processor for electron microscopy called "Leica EM TP" with its light microscopy processing attachment. Does anybody has experience with this stuff? Do you recommend using it? As you know, these are very expensive equipment. We want to learn advantages and disadvantages of working with it. For example is it cost effective comparing with manual method?

Thanks in advance...

Dr. Necat Yžlmaz
Mersin Üniversitesi Tžp Fakültesi
Histoloji ve Embriyoloji Anabilim Dalž
0 324 3413066

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 08:19:58 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (seversong-at-dpg.army.mil) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Monday, October 18, 2004 at 17:26:52
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Email: seversong-at-dpg.army.mil
Name: Grant Severson

Organization: U.S. Army Dugway Proving Ground

Education: Graduate College

Location: Dugway, UT

Question: I was wondering if you could recommend a good course in fluorescent microscopy techniques.

Thanks,
Grant

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From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 08:47:51 2004

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Benjamin,
It looks like you had a Glut/OsO4/PO4 reaction. I would not
osmicate in phosphate, in fact switch to 0.1 M cacodylate either before
osmium or from primary fix. Also I would use(0.8% K4FeCN6) reduced (1%) osmium, you will get better myelin structure. I also advocate en-bloc
2% uranyl acetate before ethanol.
Good Luck

Michael Delannoy
Associate Director
JHSM Microscope Facility
Baltimore Md

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 11:51:12 2004

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Chris,

I think, all of these calculations come to approximately the same numbers
for the total information content of a negative, something of the order of
one to several hundred MBytes. I think, you are also right in that the
calculations yield MBit instead of MByte due to the binary nature of the
silver grains.

However, what we are talking of is the total information content of a
negative. In the overwhelming number of cases, people don't need or don't
even want this amount of information. Typical cases are Pathologists, who
want to see the information on the entire negative, but don't care so much
about the details embedded in the film at the grain level, or people who do
high-resolution TEM. They are mostly interested in the highest resolution
they can get, but not across the entire negative.

In my opinion (as a vendor of digital systems), the digital cameras have
already surpassed film in terms of usability and other parameters. The total
information content of film is higher, but to me that's like a newspaper:
Some people want to read the comics, others the stock listings, a third
person might prefer the political or foreign news. On a day to day basis,
nobody really needs all the information that is in the newspaper.

And in the rare case that someone actually does need the full information
content, you can always mosaic several TEM images into a large one.

Michael Bode

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Tuesday, October 19, 2004 02:59
To: John J. Bozzola
Cc: microscopy-at-msa.microscopy.com

John
Your estimate of 180mpixels is close to mine.
Fine-grained b&w film can resolve ~80 lines per mm. Actually line
pairs per mm, since
a line is not a line unless seen against a background of different
intensity.
to resolve 80 lines you need 2 pixels per line: With 80 pixels per mm,
80 lines per mm
merge into solid grey, so *a minimum* 160 pixels per mm required,
assuming the
spacing and position of the lines exactly corresponds with the pitch
of the pixels.
If not, again all you see is solid grey.

for 3.25x4" film = 13208 x 16256 pixels = 214.7 mega pixels
for 35mm film = 5760x3840 = 22.1 mega pixels

Some high-performance films like Kodak Technical Pan can resolve
better than 80 line pairs per mm

Note that for TEM film in particular you may need more than 8 bits to
record the dynamic range of the film.
Which is paradoxical, because at limiting resolution, film is a binary
medium. A silver grain is there, or it isn't.

Chris

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "John J. Bozzola" {bozzola-at-siu.edu}
To: {Microscopy-at-msa.microscopy.com}
Sent: Monday, October 18, 2004 10:26 PM

Mike
Yes, it is horses for courses. The astronomers up the road from here
at Edinburgh Royal Observatory routinely scan 8" x 10" negatives at 8µm
resolution, which gives huge
digital images. (No way is the scanner made by Epson). I agree we don't all
need that. But in a TEM,
silver film is still the only straightforward way to
have both widefield and high resolution, without stitching digital images
together. Because the size and
resolution of digital sensors is more limited one still has to choose
whether to put the sensor in the 35mm port for
widefield and lower resolution, or in the sheet-film position (or below) for
high resoution with tunnel vision.
Beyond that, I am not going to argue with you about the advantages of
digital cameras. They're great, convenient,
sometimes extremely sensitive, you get the image straight way, and much
more. I use them myself (though not on the EM, alas).
It is just that the performance envelope of the one does not yet coincide
with the other.

I think you slightly mis-read my point about the binary nature of the silver
image.
Like newsprint, it is composed of black bits and white bits. My point is
that as soon as
we start talking of requiring high bit-depth to contain the grey-scale data
we must be sampling
at resolution that encompasses whole populations of grains, rather than
single grains
close to the spatial resolution limit of the film.

Chris Jeffree

----- Original Message -----
} From: "Mike Bode" {mb-at-soft-imaging.com}
To: {microscopy-at-msa.microscopy.com}
Cc: "'Chris Jeffree'" {c.jeffree-at-ed.ac.uk}
Sent: Tuesday, October 19, 2004 5:56 PM

Jeff,

I think you expressed nicely what I wanted to say: "It is just that the
performance envelope of the one does not yet coincide with the other." My
point was that most people don't even need the film's high resolution AND
field of view at the same time. You can trade off what you don't need in
film for other parameters like linearity or convenience.

About the newspaper analogy: I only wanted to say that there is more
information in a newspaper than you usually need on a daily basis. Period.

Regarding the binary nature of the film grains: I agree with you. If you
only look at single grains, you talk about bits (1 or 0) of information, not
bytes. To get to bytes you have to look at several grains, as you suggested.

Looks like we're saying the same thing ;-)

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Tuesday, October 19, 2004 12:08
To: Mike Bode
Cc: microscopy-at-msa.microscopy.com

Hi, All-

A zoologist here wants to measure the depth of a couple of types of coral
calices. I told him I wasn't enthusiastic about sectioning them and
proposed breaking the coral up and looking for some fortuitous breaks for
which he could measure the depth with the light microscope (they are
appropriately sized for a stereo scope) or the SEM if he desired. But he
is now enamored of the idea of something that can give the topography
"like how they map the ocean floor". Would this be acoustic microscopy?
Some other type of microscopy? Any other ideas? I have TEMs, SEMs, light
and confocal microscopes at my disposal, but he would be happy to send it
somewhere for this analysis.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 14:43:15 2004

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Chris and all,

I want to move slightly off the subject of the digital size equivalency of
film. The point I want to make is about the number of pixels necessary to
obtain specific resolution.

The concept of resolution defined as the ability to resolve two points
(respectively two lines) is not very useful practical approach.
Two pixels per line is hardly enough to properly image the size and shape of
an object with an arbitrary shape.

Something in the range of 5 to 10 pixel per line is an adequate measure to
obtained good resolution and true shape and size of objects.

This requirement is close to a lower limit of 5 for film where the crystal
grains are randomly distributed. For a square net of digital pixel system a
value close to 10 pixel per line would be necessary for proper imaging.

With film capable of resolving about 160 lines per mm we can get about 15 to
30 lines per mm PROPERLY RESOLVED on film.

Krassimir.

---------------------------------------------------------
Krassimir N. Bozhilov, PhD
EM Scientist and Manager
Central Facility for Advanced Microscopy and Microanalysis
University of California
Riverside, CA 92521

Tel 951 827 2998
Fax 951 827 2489
--------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 15:52:39 2004

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Tina;

I have no notion what a "coral calice" may be but I do use acoustic
microscopes. There are two commercially available that I have used.
The manufacturers are Sonoscan, Inc. and Sonix. Acoustic microscopy is
somewhat different than optical or electron, etc. Depending on the
spatial resolution you require this may be a good method of imaging. It
also allows for sub-surface imaging similar to sonar in naval
applications.

Some constraints may be the mechanical compliance of the material you
are imaging. Mechanically stiffer materials image much better than say
"squishy" biological specimens that are very compliant. You probably
could get a great deal of help from the eqpt. vendors and they have some
reasonably good application notes. If I recall, there may have been
some articles in Microscopy Today on bio imaging using acoustics.

Hope this is of some help.

Regards,

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Tina Carvalho [mailto:tina-at-pbrc.hawaii.edu]
Sent: Tuesday, October 19, 2004 2:53 PM
To: Microscopy Listserver

Hi, All-

A zoologist here wants to measure the depth of a couple of types of
coral calices. I told him I wasn't enthusiastic about sectioning them
and proposed breaking the coral up and looking for some fortuitous
breaks for which he could measure the depth with the light microscope
(they are appropriately sized for a stereo scope) or the SEM if he
desired. But he is now enamored of the idea of something that can give
the topography "like how they map the ocean floor". Would this be
acoustic microscopy? Some other type of microscopy? Any other ideas? I
have TEMs, SEMs, light and confocal microscopes at my disposal, but he
would be happy to send it somewhere for this analysis.

Aloha,
Tina

************************************************************************
****
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu
*
* Biological Electron Microscope Facility * (808) 956-6251
*
* University of Hawaii at Manoa *
http://www.pbrc.hawaii.edu/bemf*
************************************************************************
****

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 16:18:50 2004

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Dear Sir or Madam,

I am an undergraduate student of Materials Science at Oxford University. In a Team Design Project which is part of our course, my team has the task to design a cyclic loading stage for use in a SEM (in situ) to enable observation of samples under load and the dynamic evolution of damage during cycling.
The project does not only include the actual design but also a market evaluation. In order to get a feeling for the demand of such a stage I would like to ask for your expert advice on a few issues.
I have designed a little questionnaire which should take less than five minutes to fill out. This would greatly benefit our Design Project. Needless to say we would be very grateful for your feedback.

On behalf of my team I would like to thank you very much in advance for helping us in estimating the demand for such a cyclic loading stage.

Best regards,
Markus Mittermaier

Questionnaire: A Cyclic Loading Stage For Use in a Scanning Electron Microscope

1)
What is your primary research area:

2)
Have you ever heard of cyclic loading stages being used in SEM?
If yes, please specify:

3)
Do you encounter situations where a cyclic loading stage for a SEM would benefit your research?
If yes, please specify:

4)
Can you imagine using a cyclic loading stage of small dimensions for applications other than in a SEM?
If yes, how?

5)
What market price do you expect for such a cyclic loading stage which would have to be tailor-made (to a certain extent) or include an adapter to fit inside your microscope. Please comment on your expectation about the price (regardless of whether you would be willing to pay that amount).

A: 15000-20000 US Dollars
B: 20000-25000 US Dollars
C: 30000-35000 US Dollars
D: more than 35000 US Dollars
E: other:

6)
Which actuation mechanism to supply the load to the sample in the SEM would you prefer.
a) Hydraulic actuation
b) Piezoelectric actuation
c) Other:

7)
What is your estimate about the demand for small scale cyclic loading stages in academia and industry worldwide?

A: {10 p.a.
B: 10-20 p.a.
C: 20-30 p.a.
D: 30-50 p.a.
E: } 50 p.a.
F: } 100 p.a.
Other: ______

8)
What is your own willingness to pay for such a device?

Thank you very much.

Markus Mittermaier
University of Oxford
Mansfield College
OX1 3TF
Oxford, UK
markus.mittermaier-at-mansfield.oxford.ac.uk

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 16:47:33 2004

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Dear Tina,

Depending on the dimensions involved and the shape, you might want to try a light
section microscope and do it non-destructively. These are used in industry to
measure small height differences. The method is also contact-less, since it
involves measuring the parallax offset of a tightly collimated line of light
projected obliquely onto the surface. It can be used on wet paint or ink, for
example. In principle, it could even be used on the soft tissue of live coral.

By using a step-repeat-step-repeat process one could also record a series of
contour lines across the sample.

John Twilley

Tina Carvalho wrote:

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}
} Hi, All-
}
} A zoologist here wants to measure the depth of a couple of types of coral
} calices. I told him I wasn't enthusiastic about sectioning them and
} proposed breaking the coral up and looking for some fortuitous breaks for
} which he could measure the depth with the light microscope (they are
} appropriately sized for a stereo scope) or the SEM if he desired. But he
} is now enamored of the idea of something that can give the topography
} "like how they map the ocean floor". Would this be acoustic microscopy?
} Some other type of microscopy? Any other ideas? I have TEMs, SEMs, light
} and confocal microscopes at my disposal, but he would be happy to send it
} somewhere for this analysis.
}
} Aloha,
} Tina
}
} ****************************************************************************
} * Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
} * Biological Electron Microscope Facility * (808) 956-6251 *
} * University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
} ****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 17:54:31 2004

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When comparing resolution of film with the resolution of a digital
camera, you need to realize two things: 1) That film is not digital. It
is analog, and its frequency response is described by a modulation
transfer function. Here, for example, is the URL for the curve for Kodak
T-Max black and white film:
http://www.kodak.com/global/en/professional/support/techPubs/f4016/f002_
0542ac.gif 2) 2) Pixel counts are not resolution. Resolution is the
ability to resolve two features represented by intensity peaks.
Generally, one pixel for bright and one pixel for dark (the Nyquist
criterion-you all know that). Comparing digital to analog requires
choosing the threshold for the analog resolution, and I am not sure what
the critical criteria are for making that choice. For example, is T-max
resolution 160 line pairs per millimeter (35% Response) or is it 60 line
pairs per millimeter (90% response), or is it something in between?

John Mardinly
Intel

-----Original Message-----
} From: John J. Bozzola [mailto:bozzola-at-siu.edu]
Sent: Monday, October 18, 2004 2:26 PM
To: Microscopy-at-msa.microscopy.com

Could someone provide the digital equivalency (in terms of
resolution) of 3.25 x 4 inch TEM film.

I have read that a 6 megapixel digital file has the resolution
capability of a 35 mm grayscale negative. If this is true, then an 18
megapixel digital file would be equivalent to a TEM grayscale
negative in terms of resolution capability.

I was thinking (based on darkroom enlargement capabilities of TEM
films) that a 180 MP digital file would be more likely to exhibit the
resolution one would see in a TEM negative.

Thanks for the information.

JB
--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 18:11:14 2004

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Krassimir,

You are correct in that a certain oversampling is necessary to be able to
fully reconstruct a given signal. This was explored in detail by Shannon and
Nyquist (I can't give references here, but a web search of Nyquist will
result in many hits). In essence the result is that a given signal must be
oversampled by a factor of 2 to allow a perfect reconstruction of the
original signal. In other words: If your phosphor resolution is 5 microns (5
micron grains), you need to sample it with a pixel size of 2.5 microns. An
oversampling of less than that might lead to aliasing (convolution of
signals that cannot be corrected for), oversampling of much more than a
factor of 2 will not increase the quality significantly.

However, the final result is also influenced by the Modulation Transfer
Function of any lens or other optical element you might have between the
phosphor and the CCD. So, the number of pixels is an important number, but
if you couple a high-quality CCD with a mediocre lens, the result will be
mediocre at best.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: K.N. Bozhilov [mailto:bozhilov-at-ucr.edu]
Sent: Tuesday, October 19, 2004 13:50
To: microscopy-at-msa.microscopy.com

Chris and all,

I want to move slightly off the subject of the digital size equivalency of
film. The point I want to make is about the number of pixels necessary to
obtain specific resolution.

The concept of resolution defined as the ability to resolve two points
(respectively two lines) is not very useful practical approach.
Two pixels per line is hardly enough to properly image the size and shape of
an object with an arbitrary shape.

Something in the range of 5 to 10 pixel per line is an adequate measure to
obtained good resolution and true shape and size of objects.

This requirement is close to a lower limit of 5 for film where the crystal
grains are randomly distributed. For a square net of digital pixel system a
value close to 10 pixel per line would be necessary for proper imaging.

With film capable of resolving about 160 lines per mm we can get about 15 to
30 lines per mm PROPERLY RESOLVED on film.

Krassimir.

---------------------------------------------------------
Krassimir N. Bozhilov, PhD
EM Scientist and Manager
Central Facility for Advanced Microscopy and Microanalysis
University of California
Riverside, CA 92521

Tel 951 827 2998
Fax 951 827 2489
--------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 18:25:30 2004

Contents Retrieved from Microscopy Listserver Archives
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On Oct 19, 2004, at 12:50 PM, K.N. Bozhilov wrote:

} I want to move slightly off the subject of the digital size
} equivalency of
} film. The point I want to make is about the number of pixels necessary
} to
} obtain specific resolution.
}
} The concept of resolution defined as the ability to resolve two points
} (respectively two lines) is not very useful practical approach.
} Two pixels per line is hardly enough to properly image the size and
} shape of
} an object with an arbitrary shape.
}
} Something in the range of 5 to 10 pixel per line is an adequate
} measure to
} obtained good resolution and true shape and size of objects.
}
} This requirement is close to a lower limit of 5 for film where the
} crystal
} grains are randomly distributed. For a square net of digital pixel
} system a
} value close to 10 pixel per line would be necessary for proper imaging.
}
} With film capable of resolving about 160 lines per mm we can get about
} 15 to
} 30 lines per mm PROPERLY RESOLVED on film.
}
Dear Krassimir,
If one considers the situation in reciprocal space, one has all the
information out to a limiting spatial frequency, which is determined by
the sampling; i.e., the pixel size. It is true that the Fourier
transform of an image with continuous sampling--equivalent to unlimited
spatial frequency--which is cut off at a particular resolution, is not
exactly the same as the FFT of a pixelated image with a pixel size
corresponding to the same resolution (twice the pixel size, as
previously stated), but as one looks at features at a somewhat larger
resolution, say 2/3 of the Nyquist frequency (or three pixels), the
magnitudes and phases of the FFT are pretty close to those in the
continuous-sampling case. 5 to 10 pixels per line is OK when you are
trying to define the line, but higher-frequency information is
available from fewer pixels, and, in particular, objects smaller than 5
pixels can be determined to be individual objects. I am confident that
I can determine the structures present in a micrograph to a resolution
of 2/3 Nyquist in the case that the micrograph has sufficient contrast
and S/N ratio, both of which play a big role in the resolution one can
obtain. If, for example, one has a pattern of infinitely dark lines
separated by regions of 100% transmission, one can describe them with
sub-pixel accuracy, since a pixel at 0.3 OD (=50% transmission) is half
black, so the edge of the line must bisect the pixel. (Of course, the
line must have finite thickness to be seen at all, and I am assuming
that it is thicker than one pixel.) On the other hand, an image where
the lines are at 1 OD and the spaces are at 0.95 OD, and where there is
noise--a typical condition for frozen-hydrated biological specimens--I
would expect it to be difficult to define lines with 5 to 10 pixels.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 18:59:41 2004

Contents Retrieved from Microscopy Listserver Archives
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Thanks to everyone who sent responses to my question regarding the
comparative resolution of TEM film versus digital imaging. Since I
was giving a lecture on electron micrography and darkroom methods in
TEM, I thought it would be informative for students to understand the
advantages and disadvantages of film versus digital imaging.
Resolution is always a concern, so it is informative to be able to
compare the two technologies with data. We use both methods of
imaging in our TEMs, depending on the needs of the research project.

--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
Web: http://www.siu.edu/~image/
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 22:09:21 2004

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Hi, All-

Wow! Lots of interesting replies to my query on measuring the depth of
coral calices. Most of them asking what a coral calyx is and about how big
it would be! For the non-invertebrate-zoology types on the List, the
soft-bodied coral polyp (kind of upside-down jellyfish-like) secretes and
lives in a calcium carbonate "skeleton" (lots of which make up the world's
coral reefs). He only wants to measure the depth of some of the cups that
the polyps live in; nothing about the tissue itself. Each cup (calyx) is
probably about 0.5 - 1.5 mm deep, and about 2 mm across. I don't have an
image handy, but I found one on the Web at
http://www.uga.edu/caur/coral.jpg - it's a picture of a coral with a bunch
of calices. Try to topomap that!

Those of you who attend Microscopy & Microanalysis 2005 here next year can
put on a mask and snorkel and see for yourselves...

I have another project coming up where someone wants me to section
deep-sea soft corals and see if there are bacteria inside. I already have
found out they are not soft at all, but are armored to the max, inside and
out! But that I can deal with. I hope.

Aloha,
Tina

****************************************************************************
* Tina (Weatherby) Carvalho * tina-at-pbrc.hawaii.edu *
* Biological Electron Microscope Facility * (808) 956-6251 *
* University of Hawaii at Manoa * http://www.pbrc.hawaii.edu/bemf*
****************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 19 22:17:51 2004

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I have been following this discussion with great interest. The cryo-TEM
community has been interested in these questions for some time. The most
recent comparison of which I am aware was published by Zhang et al.,
"Automated image acquisition and processing using a new generation of 4K x
4K CCD cameras for cryo-electron microscopic studies of macromolecular
assemblies," Journal of Structural Biology, 143, 135-144 (2003). From the
abstract: "We demonstrate that at 120 kV, and at a nominal magnification of
67,000X, power spectra and signal-to-noise ratios for the new 4K CCD camera
are comparable to values obtained for film images scanned using a Zeiss
scanner to resolutions as high as ~ 1/6.5 A." In the article, the authors
noted that this camera still only had approximately one third of the area of
the TEM negative. A close examination of Figure 4 in the article showed that
the signal to noise ratio of film was noticeably better than the CCD at
higher spatial frequencies.

As one who has used both film and 1K x 1K CCD cameras for TEM imaging for
several years, I really appreciate the "instant gratification" that
accompanies the CCD camera (especially for quantitative image analysis). I
also appreciate the high resolution, large field of view available in a
3.25" x 4" TEM negative. Happily, I can choose whichever sensor (or both)
that I need to solve a particular problem.

Standard disclaimer: my employer manufactures film, solid state image
sensors, and scanners.

John Minter
jrminter-at-rochester.rr.com

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 06:20:38 2004

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take a look at the micro X-ray tomography instrument from Skyscan -
http://www.skyscan.be/next/home.htm

At 08:32 PM 10/19/2004, Tina Carvalho wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 07:12:01 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bwareham-at-utah.gov) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, October 18, 2004 at 17:01:52
---------------------------------------------------------------------------

Email: bwareham-at-utah.gov
Name: Beverly Wareham

Organization: Utah Veterinary Diagnostic Laboratory

Title-Subject: [Microscopy] [Filtered] Live cell stain

Question: Hi all,
An associate of mine is looking for a live cell stain for cell culture. If anyone has any ideas, we would appreciate hearing them.
Thank you,
Beverly Wareham

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 07:12:50 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (lynda-at-biotech.ufl.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 19, 2004 at 07:56:09
---------------------------------------------------------------------------

Email: lynda-at-biotech.ufl.edu
Name: Lynda Schneider

Organization: University of Florida

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello all,

I am in need of learning if there is a way of lifting a paraffin stained section from a glass slide for EM. I have a PI that has a case he would like to have worked up by EM but the best material he has is an H&E stained
section on a slide. Any ideas?

Thanks in advance.

Lynda Schneider

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 07:53:20 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Mike,
As a non-expert, doesn't Nyquist say the over-sampling must be greater than
2? I believe 2 can give considerable aliasing but the problem can be
overcome at 2.1. Is this correct or did I miss something?

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

-----Original Message-----
} From: Mike Bode [mailto:mb-at-soft-imaging.com]
Sent: Tuesday, October 19, 2004 7:17 PM
To: 'K.N. Bozhilov'
Cc: microscopy-at-msa.microscopy.com

Krassimir,

You are correct in that a certain oversampling is necessary to be able to
fully reconstruct a given signal. This was explored in detail by Shannon and
Nyquist (I can't give references here, but a web search of Nyquist will
result in many hits). In essence the result is that a given signal must be
oversampled by a factor of 2 to allow a perfect reconstruction of the
original signal. In other words: If your phosphor resolution is 5 microns (5
micron grains), you need to sample it with a pixel size of 2.5 microns. An
oversampling of less than that might lead to aliasing (convolution of
signals that cannot be corrected for), oversampling of much more than a
factor of 2 will not increase the quality significantly.

However, the final result is also influenced by the Modulation Transfer
Function of any lens or other optical element you might have between the
phosphor and the CCD. So, the number of pixels is an important number, but
if you couple a high-quality CCD with a mediocre lens, the result will be
mediocre at best.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: K.N. Bozhilov [mailto:bozhilov-at-ucr.edu]
Sent: Tuesday, October 19, 2004 13:50
To: microscopy-at-msa.microscopy.com

Chris and all,

I want to move slightly off the subject of the digital size equivalency of
film. The point I want to make is about the number of pixels necessary to
obtain specific resolution.

The concept of resolution defined as the ability to resolve two points
(respectively two lines) is not very useful practical approach.
Two pixels per line is hardly enough to properly image the size and shape of
an object with an arbitrary shape.

Something in the range of 5 to 10 pixel per line is an adequate measure to
obtained good resolution and true shape and size of objects.

This requirement is close to a lower limit of 5 for film where the crystal
grains are randomly distributed. For a square net of digital pixel system a
value close to 10 pixel per line would be necessary for proper imaging.

With film capable of resolving about 160 lines per mm we can get about 15 to
30 lines per mm PROPERLY RESOLVED on film.

Krassimir.

---------------------------------------------------------
Krassimir N. Bozhilov, PhD
EM Scientist and Manager
Central Facility for Advanced Microscopy and Microanalysis
University of California
Riverside, CA 92521

Tel 951 827 2998
Fax 951 827 2489
--------------------------------------------------------

___________________________________________________________
$0 Web Hosting with up to 120MB web space, 1000 MB Transfer
10 Personalized POP and Web E-mail Accounts, and much more.
Signup at www.doteasy.com

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 08:40:01 2004

Contents Retrieved from Microscopy Listserver Archives
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What you need to do is invert a beem capsule with epon on top of the section,
polymerize, and then dip in liquid nitrogen - the block will pop off with
section embedded. (Of course, remove the coverslip first!)

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: lynda-at-biotech.ufl.edu [mailto:lynda-at-biotech.ufl.edu]
Sent: Wednesday, October 20, 2004 8:20 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by
(lynda-at-biotech.ufl.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
October 19, 2004 at 07:56:09
---------------------------------------------------------------------------

Email: lynda-at-biotech.ufl.edu
Name: Lynda Schneider

Organization: University of Florida

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello all,

I am in need of learning if there is a way of lifting a paraffin stained section
from a glass slide for EM. I have a PI that has a case he would like to have
worked up by EM but the best material he has is an H&E stained
section on a slide. Any ideas?

Thanks in advance.

Lynda Schneider

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 08:54:02 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Benjamin:

I agree with Michael that the phosphate buffer is the factor contributing to
the contamination you have observed. Next time use cacodylate buffer.
Maunsbach and Afzelius book: "Biomedical Electron Microscopy, Illustrated
methods and interpretations" comments on pages 76 & 77 on phosphate buffer
precipitate which is not generally well understood. They later comment on
the vulnerablity of lipid rich tissue (yours had myelin) to this artifact
and how this only occurs with phosphate buffers. They reference an article
from Stain Technology, 1979 by Ellis, E.A. & Anthony, D.W. vol. 54:282-285
which discusses how to remove this precipitate.

Hope this helps!

Karen Bentley

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

-----Original Message-----
} From: BENJAMIN K AUGUST [mailto:bkaugust-at-facstaff.wisc.edu]
Sent: Monday, October 18, 2004 5:24 PM
To: microscopy-at-msa.microscopy.com; microscopy-at-msa.microscopy.com

Our lab has routinely processed samples according to the methods
posted at http://www.micro.wisc.edu/smith in the past without
artifacts, but recently we have encountered an unknown contaminant
seen as an electron dense (opaque) amorphic precipitate. Please visit
the web-site listed above for examples of the artifact and detailed
processing methods. We would like your opinions as to the source of
this contamination so we might avoid it in future experiments. Your
comments are much appreciated.

Ben August
U.W. Electron Microscopy Facility
Medical School
University of Wisconsin - Madison
bkaugust-at-facstaff.wisc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 09:06:21 2004

Contents Retrieved from Microscopy Listserver Archives
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Ken,

It's been a while since I dove into the details of the Nyquist theorem. The
theorem is usually stated like this:

Nyquist's theorem: A theorem, developed by H. Nyquist, which states that an
analog signal waveform may be uniquely reconstructed, without error, from
samples taken at equal time intervals. The sampling rate must be equal to,
or greater than, twice the highest frequency component in the analog signal.

The "equal to" would imply that a factor of 2 is sufficient.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Ken Converse [mailto:kenconverse-at-qualityimages.biz]
Sent: Wednesday, October 20, 2004 07:00
To: 'Mike Bode'
Cc: MSA Listserver

Krassimir,

You are correct in that a certain oversampling is necessary to be able to
fully reconstruct a given signal. This was explored in detail by Shannon and
Nyquist (I can't give references here, but a web search of Nyquist will
result in many hits). In essence the result is that a given signal must be
oversampled by a factor of 2 to allow a perfect reconstruction of the
original signal. In other words: If your phosphor resolution is 5 microns (5
micron grains), you need to sample it with a pixel size of 2.5 microns. An
oversampling of less than that might lead to aliasing (convolution of
signals that cannot be corrected for), oversampling of much more than a
factor of 2 will not increase the quality significantly.

However, the final result is also influenced by the Modulation Transfer
Function of any lens or other optical element you might have between the
phosphor and the CCD. So, the number of pixels is an important number, but
if you couple a high-quality CCD with a mediocre lens, the result will be
mediocre at best.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: K.N. Bozhilov [mailto:bozhilov-at-ucr.edu]
Sent: Tuesday, October 19, 2004 13:50
To: microscopy-at-msa.microscopy.com

Chris and all,

I want to move slightly off the subject of the digital size equivalency of
film. The point I want to make is about the number of pixels necessary to
obtain specific resolution.

The concept of resolution defined as the ability to resolve two points
(respectively two lines) is not very useful practical approach.
Two pixels per line is hardly enough to properly image the size and shape of
an object with an arbitrary shape.

Something in the range of 5 to 10 pixel per line is an adequate measure to
obtained good resolution and true shape and size of objects.

This requirement is close to a lower limit of 5 for film where the crystal
grains are randomly distributed. For a square net of digital pixel system a
value close to 10 pixel per line would be necessary for proper imaging.

With film capable of resolving about 160 lines per mm we can get about 15 to
30 lines per mm PROPERLY RESOLVED on film.

Krassimir.

---------------------------------------------------------
Krassimir N. Bozhilov, PhD
EM Scientist and Manager
Central Facility for Advanced Microscopy and Microanalysis
University of California
Riverside, CA 92521

Tel 951 827 2998
Fax 951 827 2489
--------------------------------------------------------

___________________________________________________________
$0 Web Hosting with up to 120MB web space, 1000 MB Transfer
10 Personalized POP and Web E-mail Accounts, and much more.
Signup at www.doteasy.com

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 09:38:45 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi,

I am trying to find information on physical cell sizes, such as diameter
(volume) of the nucleus, etc., for various human cell types (cell lines)
? Are there on-line resources where this kind of general information is
available ? I did not find this information on the ATCC website.

Regards,

Peter Van Osta

----------------------------------------------
Peter Van Osta, MD

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 09:49:21 2004

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} As a non-expert, doesn't Nyquist say the over-sampling must be
} greater than 2?
} I believe 2 can give considerable aliasing but the problem can be
} overcome at 2.1.

2 is the Nyquist *limit*. Anything less than that and you are guaranteed to
alias. At exactly 2 samples per cycle, you might get lucky or not get lucky.
Consider sampling a sine wave at two samples per cycle. If you are lucky,
you will pick the peaks of the sine wave and you will be able to reconstruct
the wave perfectly (along with the a priori knowledge that it is a sine).
But if you are unlucky, you will pick the zero crossings and you will
reconstruct a zero frequency, zero amplitude wave.

If you sample at a higher frequency, then you can reconstruct the proper
wave but, again, you must also add the a priori knowledge that it is a
sine/cosine wave. The implication of the a priori knowledge is that if you
have a wave that is more complex than a sine or cosine, you would need to do
a Fourier decomposition of the wave to determine the highest non-negligible
frequency component. Let's call that frequency F. You would then have to
sample the wave at a frequency of at least 2F, preferably a little higher,
to reconstruct the original wave properly.

Bruce Girrell

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 09:47:13 2004

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Hi,

One reason for (slight) oversampling is that if you sample at exactly 2x
the maximum spatial frequency, you might by accident sample at the
moment where the signal goes through all zero's.

http://members.aol.com/ajaynejr/nyquist.htm
http://ourworld.compuserve.com/homepages/pvosta/pcrnyq.htm

Regards,

Peter Van Osta

----------------------------------------------
Peter Van Osta, MD

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------
========================================================
Ken Converse wrote:
}
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} Mike,
} As a non-expert, doesn't Nyquist say the over-sampling must be greater than
} 2? I believe 2 can give considerable aliasing but the problem can be
} overcome at 2.1. Is this correct or did I miss something?
}
} Ken Converse
}
} owner
} QUALITY IMAGES
} Servicing Scanning Electron Microscopes
} Since 1981
} 16 Creek Rd.
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} 717-456-5491
} Fax 717-456-7996
} kenconverse-at-qualityimages.biz
} qualityimages.biz
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 10:07:37 2004

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} Email: lynda-at-biotech.ufl.edu
} Name: Lynda Schneider}
} Organization: University of Florida
} Question:
} I am in need of learning if there is a way of lifting a paraffin stained
} section from a glass slide for EM. I have a PI that has a case he would like
} to have worked up by EM but the best material he has is an H&E stained
} section on a slide. Any ideas?
}
} Thanks in advance.
} Lynda Schneider
---------------------------------------------------------------
Lynda,
I have a protocol from the late 60's but never needed to try it.
I do not know if it was published but the info. I have is as follows:
Harvey Blank, MD and Carol Collins
Dept. of Dermatology, Univ. of Miami

1. Clean slide and remove all stickers etc.
2. Slide into xylol several days to remove coverslip.
3. Slide coverslip without force off the slide.
4. Slide in fresh xylol to assure removal of all mounting medium.
5. Dip slide into 50% xylol + 50% propylene oxide (no time given)
6. Dip slide into 100% prophylene oxide
7. Dip slide into 50% prophylene oxide + 50% embedding medium (Epon type)
8. Invert slide, sections down, over a small dish filled with embedding medium
(I would suggest using a mold or polypropylene plastic instead of glass and

make a few blank Beem Capsules to be used in step 13.)
9. Put into 60 degree C. oven over night to cure.
10.Remove slide from cured plastic while still warm.
(They slide a fresh razor blade between the slide and the plastic. Some use
liquid nitrogen to pop it off. Other comments welcome!)
11.Determine area of interest (LM) and scribe a box around it.
12.Cut out the area of interest. (Jeweler's saw works well or new razor blade)
13.Mount tissue side UP on a blank (with some reserved epoxy and put back into
the oven 'til the next morning.)

I have found that if I put black Sharpie marker ink on the top
of the blank and let it dry a bit before mounting the embedded tissue,
it makes it much easier to align the block for sectioning.

I have heard that the result should be better than LM but not near
as good as if the specimen was originally run up for TEM.

Lots of Luck,
Pat Connelly
Univ. of Pennsyvania
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 10:17:58 2004

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Lynda:

Well I have published several "pop-off" technique papers and will give you
the references:

de Mesy Jensen, K.L.: "Pop-off" technique for FNA smears for diagnostic
electron microscopy. Tech. Sample CY-1, American Society of Clinical
Pathologists, 1987

de Mesy Jensen, K.L.: "Pop-off" technique for FNA smears for diagnostic
electron microscopy. Tech. Sample CY-1, American Society of Clinical
Pathologists, 1987

de Mesy Jensen, K.L., di Sant'Agnese, P.A.: Large block embedding and
"pop-off" technique for immunoelectron microscopy with applications to
prostatic endocrine-paracrine cells. Ultrastructural Pathology 16:51, 1992.

Here's the summary of what you should do:

You can look at an H & E section by "popping off" the section. All
you have to do is remove the coverslip, rehydrate the slide from xylene to
H2O and post fix in 1% OsO4 for 20 min., then dehydrate the slide (I use a
plastic (5) slide mailer for processing) to 100% x 3 and infiltrate with
epoxy resin. I always use Spurr resin for "popping off" a section. After
the infiltration steps (usually 4 hrs. or overnight) you take a BEEM capsule
with the cap removed, fill with liquid resin (up to top of capsule and
slightly concave), quickly invert and place over the area you want to
"pop-off" on the slide. Place the slide in the oven and polymerize
overnight. The next day you can break the surface tension between the
polymerized capsule and the glass by dipping the slide in liquid nitrogen
(dip several times without submersing the capsule, just the base of the
capsule attached to the slide) Wiggle the capsule and it should "pop-off",
if it won't, then dip for several seconds more and try again.

Keep in mind the appearance of the "popped off" tissue will not look to
good, since it was processed and stained onto a slide. Sometimes, it is
better to take the paraffin block and core out the area of interest matched
with the area of interest on the slide. Then I deparaffinize the tissue and
post-fix in glut, OsO4 and process as if it were a normal EM specimen.
Usually the tissue looks better than what you see on EM from a "popped off"
tissue section.

Karen L. de Mesy Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

-----Original Message-----
} From: lynda-at-biotech.ufl.edu [mailto:lynda-at-biotech.ufl.edu]
Sent: Wednesday, October 20, 2004 8:20 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (lynda-at-biotech.ufl.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, October 19, 2004 at 07:56:09
---------------------------------------------------------------------------

Email: lynda-at-biotech.ufl.edu
Name: Lynda Schneider

Organization: University of Florida

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello all,

I am in need of learning if there is a way of lifting a paraffin stained
section from a glass slide for EM. I have a PI that has a case he would like
to have worked up by EM but the best material he has is an H&E stained
section on a slide. Any ideas?

Thanks in advance.

Lynda Schneider

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 11:17:45 2004

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Molecular Probes

http://www.probes.com/

sell several live fluorescent stains. I have used some of them on various
cell types in culture, and they worked very well.

Lesley Weston.

on 20/10/2004 5:19 AM, by way of MicroscopyListserver at bwareham-at-utah.gov
wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
----------------------------------------------------------------------------
--} -
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted
} by (bwareham-at-utah.gov) from
} http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday,
} October 18, 2004 at 17:01:52
} ---------------------------------------------------------------------------
}
} Email: bwareham-at-utah.gov
} Name: Beverly Wareham
}
} Organization: Utah Veterinary Diagnostic Laboratory
}
} Title-Subject: [Microscopy] [Filtered] Live cell stain
}
} Question: Hi all,
} An associate of mine is looking for a live cell stain for cell culture. If
} anyone has any ideas, we would appreciate hearing them.
} Thank you,
} Beverly Wareham
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 11:03:45 2004

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Be careful of any data you find. Cell of a given type vary in diameter, and
thickness, depending on how they're prepared. Cultured cells spread out
very thinly and so will be wider in diameter, and thinner, then, for
example, cells collected in preservative, which will "round up" and be
smaller in diameter. How much smaller depends on the type and concentration
of preservative, and what happens to the cells next (e.g., applied to a
slide [clear or dirty makes a difference]) and fixed, or applied to a slide
and allowed to air-dry. Such details should be specified in conjunction
with any cell size measurements.

For example, there is a 6-fold difference in area between mesothelial cells
collected in 50% ethanol that are applied to a slide and wet-fixed, and
fresh mesothelial cells that are applied to a slide and air-dried.

Gary Gill

-----Original Message-----
} From: Peter Van Osta [mailto:pvosta-at-maia-scientific.com]
Sent: Wednesday, October 20, 2004 9:46 AM
To: MSA

Ken you are right, 2 is not enough - think about two pixels the same
intensity next to each other and you'll see immediately that you can not
distinguish a single two pixel by one pixel object from two adjacent
single pixel objects. I believe that the number is something like 2.3 over
sampling.

Bill

At 09:00 AM 10/20/2004, Ken Converse wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 12:46:27 2004

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Greetings,
A lower cost alternative to the designer probes if a simple viability
test is needed is to use fluorescien diacetate and propidium iodide
(available from Sigma). Live cells = green because an enzyme in the
cell cleaves the membrane permeable fluorescien diacetate and dead cells
exhibit red nuclei (after plasma membrane is compromised). See:

Jones and Senft. (1985). "An Improved Method to Determine Cell Viability
by Simultaneous Staining with Fluorescien Diacetate-Propidium Iodide."
J. Histochem. Cytochem. 33, 1, 77-79.

Regards,
Karl

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 13:10:11 2004

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I have following question:

I have a glass-ceramic material, where glass and crystallites have the
same composition. I want to perform the EBSD on crystallites of this
material. I can not coat the material because I have to do diffraction.
I used SE mode with 0.3 torr water pressure but the image quality is not
good enough for 5 micron size crystallites which have the same
composition as the glass and which are sticking out only few nanometer
out of the glass surface (50-60 nm, i can make it 100-200 nm but etching
but still having difficulty in finding out crystallites). I used the gas
detector with 1 torr pressure (i can't go below that) and image quality
improved but the diffraction pattern quality degraded to a level that I
can not map it properly. Is there a simple way to do EBSD of these
materials?

Sincerely
Pradyumna
Lehigh University

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 13:59:11 2004

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Karen,

We follow a similar procedure for lifting a paraffin section( unstained
would produce better results). However,the procedure we use for
processing tissue out of paraffin and sections does not reguire
hydrating down to
OsO4. We make up a 2%Osmium/xylene and start the processing at that
point.
It actually is shorter than starting with wet tissue,since the next step
is
into propelyne oxide,then resin mixtures.

Reference :

Kai Chien,R.L.Van de Velde and R.C. Heusser
A One-Step Method for Re-embedding Paraffin Embedded Specimens for
Electron Microscopy.
EMSA 1982 pp356-357

Connie Gillies

-----Original Message-----
} From: Bentley, Karen [mailto:Karen_Jensen-at-URMC.Rochester.edu]
Sent: Wednesday, October 20, 2004 11:26 AM
To: 'microscopy-at-msa.microscopy.com'

Lynda:

Well I have published several "pop-off" technique papers and will give
you
the references:

de Mesy Jensen, K.L.: "Pop-off" technique for FNA smears for diagnostic
electron microscopy. Tech. Sample CY-1, American Society of Clinical
Pathologists, 1987

de Mesy Jensen, K.L.: "Pop-off" technique for FNA smears for diagnostic
electron microscopy. Tech. Sample CY-1, American Society of Clinical
Pathologists, 1987

de Mesy Jensen, K.L., di Sant'Agnese, P.A.: Large block embedding and
"pop-off" technique for immunoelectron microscopy with applications to
prostatic endocrine-paracrine cells. Ultrastructural Pathology 16:51,
1992.

Here's the summary of what you should do:

You can look at an H & E section by "popping off" the section.
All
you have to do is remove the coverslip, rehydrate the slide from xylene
to
H2O and post fix in 1% OsO4 for 20 min., then dehydrate the slide (I use
a
plastic (5) slide mailer for processing) to 100% x 3 and infiltrate with
epoxy resin. I always use Spurr resin for "popping off" a section.
After
the infiltration steps (usually 4 hrs. or overnight) you take a BEEM
capsule
with the cap removed, fill with liquid resin (up to top of capsule and
slightly concave), quickly invert and place over the area you want to
"pop-off" on the slide. Place the slide in the oven and polymerize
overnight. The next day you can break the surface tension between the
polymerized capsule and the glass by dipping the slide in liquid
nitrogen
(dip several times without submersing the capsule, just the base of the
capsule attached to the slide) Wiggle the capsule and it should
"pop-off",
if it won't, then dip for several seconds more and try again.

Keep in mind the appearance of the "popped off" tissue will not look to
good, since it was processed and stained onto a slide. Sometimes, it is
better to take the paraffin block and core out the area of interest
matched
with the area of interest on the slide. Then I deparaffinize the tissue
and
post-fix in glut, OsO4 and process as if it were a normal EM specimen.
Usually the tissue looks better than what you see on EM from a "popped
off"
tissue section.

Karen L. de Mesy Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

-----Original Message-----
} From: lynda-at-biotech.ufl.edu [mailto:lynda-at-biotech.ufl.edu]
Sent: Wednesday, October 20, 2004 8:20 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (lynda-at-biotech.ufl.edu) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, October 19, 2004 at 07:56:09
------------------------------------------------------------------------
---

Email: lynda-at-biotech.ufl.edu
Name: Lynda Schneider

Organization: University of Florida

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Hello all,

I am in need of learning if there is a way of lifting a paraffin stained
section from a glass slide for EM. I have a PI that has a case he would
like
to have worked up by EM but the best material he has is an H&E stained
section on a slide. Any ideas?

Thanks in advance.

Lynda Schneider

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 20 14:23:42 2004

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An Anthropology student came into our EM facility with a sample I don't
know how to handle. She wants to study the rate and extent of
bacterial penetration into buried animal bones. She has a few previous
papers showing methods for doing this, but the pictures are poor and
methods are not always complete. Some people mention SEM, but don't
show pictures. More often they seem to be using light microscopy of
sections (30 microns) of resin embedded material.

We could do SEM but it isn't clear that this is the best approach, nor
do we know which prep method to use if it is. Some groups critical
point dry and use an SE detector. Others embed and use a backscatter
detector. For LM we don't have any microtomes that will cut 30 micron
sections and the histology group in another department has only cut
decalcified material. The geology department has a diamond saw, but I
don't know if this can be used on embedded material or whether we would
get too much distortion if we try to cut or polish unembedded material.

Before we waste a lot of time trying all these options out, do any of
you have experience with this type of work? Would she need to
decalcify the bone? Should it be embedded? Would it be better to
grind the surface and do SEM or cut sections and do light microscopy?

Thanks in advance for any suggestions you can offer.

Marie

Dr. Marie E. Cantino
Director, Electron Microscopy Laboratory
Associate Professor of Physiology and Neurobiology
University of Connecticut Unit 3242
Storrs, CT 06269-3242
Phone: 860-486-3588
Fax: 860-486-6369

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 07:20:48 2004

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Hi,

I am looking for some information on the interaction of some popular
cell culture compounds on image formation in digital (brightfield)
microscopy.

Is there any information available on optical density (O.D.)
spectroscopical analysis and turbity of Fetal Bovine Serum (FBS) and
Fetal Calf serum (FCS) ? FCS causes a cell culture medium to become red
and only partially transluscent instead of clear.

Phenol red (phenolsulfonphthalein, pH range 6.8 - 8.4) is a popular
reagent to indicate pH changes in a cell culture, but it changes color
from red to yellow with decreasing pH.

Are there measurements available to relate the concentration of phenol
red to its capacity to absorb light (O.D.) and its influence on the
overall color of cell cultures (spectroscopical analysis) ?

Regards,

Peter Van Osta

----------------------------------------------
Peter Van Osta, MD

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 07:47:19 2004

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Hi, all,

I have a collaborator who is interested in looking at some plant material using the LM. He is interested in the staining of lignin and pectin using conventional techniques ( staining these with coloured stains where the components would stain different colours and could be distinguished from each other). My background is EM, and I am not set up for paraffin embedding, so it will have to be some sort of plastic embedding.

I know that there has been some discussion before on the use of LM stains on plastic sections. I'm wondering if the stains (such as Triarch quadruple stain) normally used for lignin and pectin and other plant materials would work if the plastic sections were etched or the plastic removed altogether. Or if there are other stains which I could use.

I hope to do some immuno work on these samples eventually, and maybe some TEM, but the LM has to be done first for us to decide whether to do the other techniques.

So, my questions are:
1. Can the specific botanical stains be used on plastic sections
2. Is there a preferred embedding plastic which I could use (LR white, methacrylate, other???)

Right now the samples are sitting in 2.5% glutaraldehyde in 0.05 M cacodylate buffer.

Thanks for any help with this.

Kind regards,

Paula.

Paula M. Allan-Wojtas
Research Scientist - Food Microstructure/chercheur scientique - microstructure des aliments
Food Safety and Quality team/ Salubrité et qualité des aliments
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 902-679-5566
Facsimile/Télécopieur: 902-679-2311
32 Main Street/ 32, rue Main
Kentville, Nova Scotia/ Kentville (Nouvelle-Écosse)
B4N 1J5

allanwojtasp-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 08:20:19 2004

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Marie,

Assuming these bones aren't museum or type specimens that must remain
unaltered ...
We've done SEM of sub-perisosteal bacteria on bone, and superficial
bacteria using the usual sort of glut fix/EtOH dehydration/CPD, and
this works fine. For bacteria that penetrate bone, though ... if I
had to do SEM, I'd use the standard ("standard") procedures, adding
EtOH cryofracture in LN2 after the last 100% EtOH step to expose the
interior. And, I'd try not doing this, but rather the usual methods
and cracking the bone open after CPD.
And then I won't accept it as definitive or the answer to the
question, merely more information. You mostly likely will need to
section decalcified bone to look for the bacteria, and your best
resource is the collection of boneheads on histonet:
List-Post: {mailto:histonet-at-lists.utsouthwestern.edu}
List-Subscribe: {http://lists.utsouthwestern.edu/mailman/listinfo/histonet} ,
{mailto:histonet-request-at-lists.utsouthwestern.edu?subject=subscribe}
List-Unsubscribe: {http://lists.utsouthwestern.edu/mailman/listinfo/histonet} ,
{mailto:histonet-request-at-lists.utsouthwestern.edu?subject=unsubscribe}
List-Archive: {http://lists.utsouthwestern.edu/pipermail/histonet}
List-Help: {mailto:histonet-request-at-lists.utsouthwestern.edu?subject=help}

There are several very good people well versed with bone
histotechnique. I'd ask them.

Phil

} An Anthropology student came into our EM facility with a sample I
} don't know how to handle. She wants to study the rate and extent of
} bacterial penetration into buried animal bones. She has a few
} previous papers showing methods for doing this, but the pictures are
} poor and methods are not always complete. Some people mention SEM,
} but don't show pictures. More often they seem to be using light
} microscopy of sections (30 microns) of resin embedded material.
}
} We could do SEM but it isn't clear that this is the best approach,
} nor do we know which prep method to use if it is. Some groups
} critical point dry and use an SE detector. Others embed and use a
} backscatter detector. For LM we don't have any microtomes that will
} cut 30 micron sections and the histology group in another department
} has only cut decalcified material. The geology department has a
} diamond saw, but I don't know if this can be used on embedded
} material or whether we would get too much distortion if we try to
} cut or polish unembedded material.
}
} Before we waste a lot of time trying all these options out, do any
} of you have experience with this type of work? Would she need to
} decalcify the bone? Should it be embedded? Would it be better to
} grind the surface and do SEM or cut sections and do light microscopy?
}
} Thanks in advance for any suggestions you can offer.
}
} Marie
}
}
} Dr. Marie E. Cantino
} Director, Electron Microscopy Laboratory
} Associate Professor of Physiology and Neurobiology
} University of Connecticut Unit 3242
} Storrs, CT 06269-3242
} Phone: 860-486-3588
} Fax: 860-486-6369

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 09:56:13 2004

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Try Unicryl. It is a reliable dual-use EM/LM resin.
LR White may work for you too.

usual disclaimers apply (to both).
Chris

----- Original Message -----
} From: "Allan-Wojtas, Paula" {AllanWojtasP-at-AGR.GC.CA}
To: {microscopy-at-msa.microscopy.com}
Sent: Thursday, October 21, 2004 1:53 PM

Paula,
Generally, stains that 'work' in paraffin also work in
plastic. There is not even any need to etch. THe stains are small
molecules and they penetrate easily.

To get information about specific stains, check the book by
Steve Ruzin called Plant Micrototechnique and Microscopy, or
Botanical Microtechnique and Cytochem by Berlyn and Miksche. Or if
you can find it the book by O'Brian and McCully.

Having said that, if contrast is the only issue, its fine.
But if you really want to know that the color is pectin, it is
probably better to use antibody staining. There are quite a few good
ones of those available. I think the dye stains for lignin are
reliable, and I don't know of ab's for that.

For plant material and immuno, I have had very nice results
with butyl-methyl-methacrylate, and I'd be happy to send you a
protocol if you like (mainly for light level work).

As ever,
Tobias

}
} Hi, all,
}
} I have a collaborator who is interested in looking at some plant
} material using the LM. He is interested in the staining of lignin
} and pectin using conventional techniques ( staining these with
} coloured stains where the components would stain different colours
} and could be distinguished from each other). My background is EM,
} and I am not set up for paraffin embedding, so it will have to be
} some sort of plastic embedding.
}
} I know that there has been some discussion before on the use of LM
} stains on plastic sections. I'm wondering if the stains (such as
} Triarch quadruple stain) normally used for lignin and pectin and
} other plant materials would work if the plastic sections were etched
} or the plastic removed altogether. Or if there are other stains
} which I could use.
}
} I hope to do some immuno work on these samples eventually, and maybe
} some TEM, but the LM has to be done first for us to decide whether
} to do the other techniques.
}
} So, my questions are:
} 1. Can the specific botanical stains be used on plastic sections
} 2. Is there a preferred embedding plastic which I could use (LR
} white, methacrylate, other???)
}
} Right now the samples are sitting in 2.5% glutaraldehyde in 0.05 M
} cacodylate buffer.
}
} Thanks for any help with this.
}
} Kind regards,
}
} Paula.
}
} Paula M. Allan-Wojtas
} Research Scientist - Food Microstructure/chercheur scientique -
} microstructure des aliments
} Food Safety and Quality team/ Salubrité et qualité des aliments
} Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
} Telephone/Téléphone: 902-679-5566
} Facsimile/Télécopieur: 902-679-2311
} 32 Main Street/ 32, rue Main
} Kentville, Nova Scotia/ Kentville (Nouvelle-Écosse)
} B4N 1J5
}
} allanwojtasp-at-agr.gc.ca
}
}
}

--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 12:03:25 2004

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Hello:
I am embedding small-grained materials using M-bond 610. I put the materials in
Small capsule with M-bond, keeping ~70 C degree in an oven. However, it seems
that M-bond is evaporated. I appreciate any suggestions you might have. The
reason I am using M-bond is that thinning rate is low during ion-milling.

Thank you,

Hiromi Konishi
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 12:32:04 2004

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Pradyumna:

When doing EBSD with non-conductive small geologic particulates I've
actually had the best using an extremely thin carbon coat and high vac rather
than low vacuum. Never having measured it, my best guess is the coating is 5-
10nm - or as absolutely thin as you can get it, using a good vacuum (10-7
mbar range).

Just a suggestion.

}
} I have following question:
}
} I have a glass-ceramic material, where glass and crystallites have the
} same composition. I want to perform the EBSD on crystallites of this
} material. I can not coat the material because I have to do diffraction.
} I used SE mode with 0.3 torr water pressure but the image quality is not
} good enough for 5 micron size crystallites which have the same
} composition as the glass and which are sticking out only few nanometer
} out of the glass surface (50-60 nm, i can make it 100-200 nm but etching
} but still having difficulty in finding out crystallites). I used the gas
} detector with 1 torr pressure (i can't go below that) and image quality
} improved but the diffraction pattern quality degraded to a level that I
} can not map it properly. Is there a simple way to do EBSD of these
} materials?
}
} Sincerely
} Pradyumna
} Lehigh University
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 15:04:54 2004

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Dear Pradymna,
I would not etch the material at all, EBSD requires a very flat surface. The
best is to go down all the steps of grinding and polishing to one micron
diamond, then long polishing with 0.05 micron silica colloid (Syton). You
may well find that the conditions for good EBSD are the opposite of the
conditions for good imaging, you just change the conditions for each one.
You will find that BSE imaging is best and works at any pressure.
A colleague who did minerals said he polished, then did a very thin carbon
coat, then polished again, then coated again, etc. This filled in any tiny
cracks. A very thin carbon coat will not harm x-ray diffraction studies, it
is invisible to the x-rays.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Pradyumna Gupta" {png2-at-lehigh.edu}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, October 20, 2004 11:17 AM

Dear Hiromi,
I understand that M-610 needs 100 to 120 degrees C to harden. It is usually
used as a thin glue to stick pieces together for cross-sectioning, I do not
know if it can be used as a mounting material.
Good luck,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: {hkonishi-at-indiana.edu}
To: {Microscopy-at-microscopy.com}
Sent: Thursday, October 21, 2004 10:10 AM

Hello,

There is a possibility I might need to work with large gelatin capsules
for inclusion/polymerization of hydrophilic resins (LR White or Unicryl).

However I will need a flat suppor for anatomic orientation.

I thought in cutting ACLAR film to provide flat support, as suggested here
in a previous question about LR White and large samples embedding.

However I have some doubts, and since I have no experience I decided to
post my doubts and ask for your advices.

-If I use large gelatin capsules as thos from Electron Microscopy Sciences
(13 up to 22 mm diameter), I know I can cut a corresponding size ACLAR
round fragment. I can then fill a little resin (to avoid oxygen bubble),
put my ACLAR inside, then my sample and then fill with more resin, and
then go to polymerization. Is this right?

-May I, perhaps cut one rounded ending of the gelatin capsule and glue it
in an ACLAR sheet and then cut around, and then embed and polymerize?
If this is factible, which glue can be used which seals properly and
support either heat or cold UV polymerization? Cyanoacrilate(Super-Bonder,
Loctite®)?

Thanks,
Silvia

_______________________________________________________
Yahoo! Acesso Grátis - Internet rápida e grátis. Instale o discador agora! http://br.acesso.yahoo.com/

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 21 19:41:40 2004

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Hello Microscopists !

As an avid collector/user of Bausch & Lomb metallographs at home
and in my little business, I'd like to tell a story about amazing good
luck ... and ask for a little help in finding a few things.

Years ago I happened upon some Leitz immersion objectives at a flea
market. Many years later, I bumped into a buddy who was very interested
in those objectives, but rather than give them away or try to fleece him, I
suggested that he find and trade a B&L accessory that I had seen touted in
the user's manual of the B&L Balphot I metallograph, the work horse of
production metallography in the period during and after WWII. The
accessory permits use of phase contrast in viewing opaque objects. My
buddy searched for two years to no avail. I eventually traded for something
else so he could acquire the Leitz objectives that he wanted. Fast forward
another five years or so. My excellent microscope service person, John
Sowers of Claymont, DE, came to my office for a regular service call with,
to my astonishment, exactly one of those phase contrast accessories
for the Balphot I. Fits perfectly, works like a charm. Now fast forward
another five years or so. A B&L Research I metallograph appears on
eBay, but in several disjointed pieces. I was lucky enough to get all the
pieces plus a couple of giveaway parts from the seller. At about the
same time, I found and purchased _another_ phase contrast accessory by
B&L, very similar to the firat one but intended to fit a different 'scope.
When it arrives, I discover to my amazement that it's the version that
was intended to fit the Research metallograph. What luck ! But wait,
that's not all. The Research I is missing the binocular eyepiece module,
and I become resolved to making/adapting/fudging in order to gain
easier access to those brilliant images. So I grab a pair of dimly
illustrated binocular modules from eBay and discover to my delight that
one is the missing Research I module and the other fits my Balphot I
exactly as well. So I'm almost "there."

What's still missing is a 20X objective - the type with a tall, thin
barrel and a wide base to accommodate the dark field illumination -
and the parabolic reflectors that complete the dark field light path.
Has anyone got surplus items in this category ? I'm not begging;
I've been purchasing the other items out in the open market, so don't
be bashful. I have all the other objectives that I'll ever need.

Word has it that those phase contrast accessories were never well
accepted in the metallographic community, so extremely few were
ever made. Anyone seen one in serious use out there ?

One more thing - the Research I metallograph had a weak method
of attaching the two major portions of the main microscope body to
each other - four tiny screws that easily strip their threads. I made
and used successfully a jig to bore out the damaged threads, retap
them, fit plugs with tapped holes the same size as the original screws,
and machine flush the plugs. If anyone is in a similar dilemma, I'll
gladly lend you the jig and associated tools. Nothing more than an
eggbeater hand drill and a tap wrench are needed to complete the
repair, once the jig is put to use.

Thanks,
George Langford
amenex-at-amenex.com

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 22 07:58:51 2004

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There is an easier way if an eppendorf type tube is large enough for
you. Check out this web page:
http://www.biotech.ufl.edu/EM/data/disk.html

At 08:17 PM 10/21/2004 -0300, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 22 08:37:36 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rachel-wolf-at-uiowa.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, October 21, 2004 at 14:54:23
---------------------------------------------------------------------------

Email: rachel-wolf-at-uiowa.edu
Name: Rachel Wolf

Organization: University of Iowa

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone know of a seminar of some kind that gives training on Confocal microscopes?? We just got one at our lab and I will be the one using it, but I would like to have more education and background in using one before I jump all the way in. Thanks.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 22 08:52:13 2004

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Announcing the Annual Lehigh Microscopy School.

June 5-17, 2005
Lehigh University
Bethlehem, PA USA

Courses include:

Introduction to SEM and EDS for the New SEM Operator
Scanning Electron Microscopy and X-ray Microanalysis
Problem Solving with Scanning Electron Microscopy
Quantitative X-ray Microanalysis of Bulk Specimens and Particles
Analytical Electron Microscopy
Focused Ion Beam Instrumentation and Applications
Particle and Fiber Characterization
Scanning Probe Microscopy: from Fundamentals to Advanced Applications

Telephone: (610) 758-5133
Fax: (610) 758-4244
E-mail: sharon.coe-at-lehigh.edu
URL: www.lehigh.edu/microscopy

For additional information please contact:
--
********************************
Sharon L. Coe
Events Coordinator
Lehigh Microscopy School
5 East Packer Avenue
Bethlehem, PA 18015
610-758-5133 (phone)
610-758-4244 (fax)
slc6-at-lehigh.ed
www.lehigh.edu/microscopy

********************************

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 22 11:59:47 2004

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Hello

I was wondering if anyone out there in ListServer land has had any
experience with black and white laser printers used for printing electron
micrographs.

Thank you

Ronald L. Austin
Research Associate
Dept. of Pathology
LSU Medical Ct. Shreveport, LA. 71130
rausti-at-lsuhsc.edu
318-675-4557

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 22 18:08:53 2004

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I was shown how RIP software can be used with the Epson 2200, 4000 and up
model printers to print really great B&W prints. Anybody do that on this
list? What are your thoughts and experience.

Damian Neuberger

Hello

I was wondering if anyone out there in ListServer land has had any
experience with black and white laser printers used for printing electron
micrographs.

Thank you

Ronald L. Austin
Research Associate
Dept. of Pathology
LSU Medical Ct. Shreveport, LA. 71130
rausti-at-lsuhsc.edu
318-675-4557

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 07:46:25 2004

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If you are interested in printing Ansel Adams quality EM prints a dedicated
ink jet printer with Quad Black inks is the way to go - to get it right
though requires RIP software..

Bill Miller

At 07:15 PM 10/22/2004, Damian Neuberger wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 09:20:24 2004

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Bill, Damian

What is RIP software?
Chris

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "Bill Miller" {microbill-at-mohawk.net}
To: "Damian Neuberger" {neuberger1234-at-comcast.net} ; "Austin, Ronald"
{RAusti-at-lsuhsc.edu} ; {microscopy-at-msa.microscopy.com}
Sent: Saturday, October 23, 2004 1:52 PM

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 09:58:05 2004

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RIPs (Raster Image Processors)

At 10:26 AM 10/23/2004, Chris Jeffree wrote:
} Bill, Damian
}
} What is RIP software?
} Chris
}
} Dr. Chris Jeffree
} University of Edinburgh
}
} ----- Original Message ----- From: "Bill Miller" {microbill-at-mohawk.net}
} To: "Damian Neuberger" {neuberger1234-at-comcast.net} ; "Austin, Ronald"
} {RAusti-at-lsuhsc.edu} ; {microscopy-at-msa.microscopy.com}
} Sent: Saturday, October 23, 2004 1:52 PM
} Subject: [Microscopy] Re: RE: Laser printers
}
}
} }
} }
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 11:14:19 2004

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OK, sounds like this may be a MAC thing.
Chris

----- Original Message -----
} From: "Bill Miller" {microbill-at-mohawk.net}
To: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
Cc: {microscopy-at-msa.microscopy.com}
Sent: Saturday, October 23, 2004 4:04 PM

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 11:31:53 2004

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We have a Zeiss 109 TEM that was very lightly used and needs to be moved.
This microscope blew it's turbo pump a few years ago and has not been under
vacuum since. So it is not working and I would not guarantee that it could
be gotten up and running. However, it is a gold mine as to parts as it
probably only has about 100-150 beam hours on it.

Free to academic home but you must arrange for transfer within 2 weeks.
Small negotiable charge for commercial use. (i.e. Where parts are going to
be resold).

Contact soon as it will be out the door in two weeks.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 12:21:55 2004

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To see 2 popular RIPs go to:

StudioPrint at http://www.ergosoftus.com/index.php

ImagePrint at http://www.colorbytesoftware.com/

} What is RIP software?
} Chris
}
} Dr. Chris Jeffree
} University of Edinburgh
}
} ----- Original Message -----
} } From: "Bill Miller" {microbill-at-mohawk.net}
} To: "Damian Neuberger" {neuberger1234-at-comcast.net} ; "Austin, Ronald"
} {RAusti-at-lsuhsc.edu} ; {microscopy-at-msa.microscopy.com}
} Sent: Saturday, October 23, 2004 1:52 PM
} Subject: [Microscopy] Re: RE: Laser printers
}
}
} }
} }
} }
----------------------------------------------------------------------------
-} } -
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -----------------------------------------------------------------------------
} } --
} }
} } If you are interested in printing Ansel Adams quality EM prints a
} } dedicated ink jet printer with Quad Black inks is the way to go -
} } to get it right though requires RIP software..
} }
} } Bill Miller
} }
} } At 07:15 PM 10/22/2004, Damian Neuberger wrote:
} }
} }
} } } ----------------------------------------------------------------------------
} } } --
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } } America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help
} } } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } } ----------------------------------------------------------------------------
} } } ---
} } }
} } } I was shown how RIP software can be used with the Epson 2200, 4000
} } } and up
} } } model printers to print really great B&W prints. Anybody do that on
} } } this
} } } list? What are your thoughts and experience.
} } }
} } } Damian Neuberger
} } }
} } } Hello
} } }
} } } I was wondering if anyone out there in ListServer land has had any
} } } experience with black and white laser printers used for printing
} } } electron
} } } micrographs.
} } }
} } } Thank you
} } }
} } } Ronald L. Austin
} } } Research Associate
} } } Dept. of Pathology
} } } LSU Medical Ct. Shreveport, LA. 71130
} } } rausti-at-lsuhsc.edu
} } } 318-675-4557
} }
} }
} }
} }
}
}

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 12:28:46 2004

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Chris

Nope, RIP is not a "Mac thing" but a more general combination of hardware and software
which a printer uses to convert vectorized objects text, lines, objects, etc... into the bitmaps
(i.e. array of dots) which are printable using " printing" technologies
that a modern printers employ.

All high end printers have RIP's built into their processors. The low end
printers require your local CPU to convert objects into bitmaps which are
then transferred to the printhead.

Postscript fonts and vector graphics for example have to be rasterized to be printed.

While images (BMP, TIFF, GIF, JPEG) are essentially already bitmaps and
do not have to be processed (as much) to be output.

Nestor
Your Friendly Neighborhood SysOp.

} X-Authentication-Warning: ns.microscopy.com: mail set sender to MicroscopyL-request-at-ns.microscopy.com using -f
} From: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
} To: "Bill Miller" {microbill-at-mohawk.net}
} Cc: {microscopy-at-msa.microscopy.com}
} Subject: [Microscopy] Re: Re: RE: Laser printers
} Date: Sat, 23 Oct 2004 17:20:28 +0100
} X-Priority: 3
} Status:
}
}
}
} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 12:44:27 2004

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No, available for Windows and Macs
Damian

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Saturday, October 23, 2004 11:20 AM
To: Bill Miller
Cc: microscopy-at-msa.microscopy.com

OK, sounds like this may be a MAC thing.
Chris

----- Original Message -----
} From: "Bill Miller" {microbill-at-mohawk.net}
To: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
Cc: {microscopy-at-msa.microscopy.com}
Sent: Saturday, October 23, 2004 4:04 PM

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 13:36:05 2004

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When I first took over Microscopy Today and sent my Adobe InDesign files
that contained the "camera ready" version of the current MT issue to the
printer, the printer prepress contractor said they would RIP it. I was upset
naturally, given all the work I had put into it.

I since learned that RIP is a hardware-software combination that converts a
vector image into a bit-mapped image. All PostScript printers contain a RIP
that converts the PostScript commands into bit-mapped pages that the printer
can output. The RIP is at the heart of the digital imaging process and does
all the work. The ultimate result is a printed or imaged page, panel, sheet
of film, or four half-tone screens for each of the printing press print
stations (CMYK). In MT's case it is the four screens that are loaded into
the printing press the prints MT. Hence the quotes around "camera ready",
above. There is no camera in this century.

Ron Anderson

-----Original Message-----
} From: Bill Miller [mailto:microbill-at-mohawk.net]
Sent: Saturday, October 23, 2004 11:04 AM
To: Chris Jeffree
Cc: microscopy-at-msa.microscopy.com

RIPs (Raster Image Processors)

At 10:26 AM 10/23/2004, Chris Jeffree wrote:
} Bill, Damian
}
} What is RIP software?
} Chris
}
} Dr. Chris Jeffree
} University of Edinburgh
}
} ----- Original Message ----- From: "Bill Miller" {microbill-at-mohawk.net}
} To: "Damian Neuberger" {neuberger1234-at-comcast.net} ; "Austin, Ronald"
} {RAusti-at-lsuhsc.edu} ; {microscopy-at-msa.microscopy.com}
} Sent: Saturday, October 23, 2004 1:52 PM
} Subject: [Microscopy] Re: RE: Laser printers
}
}
} }
} }
} } --------------------------------------------------------------------------
----
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 15:23:06 2004

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Nestor
OK, I'll admit I was just being gratuitously provocative,
but we're still no nearer having an answer to the question
arising from Bill & Damian's comments about RIPs: namely
if (as implied) there is an advantage in using RIP software compared
with printing the image direct from Adobe Photoshop using
the standard Epson printer driver then why does that arise?

Best wishes
Chris Jeffree

----- Original Message -----
} From: "Nestor J. Zaluzec" {zaluzec-at-microscopy.com}
To: {microscopy-at-microscopy.com}
Sent: Saturday, October 23, 2004 6:36 PM

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 23 16:22:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jmo12505-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, October 23, 2004 at 15:06:00
---------------------------------------------------------------------------

Email: jmo12505-at-yahoo.com
Name: Judy

Organization: Saint Louis University

Title-Subject: [Microscopy] [Filtered] Advice on plastic options

Question: I have been using Epon Araldite plastic for many years for both EM and LM (1 micron) sectioning. I am gearing up for a new project that will involve embedding and 1 micron sectioning of a fairly large number of mouse brains. I will not need to do any EM on this tissue. I also have several undergraduates who are interested in participating in the project but have no prior histology experience. Are any of the newer plastics easier to work with for embedding and sectioning?
Thanks in advance,
-Judy

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 24 10:48:02 2004

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hello,

We are in urgent need of Freon gas for Jeol 1200 EXII
We are ready to pay the charges

Regards
Arti

_______________________________
Do you Yahoo!?
Declare Yourself - Register online to vote today!
http://vote.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 25 08:21:53 2004

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SEM WORKSHOP
Presented by:
Midwest Microscopy and Microanalysis Society

Affiliate of the Microscopy Society of America and the Microbeam Analysis Society of America

November 19th, 2004
8:00AM - 5:00PM
Baxter Corporate Headquarters
Deerfield, IL
Directions and map at http://www.microscopy.org/MSALAS/MMMS

Registration Fees:
MMMS members: before Nov. 5th - $ 25.00 after Nov. 5th - $ 35.00
Non-members: before Nov. 5th - $35.00, after Nov 5th - $ 45.00 (MMMS membership included in fee)
Students: before Nov. 5th - $15.00, after Nov 5th - $ 25.00 (MMMS Student membership $5)

Vendors: We welcome vendors, tables for literature & exhibits available. Contact us for details.

8:00AM - 8:45AM Setup and registration

8:45 - 10:15AM - James Pawley, University of Wisconsin, What FE does for SEM?

10:15 - 10:45AM Break

10:45AM - 12:15PM - John Mackenzie, North Carolina State University,
Work flow for digital imaging in a modern microscopy laboratory II

12:15PM - 1:15PM LUNCH - Included

1:15PM - 2:45PM - Alwyn Eades, Lehigh University, Crystallographic analysis in the Scanning Electron Microscope

2:45 - 3:15PM Break

3:15 - 4:45PM - Dennis Ward, Federal Bureau of Investigation, Microanalysis - A New Tool in Combating Terrorism

Directions to Baxter Corporate Headquarters: 1 Baxter Parkway, Deerfield Illinois, 60015.

Please RSVP via email, phone, or fax to:
Arvid Casler - MMMS Program Coordinator
847-566-7716 Voice Mail and Fax
arvid_casler-at-fmo.com

NOTE: RSVPs will be responsible for registration fees

Robert Mierzwa
Midwest Regional Sales Manager
JEOL USA, Inc.
3906 Lisa Ave.
Sheboygan WI 53083
TEL (920) 803-8945
FAX (920) 803-8946
Email: mierzwa-at-jeol.com

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 25 09:56:21 2004

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Hi Debby,
I sent your note to a friend who works on Zeiss scopes and has parts
for the older orange-column scopes. He says he can have your 109
resurrected for a few thousand dollars. Are you sure you want to get
rid of this scope? I will be happy to share service info with you.
best,
Beth

On Saturday, October 23, 2004, at 12:38 PM, Debby Sherman wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
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} --------
}
} We have a Zeiss 109 TEM that was very lightly used and needs to be
} moved.
} This microscope blew it's turbo pump a few years ago and has not been
} under
} vacuum since. So it is not working and I would not guarantee that it
} could
} be gotten up and running. However, it is a gold mine as to parts as it
} probably only has about 100-150 beam hours on it.
}
} Free to academic home but you must arrange for transfer within 2 weeks.
} Small negotiable charge for commercial use. (i.e. Where parts are
} going to
} be resold).
}
} Contact soon as it will be out the door in two weeks.
}
} Debby
}
} Debby Sherman, Manager Phone: 765-494-6666
} Life Science Microscopy Facility FAX: 765-494-5896
} Purdue University E-mail: dsherman-at-purdue.edu
} S-052 Whistler Building
} 170 S. University Street
} West Lafayette, IN 47907
} http://www3.agriculture.purdue.edu/microscopy
}
}
}
}
**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 25 11:01:34 2004

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Dear All EM Specialists:

I have a question about how to prepare SEM sample of automobile catalyst with metallic substrate. For the catalyst on ceramic substrate we drill a core, embed it in Epoxy and polish it. It is very hard to get a core from metallic substrate but still keep the original washcoat distribution without shaking it off by the strong vibration during cutting. Is there any special tool for cutting? After getting a core do I need to embed it in Epoxy and polish it?

Could you please kindly share your experience with me?

Thanks

Ying Shi

Analytical Scientist
Delphi Catalyst

Tel:918-266-4942
Fax:918-266-4983
E-mail:ying.shi-at-delphi.com

****************************************************************************************

Note: The information contained in this message may be privileged and confidential and thus protected from disclosure. If the reader of this message is not the intended recipient, or an employee or agent responsible for delivering this message to the intended recipient, you are hereby notified that any dissemination, distribution or copying of this communication is strictly prohibited. If you have received this communication in error, please notify us immediately by replying to the message and deleting it from your computer. Thank you.

****************************************************************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 25 15:56:10 2004

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Wise ones in netland,
This is a little off straight up microscopy but not
all that far. My colleague Louis Cardenes asks:

I want to know how to make good microinjection needles with a
Flaming/Brown micropipette Puller from Sutter Instrument.
The needles are desired to be around 0.2 micrometer (internal
diameter) and will be used for plant cell injections. What I need is
a good protocol and the right platinum filament that should be used.

Can anyone help? Even to the point of suggesting an electrophys email
listserver? Please include Louis' address (luisc-at-ibt.unam.mx) in your
reply because he doesn't subscribe to this list.

Thanks all,
Tobias
--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 25 17:20:01 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (m.serracino-at-igag.cnr.it) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, October 25, 2004 at 08:55:29
---------------------------------------------------------------------------

Email: m.serracino-at-igag.cnr.it
Name: Marcello Serracino

Organization: Institute of Environmental Geology and Geoengineering

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Our Link eXL computer graphics board c1907 has died and we are scrambling for a quick replacement. Does anyone have a graphics board c1907 or have any not very expensive suggestions?
Thanks to all who responded to the crisis of repairing or replacing the board.

Marcello Serracino
m.serracino-at-igag.cnr.it
Sx50 microprobe operator
Institute of Environmental Geology and Geoengineering

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Oct 25 21:59:59 2004

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Dear All,

I did read some note about the external connection of JEOL Sem 840 with PC.

There is a person from Alcoa Technical center proposed to use the MACADios
card. It is able to interface the SEM and PC to grab SEM images. Does anyone
has the contact and fax of the GW instruments who selling MAC ADios IIJr ?
Let me know in your next email.

Thanks
Kok Swee

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 07:20:05 2004

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Thomas, depending on what kind of resolution you need and types of
samples, you might try Profilometry. Zygo Corp. may be able to help you
and they're right here in CT. The link is: www.zygo.com. Contact them
of feel free to contact myself if you have any questions.

Ed Komarnicki
Sr. Analytical Chemist
MacDermid Inc.
(203) 575-5750

Disclaimer: I have no capital interest in this company.

"Thomas Sadowski" {tommy91779-at-hotmail.com}
10/10/04 06:43 PM

To
Microscopy-at-MSA.Microscopy.Com
cc

Subject
Using Texture Parameters

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hello everyone,

I am currently involved in a research project that is using many different
imaging modalities to look at objects of a variety of sizes. I am
interested
in using texture parameters to try to classify this material and was
wondering if there was any existing computer programs or relevant papers
written that could help my with my project.

Please feel free to email me if you think you can help. Thank you all for
your time.

Thomas Sadowski
Southern Connecticut State University

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 09:17:31 2004

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RESEARCH ASSOCIATE POSITION

COMPOSITE MATERIALS AND STRUCTURES CENTER

MICHIGAN STATE UNIVERSITY

EAST LANSING, MI 48824-1326

A research associate is sought to serve as principle investigator and
primary operator of the Digital Instruments Scanning Probe Microscope
which is operated as a University user and outreach facility. The
individual in this position will conduct research on materials
characterization and behavior with the SPM and interact with faculty and
students as well as industrial and governmental personnel. Materials and
processing research involving composite materials, metals, ceramics,
polymers, cement, asphalt, food, packaging materials, soils, and plants is
being conducted with the SPM. In particular this unit is equipped with
stages capable of varying temperature, ambient environment, tapping mode
capabilities, scanning tunneling head, and indentation modules as part of
the research studies on these materials. The person occupying this
position will be responsible for the operation and maintenance of the
unit, provide training of faculty, staff, graduate students and off-campus
users and conduct research with this unit. In addition this person will
be expected to develop contacts with potential users from off campus in
the local and state-wide community to assist in generating research funds
as part of the outreach activity of the SPM facility.

Qualifications: A Ph.D. in Materials Science, Physics, Chemistry, or
Engineering is required. Experience with scanning probe microscopy
required, with preferred experience with Digital Instruments Nanoscope
series of controllers. The applicant must exhibit very high levels of
English oral and written communication skills.

Applications: Position is open until filled. Salary is dependent on
qualifications and experience. Send a complete curriculum vitae, graduate
level transcript and three references to Michael J. Rich, Michigan State
University, Composite Materials and Structures Center, 2100 Engineering
Building, East Lansing, MI 48824-1226, ; Email: RICH-at-EGR.MSU.EDU

Additional information describing the Composite Materials and Structures
Center facility is available at: http://www.egr.msu.edu/cmsc

MSU is an affirmative action, equal opportunity institution.

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 10:03:31 2004

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Colleagues

I cannot unfortunately help Marcello Serracino with his eXL graphics board woes
but I have the following eXL PC boards available (FREE) to whomever
could use them from a circa 1991 Oxford/Link eXL microanalysis system
which I decommissioned only yesterday.

PC2300 M.D.I (Mk.2) BD
PC1789 MUX BD
PC2733 GSP BD
PC2391 Electron Signal Cond. BD
PC1585 M.D.I Bd
PC 1171-V1 W.D. Interface BD.

Nestor
Your Friendly Neighborhood SysOp
--
===========================================
Dr. Nestor J. Zaluzec
Argonne National Lab
Materials Science Division/Bldg 212
9700 S. Cass Ave
Argonne, Illinois 60439 USA
Tel: 630-252-7901, Fax: 630-252-4798
Email: Zaluzec-at-aaem.amc.anl.gov
===========================================
TPMLab: http://tpm.amc.anl.gov
NEESLab: http://neestpm.mcs.anl.gov
MMSite: http://www.amc.anl.gov
===========================================

The box said ...
"This program requires Win 95/98/NT or better..."
So I bought a G3 Mac !

===========================================

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 10:14:09 2004

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Oops... Nestor was wrong...

Marcello, in the another old box of electronic components hidden away in
a corner I found a complete eXL GDP PC 1907 graphics board. !

I had forgotten that I replaced the eXL video system with a more
modern display board
which is VGA compatible. The 1907 board only works with the old
style eXL monitors.

It hasn't been used in years, however I will mail it to you, if you still
need it. Just contact me off line.

Nestor

Your Friendly Neighborhood SysOp

------------------------------------------------------------------------------
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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (m.serracino-at-igag.cnr.it) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Monday, October 25, 2004 at 08:55:29
---------------------------------------------------------------------------

Email: m.serracino-at-igag.cnr.it
Name: Marcello Serracino

Organization: Institute of Environmental Geology and Geoengineering

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Our Link eXL computer graphics board c1907 has died and we
are scrambling for a quick replacement. Does anyone have a graphics
board c1907 or have any not very expensive suggestions?
Thanks to all who responded to the crisis of repairing or replacing the board.

Marcello Serracino
m.serracino-at-igag.cnr.it
Sx50 microprobe operator
Institute of Environmental Geology and Geoengineering

---------------------------------------------------------------------------
--
===========================================
Dr. Nestor J. Zaluzec
Argonne National Lab
Materials Science Division/Bldg 212
9700 S. Cass Ave
Argonne, Illinois 60439 USA
Tel: 630-252-7901, Fax: 630-252-4798
Email: Zaluzec-at-aaem.amc.anl.gov
===========================================
TPMLab: http://tpm.amc.anl.gov
NEESLab: http://neestpm.mcs.anl.gov
MMSite: http://www.amc.anl.gov
===========================================

The box said ...
"This program requires Win 95/98/NT or better..."
So I bought a G3 Mac !

===========================================

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 12:21:13 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Colleagues,
I would like to thank one and all for their input concerning the laser
printer question I posted.

Sincerely

Ronald L. Austin
Research Associate
Dept. of Pathology
LSU Medical Ct. Shreveport, LA. 71130
rausti-at-lsuhsc.edu
318-675-4557

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 15:32:59 2004

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Are single wall and multi-wall nanotube probes readily and commercially available for AFM? for STM?

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 15:40:11 2004

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Dear colleagues,

We are in need of Si (111) TEM sample (3mm disk) for
our JEM-2010F CBED pattern test urgently. If you
happen to have it, could you please mail me one sample
as soon as possible? If you still need this sample, I
will return it after our test. We appreciate your
timely help.

Following is my mailing address:
Qi Zhang
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599-3255.

Thank you very much!

Regards,
**************************************************
Qi Zhang, Ph.D
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599
Tel: 919-843-2407 (Office)
919-843-0974 (EM Lab)
Fax: 919-962-0480
E-mail: qizhang-at-physics.unc.edu

__________________________________
Do you Yahoo!?
Yahoo! Mail - Helps protect you from nasty viruses.
http://promotions.yahoo.com/new_mail

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 16:46:02 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (qizhang-at-physics.unc.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 26, 2004 at 16:34:14
---------------------------------------------------------------------------

Email: qizhang-at-physics.unc.edu
Name: Qi Zhang

Title-Subject: [Microscopy] [Filtered] MListserver: need Si [111] TEM sample (3mm disk)

Question: Dear colleagues,

We are in great need of Si [111] TEM sample (3mm disk) for
our JEM-2010F CBED pattern test urgently. If you
happen to have it, could you please mail me one sample
as soon as possible? If you still need this sample, I
will return it after our test. We appreciate your
timely help.

Following is my mailing address:
Qi Zhang
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599-3255.

Thank you very much!

Regards,
**************************************************
Qi Zhang, Ph.D
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599
Tel: 919-843-2407 (Office)
919-843-0974 (EM Lab)
Fax: 919-962-0480
E-mail: qizhang-at-physics.unc.edu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 16:45:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (spradhan-at-siu.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 26, 2004 at 14:55:46
---------------------------------------------------------------------------

Email: spradhan-at-siu.edu
Name: sailesh

Organization: Southern Illinois University

Title-Subject: [Microscopy] [Filtered] MListserver: A used stage for the SEM

Question: hello everyone!

i am looking to see if there are any used loading stages for the hitachi S-2460N SEM. i am working on a project with a professor and we want to take some images of a thin-film under loading using the SEM(we want to work on speckle
pattern interferometry with electron microscopy).
what we have in mind is a stage(a door and a pass-through) that is designed for such purposes and can enable us to perform the tests on the SEM without having to go through the entire process of building it from scratch. so it would be nice to know of any such stages that are available. i would appreciate it very much if you could even give me a rough estimate of how much anything like it would cost.
thank you...i shall look forward to hearing from you soon.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Oct 26 18:07:35 2004

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Hi All,

When I called to order chemicals for our AGFA Rapidoprint Processor (AGFA
Rapidoprint Activator G182B and AGFA Rapidoprint Fixer QSO4A), I was told
by my supplier that AGFA is no longer manufacturing them. I called the
AGFA technical support line, but they could not suggest direct
replacements nor would they share the formulas for the discontinued
products with me so that I can make them myself. The ingredients in the
two are common photo chemicals (for the activator water, ammonium
thiosulfate and sodium sulfite; for the fixer water, sodium hydroxide and
sodium sulfite).

Has anyone already grappled with this problem and found suitable
replacements? I could find nothing on the web and the compositions of the
products are not given in the Morgan & Morgan Photo Lab Index - at least
not in the vintage copy in our library.

Least you think we're in the dark ages here, we do have a film scanner.
There are just some old fashioned microscopists here (mainly me!) who
still prefer stacks of study prints for data analysis over stacks of CDs.

Thanks for any forthcoming solutions ;)

Heather Owen

Dr. Heather A. Owen, Director
Electron Microscope Laboratory
Department of Biological Sciences
University of Wisconsin - Milwaukee
Lapham Hall, P.O. Box 413
Milwaukee, WI 53210
USA

Phone: (414)229-6816

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 01:17:13 2004

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Hello Heather,

Afraid I haven't found the specific formulas, and not terribly familiar
with machine processing, but have some thoughts that I hope will be helpful.

First, to mention that whoever told you of the chemistry you described
has things reversed. Sodium hydroxide is a common high-energy alkalai
"accelerator" used in some developers, while ammonium thiocyanate has long
been a standard replacement for sodium thiosulfate in rapid fixers. I think
rapidoprint is a paper that has the developing agent as well as restrainer
built-in, and so the "developer" itself may be no more than the NaOH-sulfite
solution, and if so it might just be a question of playing around with
solution percentages. And in a very old copy of P.L.I. (1946) I find the
following: "A 15-20% solution of ammonium thiosulfate is capable of more
rapid fixation than a 35-40% solution of sodium hydroxide."

My own guess is that the one risk with experimenting with chemistry in
the machine would be related to burning of the seals and possibly filters,
but I find it hard to imagine any other ingredients than those you mentioned
could be more corrosive than the hydroxide.

There's a site on the web called the Analog Photography Users Group,
which has a forum dealing with traditional processes, and some of the
members might be familiar with machine chemistry. Give it a try:

http://www.apug.org/forums/home.php

Finally, me being an old and "old fashioned" photographer, I'd encourage
you: never, NEVER, apologize for using silver processes!!!!! (ad infinitum
!!!!!'s)

Cheers, hope this helps,
Larry Weissmann
Tweed, Ontario, Canada
Tel: (613) 478-4743

**********************************
HEATHER OWEN WROTE

Hi All,

When I called to order chemicals for our AGFA Rapidoprint Processor (AGFA
Rapidoprint Activator G182B and AGFA Rapidoprint Fixer QSO4A), I was told
by my supplier that AGFA is no longer manufacturing them. I called the
AGFA technical support line, but they could not suggest direct
replacements nor would they share the formulas for the discontinued
products with me so that I can make them myself. The ingredients in the
two are common photo chemicals (for the activator water, ammonium
thiosulfate and sodium sulfite; for the fixer water, sodium hydroxide and
sodium sulfite).

Has anyone already grappled with this problem and found suitable
replacements? I could find nothing on the web and the compositions of the
products are not given in the Morgan & Morgan Photo Lab Index - at least
not in the vintage copy in our library.

Least you think we're in the dark ages here, we do have a film scanner.
There are just some old fashioned microscopists here (mainly me!) who
still prefer stacks of study prints for data analysis over stacks of CDs.

Thanks for any forthcoming solutions ;)

Heather Owen

Dr. Heather A. Owen, Director
Electron Microscope Laboratory
Department of Biological Sciences
University of Wisconsin - Milwaukee
Lapham Hall, P.O. Box 413
Milwaukee, WI 53210
USA
Phone: (414)229-6816

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 01:32:06 2004

Contents Retrieved from Microscopy Listserver Archives
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Heather,

My quote from Photo Lab Index should read:

"A 15-20% solution of ammonium thiosulfate is capable of more
rapid fixation than a 35-40% solution of sodium THIOSULFATE."

Sorry for the mistake, it's 2 AM.
Larry Weissmann

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 02:05:54 2004

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Heather

I see that MACO Photo Products list processor chemistry, but I think
this could be a conventional developer formulation and not a
Rapidoprint-compatible activator. Anyway, it could be worth asking
them your question?? Also, check out the other silver photography
products they supply:
http://www.mahn.net/Frameset.htm
MACO is a division of Hans O. Mahn & Co. KG, Brookstieg 4, 22145
Stapelfeld, Germany
Hotline: 040-237 008-88 von 9:00 - 16:00Uhr,
e-mail: PHOTO-at-mahn.net

Agfa applied for a patent 1997 to extend the Rapidoprint principle
(crudely put, the developer chemistry is built-in to the emulsion) to
radiographic emulsions. In this application (which is available to
view on the internet) they quote activator and fixer formulae as
follows:

Composition of the activation liquid (per litre).

potassium hydroxide 30 g
potassium sulphite 50 g
potassium bromide 2 g
ethylene diamine tetra acetic acid, sodium salt 1.5 g

Composition of the fixing liquid (per litre).

ammonium thiosulphate 100 g
sodium sulphite 17 g
sodium acetate 15 g
citric acid 2.5 g
acetic acid 13 ml

The rinsing liquid was distilled water.

I would experiment with 3% KOH to activate and your regular ammonium
thiosulphate fixer at
appropriate dilution to fix.

Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "Heather A Owen" {owenha-at-csd.uwm.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Wednesday, October 27, 2004 12:17 AM

Dear All,

does anyone know the bethe range and Kanaya Okayama range of carbon from
20kev to 30kev. Let me know.

Many thanks
Ks

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 08:07:54 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ajenning-at-cyllene.uwa.edu.au) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, October 26, 2004 at 22:58:40
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Email: ajenning-at-cyllene.uwa.edu.au
Name: alison jennings

Organization: university of western australia

Title-Subject: [Microscopy] [Filtered] IHC and TEM of zinc-fixed tissue

Question: I was wondering if anyone has used zinc fixative (based on Zinc salts in TBS and avaailable commercially for LM-level fixation) for EM preparation. It is supposed to retain many antigens which are masked by formalin, para or glutaraldehyde, also reducing the need for antigen retrieval. So far I haven't seen any reference including ultrastructural performance, nor has there been any satisfactory explanation of how the fixative actually works. As well as 3micron paraffin immunohistochemistry, I am interested in 1 micron araldite immunostaining.
Many thanks
Alison

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Qi, A very simple way to make a Si(111) sample is to take a small piece of
Si wafer and crush it in a mortar and pestle with a bit a ethanol. Then
place a drop of the slurry on a holey carbon grid (you may have to play with
the concentration a bit). You will need to hunt around a bit to get the
correct zone axis, but you should be able to find nearly zone with out
tilting too far. Look for small thin flakes that look nearly invisible with
the TEM in focus.

Good luck, Ray

Ray D. Twesten, PhD.
Center for Microanalysis of Materials
Seitz Materials Research Laboratory
104 S. Goodwin Ave., Urbana, IL 61801
+1 217 244-6177 (Fax -2278)

-----Original Message-----
} From: Zhang Qi [mailto:qzhangtj-at-yahoo.com]
Sent: Tuesday, October 26, 2004 3:49 PM
To: MSA listserver
Cc: Lu-Chang Qin; Gary T Griego

Dear colleagues,

We are in need of Si (111) TEM sample (3mm disk) for
our JEM-2010F CBED pattern test urgently. If you
happen to have it, could you please mail me one sample
as soon as possible? If you still need this sample, I
will return it after our test. We appreciate your
timely help.

Following is my mailing address:
Qi Zhang
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599-3255.

Thank you very much!

Regards,
**************************************************
Qi Zhang, Ph.D
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599
Tel: 919-843-2407 (Office)
919-843-0974 (EM Lab)
Fax: 919-962-0480
E-mail: qizhang-at-physics.unc.edu

__________________________________
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From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 16:35:31 2004

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In the book "Scanning Electron Microscopy and X-Ray Microanalysis" (by J. I.
Goldstein et al., 2nd edition), you will find equations for calculating
Bethe's or Kanaya Okayama range (p. 88 and 89).
Here are the values for carbon as given in Table 3.2 of this book (p.89):

Bethe range:
20 keV --} 7.5 micrometers (micron)
30 keV --} 13 micrometers (micron)

Kanaya Okayama range
20 keV --} 5.3 micrometers (micron)
30 keV --} 10.4 micrometers (micron)

Jean-Paul Baďlon

++++++++++++++++++++++++++++++++++++++
Prof. Jean-Paul Baďlon jean-paul.bailon-at-polymtl.ca
Génie mécanique Tél: +1(514) 340 4711, p. 4260
École Polytechnique Fax: +1(514) 340 4468
CP 6079, Succursale Centre-Ville
Montréal (QC) Canada H3C 3A7
++++++++++++++++++++++++++++++++++++++

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 17:14:44 2004

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Hi.
I am a new user of Philips scope CM300. I have used JEOL scopes. I found some
difference in alignment procedures, and I have tubules with that.

1. I have troubles in understanding the relation between setting eucentric
height and objective lens current in Philips scope. If I set eucentric height,
it is not focus position. After I get eucentric height and I get focus position
using focus nob, I can get an objective current. Objective lens current should
be constant, but the obtaining objective lens current is not the same.

When I use JEOL scopes, I do not touch coarse focus nob, but change height (Z)
to keep the same objective lens current. Generally, how HRTEM people control
objective lens current and height in Philips scope?

2. Do HRTEM people adjust Voltage center and Coma free on CM300? Just do you do
Current center and Coma free?

Thank you,
Hiromi Konishi
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Wed Oct 27 18:11:11 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (nbiswas-at-chem.uga.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, October 27, 2004 at 12:24:50
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Email: nbiswas-at-chem.uga.edu
Name: Nilanjana Biswas

Organization: University of Georgia

Title-Subject: [Microscopy] [Filtered] MListserver: Temp. regulated microscope stage

Question: We have an Olympus BX60 microscope (upright and confocal).I need to do some temperature dependent studies of samples on glass slides for which I need a temperature range of ~20-60C. I was looking at the TS-4 and TS-4ER stages from Physitemp. I would appreciate some information on them.How good are they?If there are some other porducts please let me know.

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The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
}
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Heather -

What paper are you using in the processor. If I recall
Agfa stopped
making that Rapidoprint paper years ago. You could
possibly use whatever chemistry for the paper you are
using.

ML

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Society of America

When I called to order chemicals for our AGFA Rapidoprint
Processor (AGFA
Rapidoprint Activator G182B and AGFA Rapidoprint Fixer
QSO4A), I was told
by my supplier that AGFA is no longer manufacturing them.
I called the
AGFA technical support line, but they could not suggest
direct replacements nor would they share the formulas for
the discontinued products with me so that I can make them
myself. The ingredients in the two are common photo
chemicals (for the activator water, ammonium thiosulfate
and sodium sulfite; for the fixer water, sodium hydroxide
and sodium sulfite).

Has anyone already grappled with this problem and found
suitable replacements? I could find nothing on the web and
the compositions of the
products are not given in the Morgan & Morgan Photo Lab
Index - at least not in the vintage copy in our library.

Least you think we're in the dark ages here, we do have a
film scanner. There are just some old fashioned
microscopists here (mainly me!) who still prefer stacks of
study prints for data analysis over stacks of CDs.

Thanks for any forthcoming solutions ;)

Heather Owen

Dr. Heather A. Owen, Director
Electron Microscope Laboratory
Department of Biological Sciences
University of Wisconsin - Milwaukee
Lapham Hall, P.O. Box 413
Milwaukee, WI 53210
USA
Phone: (414)229-6816

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 02:31:47 2004

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Dear Hiromi,

There should be no real difference between a JEOL TEM and
FEI TEM. On a side entry machine the engineer should set
the eucentric height of the stage at the optimum objective
lens focus. If this is not the case I suggest you ask your
engineer to check it out.

If you are saying that the focus current changes even
though the eucentric height is set, this certainly should
not happen and should be checked out by your engineer. A
change in objective lens focus current at eucentric
height could indicate a stage, lens or HT problem.

Good luck
Ron

On Wed, 27 Oct 2004 17:24:31 -0500 hkonishi-at-indiana.edu
wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Hi.
} I am a new user of Philips scope CM300. I have used JEOL scopes. I found some
} difference in alignment procedures, and I have tubules with that.
}
} 1. I have troubles in understanding the relation between setting eucentric
} height and objective lens current in Philips scope. If I set eucentric height,
} it is not focus position. After I get eucentric height and I get focus position
} using focus nob, I can get an objective current. Objective lens current should
} be constant, but the obtaining objective lens current is not the same.
}
} When I use JEOL scopes, I do not touch coarse focus nob, but change height (Z)
} to keep the same objective lens current. Generally, how HRTEM people control
} objective lens current and height in Philips scope?
}
} 2. Do HRTEM people adjust Voltage center and Coma free on CM300? Just do you do
} Current center and Coma free?
}
} Thank you,
} Hiromi Konishi
} Indiana University
}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

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Dear Listers,

Is there a shelf life for probes for contact and
tapping modes in AFM, How do we know that the probes
used for AFM are no longer good if they are old and
unused what are the signs.
shashi singh
CCMB Hyderabad

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From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 09:41:33 2004

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STUDENT POSTER COMPETITION ANNOUNCEMENT

To be held in conjunction with the March 24,2005 meeting of the Midwest
Microscopy and Microanalysis Society

Affiliate of the Microscopy Society of America and the Microbeam
Analysis Society of America

ABSTRACT DEADLINE: Abstracts must be received in electronic format by
5PM, Wednesday, December 15, 2004.

The first quarter meeting of the Midwest Microscopy and Microanalysis
Society will be held on Thursday, March 24, 2005, in the Pancoe Life
Sciences Building, Northwestern University, Evanston, Illinois. A
student poster competition open to undergraduate and graduate students
will be held in conjunction with the meeting. Posters should illustrate
utilization of microscopy for either biological or materials science
study. Prizes will be awarded as follows:

$300 for 1st place
$200 for 2nd place
$100 for 3rd place

Abstracts must be received in electronic format by 5PM on Wednesday,
December 15, 2004. To be eligible for a prize, you must be first author
on the poster, and you must be present at the meeting. You are
encouraged to submit your entry as early as possible, as space may be
limited. Further details and an explanation of judging criteria will be
provided upon acceptance of your submission.

Please send the following information to the email address below, and
attach your abstract as a Word document:

Name Affiliation
Department Phone number
Email address

Send to:

Elaine Schumacher
MMMS Materials Science Director
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539
Tel: 630-887-7100 Fax: 630-887-7417
Email: eschumacher-at-mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 10:03:51 2004

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Dear Listers,
Some time back there was a discussion about the utility of an FEG
ESEM. Specifically that the resolution under ESEM conditions was not all
that good and that one would do just as well with a tungsten filament
ESEM. Is this the prevailing opinion of FEG ESEM users? OR are there too
few instruments in service to form a consensus?
Second, in terms of viewing hydrated biological samples and beam
sensitive polymers and other materials, would one have better results with
a cryo stage on a high vac. FEG SEM ?
Respond privately or to the list.

Thanks much, Greg Erdos

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 10:06:07 2004

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Dear TEMers,
We would like to try using membrane inserts to grow cultured cells
and process them in situ for thin section TEM. What membrane materials
have any of you used successfully?

Thanks, Greg

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 10:30:02 2004

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Agfa replaced Rapidoprint paper with Brovira-Speed paper. We use Agfa
Brovira-Speed 310 Glossy, Resin Coated paper, which comes in grades 2,3,
and 4 (for contrast.) I get it from Calumet (CalumetPhoto.com).
We have a Rapidoprint processor and we use a developer made by Solutek
Corp. (Boston.617-445-5335. Go Sox!),# RA 2201 Ready-to-use Developer,
Catalog No. 536-40. Same company makes Uni-Fix Premium Fixer,
Ready-to-use, Catalog No. 519-40.
I found a vendor for these chemicals - J. P. Walker & Co Inc.,160 Oak
Street, Glastonbury, CT, 06033, 860-633-8327. I believe they get it
from a Rhode Island supplier. I realize this is not near you, but maybe
they can help you.

Julie Gross
Research Assistant
Dept. of Neuroscience
University of CT Health Center
Farmington, CT. 06030
jgross-at-neuron.uchc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 12:25:28 2004

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All,

Does anyone have the manuals for the LaB6 gun the DSM-962? Zeiss says they
don't have any back copies. I know the SEM came with the capability to use
tungsten or LaB6 and I have the right wehnalt and maybe the right
anode...just don't have the manuals. Can anybody provide copies of the
manuals, please?

Chuck Butterick
Analytical Laboratory Supervisor
Poco Graphite, Inc.
300 Old Greenwood Road
Decatur, TX 76234
(940) 393-4287 (Phone)
(940) 393-8383 (Fax)
CButterick-at-poco.com

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 13:41:02 2004

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Hi Herather
we have an Agfa Rapiline 43 (which is up for sale since we are now
mostly digital).

We never used Agfa chemicals and paper in it. We used Ilford 2000RT
developer and fixer, and Ilford multigrade RC deluxe photographic
paper.

As long as the paper and chemicals match up, I don't see any problem
about moving to a different brand. We had excellent results.
Elaine

} Date: Wed, 27 Oct 2004 20:46:05 -0700
} From: Mei Lie Wong {wong-at-msg.ucsf.edu}
} Subject: [Microscopy] Darkroom - AGFA Rapidoprint Chemicals
} To: Heather A Owen {owenha-at-csd.uwm.edu} , microscopy-at-msa.microscopy.com
} X-UBC-Scanned: Sophos PureMessage 4.6.1.107272, Antispam-Core: 4.6.1.106808,
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--
Dr. Elaine Humphrey
Director, BioImaging Facility
President, Microscopy Society of Canada
University of British Columbia
6270 University Blvd, mail-stop Botany
Vancouver, BC
CANADA, V6T 1Z4
Phone: 604-822-3354
FAX: 604-822-6089
e-mail: ech-at-interchange.ubc.ca
website: www.emlab.ubc.ca

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Greg,
I've done a LOT of samples of cell grown on polycarbonate filters.
The ones from Costar work especially well (no financial interest).
What's really neat is that if you cut the filters from their holders
at some point during dehydration and then put them into prop. oxide
after the last 100% ethanol, they roll up like a jelly roll. I
usually cut them in half or thirds so that I end up with multiple
blocks from one insert. I put them into flat embedding molds, let
them sit in the resin for an hour of so then put them in the oven.
When you trim the blocks you get a lovely spiral with many more
cells/section than you would have if you'd cut up little bits of flat
filter.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 14:05:12 2004

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Resolution in ESEM mode is close to resolution in high vacuum
mode for "good" specimens (like Au particles). The problem is
that resolution for not coated specimens is very specimen
dependant. I can get good pictures of Au particles at magnification
of x100k with FEG ESEM, but for hydrated hard tissue, as bone
or dentin, only at x20k. I did not use magnifications above x30k
for any specimens in ESEM mode, including minerals and ceramics.
Hydrated soft tissues are usually covered with a thin layer of water
which hides small details, so for them useful magnifications
are considerably lower.
As for beam sensitive specimens I think the best results could
be obtained with coating or in low voltage mode (and for low
voltage FEG is better).

Vladimir

}
} Dear Listers,
} Some time back there was a discussion about the
} utility of an FEG
} ESEM. Specifically that the resolution under ESEM conditions
} was not all
} that good and that one would do just as well with a tungsten filament
} ESEM. Is this the prevailing opinion of FEG ESEM users? OR
} are there too
} few instruments in service to form a consensus?
} Second, in terms of viewing hydrated biological
} samples and beam
} sensitive polymers and other materials, would one have better
} results with
} a cryo stage on a high vac. FEG SEM ?
} Respond privately or to the list.
}
} Thanks much, Greg Erdos
}
}
} Gregory W. Erdos Ph.D.
} Assistant Director, Biotechnology Program
} Scientific Director, Electron Microscopy
} P.O. Box 118525
} 217 Carr Hall
} University of Florida
} Gainesville, FL 32611
} gwe-at-ufl.edu
} 352-392-1295
} fax- 352-846-0251
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 14:33:21 2004

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Greg writes ...

} Dear Listers,
} Some time back there was a discussion about the utility
} of an FEG ESEM.
} Specifically that the resolution under ESEM conditions was
} not all that good and that one would do just as well with a
} tungsten filament ESEM. ...

Correct me if I am wrong, but I believe the context for
that previous consensus was not for "ESEM" (i.e., 2500 Pa),
but rather for "VP-SEM" (i.e, 250 Pa) ... and that FEG was
somewhat useful in the the VP range of pressures(?) That is,
you'll almost always find some utility in using a brighter gun
.. unless high pressure unduely contaminates the FEG source.

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 14:42:21 2004

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}
} Dear Listers,
} Some time back there was a discussion about the utility of an
} FEG
} ESEM. Specifically that the resolution under ESEM conditions was not
} all that good and that one would do just as well with a tungsten
} filament ESEM. Is this the prevailing opinion of FEG ESEM users? OR
} are there too few instruments in service to form a consensus?
} Second, in terms of viewing hydrated biological samples and
} beam
} sensitive polymers and other materials, would one have better results
} with a cryo stage on a high vac. FEG SEM ?
} Respond privately or to the list.
}

Oooooh, I hope the responses come on the list!

This is a pretty interesting topic.

Seems to me that responses should by default be on the list rather than privately,
unless there are privacy/legal issues.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 18:14:39 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (gtwang-at-sandia.gov) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, October 28, 2004 at 10:33:51
---------------------------------------------------------------------------

Email: gtwang-at-sandia.gov
Name: George Wang

Organization: Sandia National Laboratories

Title-Subject: [Microscopy] [Filtered] MListserver: Opinions on FEI Quanta 3D vs JEOL 6480LV dual beam systems

Question: Hello,
I am designing a system which will have as one of its modules a dual beam FIB/SEM with LV/VP/ESEM capability. Two possibilities are the FEI Quanta 3D and the JEOL JSM-6480LV w/Orsay Canion gun and gas injector system. Does anyone have any experience with or opinions about either of the two systems? Ideally, I would like to have the field emission rather than the tungsten filament column, but I doubt my budget would allow this. I'm concerned about the SEM resolution in the tungsten filament versions.
Thanks,
George

George T. Wang, Ph.D
Senior Member of Technical Staff
Chemical Processing Science Department 01126
Sandia National Laboratories
P.O. Box 5800 MS 0601
Albuquerque, NM 87185
ph. 505.284.9212
fax 505.844.3211
gtwang-at-sandia.gov
__________________________________________

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From MicroscopyL-request-at-ns.microscopy.com Thu Oct 28 21:58:58 2004

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Greg,
I cannot comment on a FEG ESEM since we do not have one at present. I
have worked with a W-ESEM and an SEM with cryo-stage and came to the
following conclusion based on samples I have used:

1) A great strength of ESEM is the ability to do DYNAMIC experiments. In
this case resolution is usually secondary. However, FEG should give better
resolution than W- with APPROPRIATE samples.

2) either ESEM or low-vac can be helpful for minimizing charging when
coating is not desired but this usually compromises resolution when compared
to high vac imaging.

3) Hydrated samples are difficult to work with under the best of
circumstances and ESEM has it's own challenges.

4) Cryo-SEM is the way to go for static hydrated imaging whenever possible.
You can work with fractured samples, sublimate to remove unbound water, and
work with delicate hydrated samples such as young plants with minimum
problems. Resolution is normally acceptable for these types of samples with
preservation far superior to the samples prepped for High Vac imaging.
Charging is easily handled using coating under cryo conditions.

5) Cryo permits easy imaging of heat sensitive polymers and other delicate
materials. They can be coated at low temperature if charging is a problem
and resolution is not seriously compromised over standard high vacuum
imaging.

6) Ultimately resolution depends much more on the sample than on the
capabilities of the instrument. However, there is a greater potential to
work at higher magnifications while retaining good resolution with the FEG
and resulting increased beam coherence, smaller beam diameter, good
signal:noise ratio, and ability to work at lower kV.

My opinion is to go with FEG whenever possible providing you can afford the
increased cost of the original instrument and the service contracts. An ESEM
can still benefit from FEG in high-vac mode even if there may not be a great
difference in ESEM mode. Although it might not be needed for many samples
now, it will be helpful for some. You never know about future needs and
most of us cannot justify replacing instruments on a frequent basis.

Remember that cryo can be added to any SEM so you are not limiting that
option with either ESEM or FESEM.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 10/28/04 10:13 AM, "Greg Erdos" {gwe-at-biotech.ufl.edu} wrote:

}
}
} ------------------------------------------------------------------------------
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}
} Dear Listers,
} Some time back there was a discussion about the utility of an FEG
} ESEM. Specifically that the resolution under ESEM conditions was not all
} that good and that one would do just as well with a tungsten filament
} ESEM. Is this the prevailing opinion of FEG ESEM users? OR are there too
} few instruments in service to form a consensus?
} Second, in terms of viewing hydrated biological samples and beam
} sensitive polymers and other materials, would one have better results with
} a cryo stage on a high vac. FEG SEM ?
} Respond privately or to the list.
}
} Thanks much, Greg Erdos
}
}
} Gregory W. Erdos Ph.D.
} Assistant Director, Biotechnology Program
} Scientific Director, Electron Microscopy
} P.O. Box 118525
} 217 Carr Hall
} University of Florida
} Gainesville, FL 32611
} gwe-at-ufl.edu
} 352-392-1295
} fax- 352-846-0251
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 29 01:18:14 2004

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The 9th European Congress on Stereology and Image Analysis will be coupled
with the 7th International Conference on Stereology and Image Analysis in
Materials Science STERMAT in Zakopane - Poland 2005 .

Link http://ptst.polsl.katowice.pl/9ECS/index9ECS.htm

The main topics of the meeting will be:

Applications of image analysis and stereology
Recent advances in stereology
New image analysis tools
Young stereologists competition

Special emhasize will be devoted to:

3D data acquisition, sampling and processing
Image analysis of 3D objects
Medical applications of image analysis
Image analysis and stereology in materials science
Application of image analysis in motion control, security, automation,
etc.
Trainig in stereology and image analysis

The organizers keep in mind that the leading edge is currently the interface
between technical and biomedical sciences. Our wish is to prepare a
competent
forum for exchange of ideas in the field of widely understood image analysis
and stereology.

Special courses on stereology principles and basic as well as advanced
skills in
image analysis will accompany the meeting.

Authors of the best contributions, selected by the international advisory
board,
will be invited to prepare extended versions of their papers for publication
in
Image Analysis and Stereology or Materials Characterization.

Krzysztof Hübner
Foundry Research Institute
Kraków Poland

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 29 07:36:41 2004

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===========================================================
The 9th European Congress on Stereology and Image Analysis will be coupled
with the 7th International Conference on Stereology and Image Analysis in
Materials Science STERMAT in Zakopane - Poland 2005 .

Link http://ptst.polsl.katowice.pl/9ECS/index9ECS.htm

The main topics of the meeting will be:

Applications of image analysis and stereology
Recent advances in stereology
New image analysis tools
Young stereologists competition

Special emhasize will be devoted to:

3D data acquisition, sampling and processing
Image analysis of 3D objects
Medical applications of image analysis
Image analysis and stereology in materials science
Application of image analysis in motion control, security, automation,
etc.
Trainig in stereology and image analysis

The organizers keep in mind that the leading edge is currently the interface
between technical and biomedical sciences. Our wish is to prepare a
competent
forum for exchange of ideas in the field of widely understood image analysis
and stereology.

Special courses on stereology principles and basic as well as advanced
skills in
image analysis will accompany the meeting.

Authors of the best contributions, selected by the international advisory
board,
will be invited to prepare extended versions of their papers for publication
in
Image Analysis and Stereology or Materials Characterization.

Krzysztof H¸bner
Foundry Research Institute
KrakŰw Poland

{/x-charset}

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 29 14:19:02 2004

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All,
I have two populations of liposomes which I am examining by cryo TEM. I
would like to be able to identify which liposomes are which when mixed
together. I am thinking about incorporating a marker into one population of
liposomes - this can be done when the liposomes are made.
So far my thoughts are 1) colloidal gold 2) an electron dense stain e.g.
ammonium molybdate.

Has anyone sucessfully incorporated anything into liposomes which could help
with this problem?

Many thanks as always

Chris

Christopher J. Gilpin Ph.D.
Assistant Professor
Director, Molecular and Cellular Imaging Facility
K1.246
Department of Cell Biology
University of Texas Southwestern Medical Center
5323 Harry Hines Boulevard
Dallas, Texas 75390-9039
+1 214 648 2827 Phone
+1 214 648 6408 Fax
christopher.gilpin-at-utsouthwestern.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 29 16:38:52 2004

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Hi Listers,

We have a client looking at various incarnations of carbon (nanotubes,
etc.) in the TEM and he is very curious about a phenomenon he is seeing.
This involves dark bands traveling rapidly down lengths of carbon during
viewing and is very similar to an effect I have seen commonly when
looking at crystalline structures. I bet most, if not all, TEM users
have noted something similar at some point, such as when looking at
negatively stained specimens when part of the stain has crystallized.
When the beam hits a new area, there appears to be almost a liquid flow
within the crystal which stabilizes in a few seconds.

I have never given this much thought, assuming that this is just
electron flow within the particles somehow affecting the beam to give
this visual result. Can someone describe the physics, and possibly
significance, of this?

I know I have probably described this effect very poorly, but if anyone
wants to take a stab at it, let me know and I will forward a couple
images to you showing the movement of these bands.

Thanks for any help. Our client seriously wants to understand this, and
I don't have a clue where to start researching it (except to ask you
guys!).

Happy Halloween,
Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 29 18:34:10 2004

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I would like to hear what solutions people have come up with for
imaging cells for long times while maintaining 37C and 5-10% CO2. We
have managed to get away with using CO2 Independent medium
(Invitrogen) and a Bioptechs temp controller for everything up until
now. We now have a situation where the cells die in this medium but
are happy in RPMI in a CO2 incubator. I presume that means finding a
way to maintain the CO2 on the stage. I have seen some plexiglass
boxes with controllers for outrageous $$$ which can do this. Is that
the best solution? Any suggestions for one to go on a Zeiss Axiovert
200? Thanks- Dave
--

Dr. David Knecht
Department of Molecular and Cell Biology
University of Connecticut
91 N. Eagleville Rd. U-3125
Storrs, CT 06269-3125
knecht-at-uconn.edu
860-486-2200 860-486-4331 (fax)
home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html

From MicroscopyL-request-at-ns.microscopy.com Fri Oct 29 19:38:07 2004

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I guess it is as follows:
e-beam exposure -} structure/shape change -} beam reflection shift -}
change of diffraction contrast (just like moving of bend contours)
-CNi

-----Original Message-----
} From: Tindall, Randy D. [mailto:TindallR-at-missouri.edu]
Sent: Friday, October 29, 2004 5:49 PM
To: microscopy-at-microscopy.com

Hi Listers,

We have a client looking at various incarnations of carbon (nanotubes,
etc.) in the TEM and he is very curious about a phenomenon he is seeing.
This involves dark bands traveling rapidly down lengths of carbon during
viewing and is very similar to an effect I have seen commonly when
looking at crystalline structures. I bet most, if not all, TEM users
have noted something similar at some point, such as when looking at
negatively stained specimens when part of the stain has crystallized.
When the beam hits a new area, there appears to be almost a liquid flow
within the crystal which stabilizes in a few seconds.

I have never given this much thought, assuming that this is just
electron flow within the particles somehow affecting the beam to give
this visual result. Can someone describe the physics, and possibly
significance, of this?

I know I have probably described this effect very poorly, but if anyone
wants to take a stab at it, let me know and I will forward a couple
images to you showing the movement of these bands.

Thanks for any help. Our client seriously wants to understand this, and
I don't have a clue where to start researching it (except to ask you
guys!).

Happy Halloween,
Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 07:49:18 2004

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Bioptechs and other companies (Harvard?) sell chambers for the microscope
stage that are closed on the top & bottom but allow for perfusion during
imaging. Changing the media this way would work.

However, we simply use a WPI heated stage or a completely enclosed forced
air heat box around the micrscope for 37 degrees.

For CO2, we rent tanks of premixed 95% air / 5% CO2. We take a large
petri dish and melt a hole in the side. Using thin tubing, we force the
gas through two closed tubes of water to hydrate it and then into the
small holein the side of the petri dish turned upside-down on top of the
cells, usually in MatTek dishes, on the microscope stage. Different
people in the lab have made their own personal modifications to improve
the system, such as cutting a disk in a sponge and placeing the wet sponge
around the dish of cells to improve hydration.

Sorry we don't have photos of this on the web yet.

-Michael

On Fri, 29 Oct 2004, David Knecht wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I would like to hear what solutions people have come up with for
} imaging cells for long times while maintaining 37C and 5-10% CO2. We
} have managed to get away with using CO2 Independent medium
} (Invitrogen) and a Bioptechs temp controller for everything up until
} now. We now have a situation where the cells die in this medium but
} are happy in RPMI in a CO2 incubator. I presume that means finding a
} way to maintain the CO2 on the stage. I have seen some plexiglass
} boxes with controllers for outrageous $$$ which can do this. Is that
} the best solution? Any suggestions for one to go on a Zeiss Axiovert
} 200? Thanks- Dave
} --
}
} Dr. David Knecht
} Department of Molecular and Cell Biology
} University of Connecticut
} 91 N. Eagleville Rd. U-3125
} Storrs, CT 06269-3125
} knecht-at-uconn.edu
} 860-486-2200 860-486-4331 (fax)
} home page: http://www.sp.uconn.edu/~mcbstaff/knecht/knecht.html
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 09:13:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (lieberw-at-mpip-mainz.mpg.de) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, October 29, 2004 at 11:16:39
---------------------------------------------------------------------------

Email: lieberw-at-mpip-mainz.mpg.de
Name: Ingo Lieberwirth

Organization: Max-Planck Institute for Polymer Research

Title-Subject: [Microscopy] [Filtered] MListserver: TEM data for historical microscopes covering the last 50 years

Question: Dear Listers,

i have an unusual question. I am preparing an overview on the development of TEM over the last five decades for a talk I would like to give. But i really canĄt find any data on historical TEMĄs, like resolution power, acc voltage and price.
Does any of you have an idea where I can find such data?

Thank you in advane,

Ingo

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From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 09:13:36 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (monica.iliescu-at-polymtl.ca) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, October 29, 2004 at 15:09:43
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Email: monica.iliescu-at-polymtl.ca
Name: Monica ILIESCU

Organization: Ecole Polytechnique

Title-Subject: [Microscopy] [Filtered] SC12 and SC20 Magnetic Field Cancelling Systems

Question: Hello,
We must install an ESEM Quanta FEG 200, but we have a problem with the magnetic field.
Right now we have a room that does not meet the specifications for
magnetic field before installation (we need below 3 mG and we have 6 mG
peak to peak, in the y axis, at 1 foot, 3 foot and 6 foot high). We are
currently investigating different options in order to make the room meet
these specifications. We heard about the SC12 and SC20 Magnetic Field Cancelling Systems (via web search) and we would like to know if somebody already utilised this kind of system. If yes (I hope) how sensitive is the system?
Thank you very much!
Monica

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From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 09:15:35 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (pakdeet2-at-uwm.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Friday, October 29, 2004 at 16:27:26
---------------------------------------------------------------------------

Email: pakdeet2-at-uwm.edu
Name: Choakchai Pakdeethai

Organization: University of Wisconsin-Milwaukee

Education: Graduate College

Location: Milwaukee , WI USA

Question: I wonder if epoxy/clay nanocomposites can be cut by such regular glass knives to prepare specimens for TEM observation instead of the pricey diamond knives and what is the size and dimension of specimen should it be,thank you

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 14:06:39 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Choakchai Pakdeethai wrote:
===============================================
Email: pakdeet2-at-uwm.edu Name: Choakchai Pakdeethai

Organization: University of Wisconsin-Milwaukee

Education: Graduate College

Location: Milwaukee , WI USA

Question: I wonder if epoxy/clay nanocomposites can be cut by such regular
glass knives to prepare specimens for TEM observation instead of the pricey
diamond knives and what is the size and dimension of specimen should it be,
thank you
==============================================
The clay particles will just "laugh" at the glass knife when it sees it
coming. You can't do it that way.

Now for a word about "pricey". If you ever have the opportunity to go
through a diamond knife production facility, you would probably be wondering
why they don't cost more.

But if you do want to save money, SPI Supplies as well as some of the other
suppliers of diamond knives offer "materials science" diamond knives which
are on average, about 35% lower in cost than a so-called "life science"
diamond knife. Different vendors define their "materials science" knives
differently, but in the case of SPI, the only difference is that the knife
edge has a few slight striations that would cause it to flunk as a life
science knife but for a materials science sample they are just fine. The
reason is that on the first pass with the knife on your sample, you are
putting in striations far more profound than the few that are present when
the knife is new.

Disclaimer: SPI Supplies was the first firm in the industry (1976) to offer
commercially a materials science diamond knife and we would like to see more
people using them!

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 16:49:27 2004

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Monica: I'm using as SC12 Field Canceling system right now on my JEOL
6600FXV. It's canceling my fields to below 0.15 mG. I don't have the
specs handy right now but it should be able to handle your fields. My
system was installed by Vibration Engineering Consultants
(http://www.vibeng.com/), who sell and service Spicer units in North
America. Now I'm just waiting for my active vibration canceling system
to get rid of the 15 Hz shake in my building.

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 17:12:18 2004

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} Email: pakdeet2-at-uwm.edu
} Name: Choakchai Pakdeethai
}
} Organization: University of Wisconsin-Milwaukee
} Education: Graduate College
} Location: Milwaukee , WI USA
}
} Question: I wonder if epoxy/clay nanocomposites can be cut by such
} regular glass knives to prepare specimens for TEM observation
} instead of the pricey diamond knives and what is the size and
} dimension of specimen should it be,thank you
}
} ---------------------------------------------------------------------------
Choakchai:

I agree with Chuck Garber's comments about the need for a diamond,
but the rest of your question leaves me wondering about both your
sample and your level of knowledge of microtomy. Is your sample
already embedded? If so, did you follow a protocol specific for
clay? It's easy to change its ultrastructure with the wrong prep
method. If you're a novice at microtomy, please don't try to teach
yourself; get help from an experienced microtomist in Milwaukee, or
attend Boeckeler-RMC's materials microtomy workshop in Tucson next
March.

Caroline
--
Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/

From MicroscopyL-request-at-ns.microscopy.com Sat Oct 30 20:21:56 2004

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Can anyone point me toward a good reference on insect (primarily
caterpillar) anatomy and morphology? I am particularly interested in gut
morphology.

Thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 31 16:00:15 2004

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Listers,

Here is the November 2004 Microscopy Today table of contents. This issue ships with the Call for Papers and poster for the M&M-2005 meeting.

I will close the subscription list for this issue on Friday, 5 November 2004.
Microscopists in North America and MSA members anywhere can subscribe for free. Anyone else may subscribe for US$35 per year (to PARTIALLY cover postage). All subscriptions at http://www.microscopy-today.com Thank you.

Finding the First Fires with Microscopes
Stephen W. Carmichael, Mayo Clinic

Combining Imaging and Spectroscopy: Solving Problems with Near Infrared Chemical Imaging
E. N. Lewis, E. Lee, and L. H. Kidder, Spectral Dimensions, Inc.

Automated Functions in Electron Microscopy
Bill Tivol, California Institute of Technology

Variable Magnification Electron Holography for 2â€‘D Mapping of Semiconductor Devices
Y.Y. Wang, M. Gribelyuk, A. Domenicucci, J. Bruley, J. Gaudiello, and M. Kawasaki,* IBM Microelectronic Division, *JEOL USA

A FIB Micro-Sampling Technique for Three-Dimensional Characterization of a Site-Specific Defect
T. Yaguchi1, Y. Kuroda1, M. Konno1, T. Kamino1, T. Ohnishi2, T. Hashimoto2, K. Umemura2, K. Asayama3; 1Hitachi Science Systems, 2Hitachi High-Technologies Corp., 3 Renesas Technology Corp., Japan

Color Matching to Ink Jet Printers from a Computer Screen, Part 1
Jerry Sedgewick, University of Minnesota

FIB Lift-Out and Milling of Cylindrical Specimens for Electron Tomography (or Atom Probe Field Ion Microscopy)
Lucille A. Giannuzzi, FEI Company

A New Improved Silicon Multi-Cathode Detector (SMCD) for Microanalysis and X-Ray Mapping Applications
S. Barkan*, V. D. Saveliev*, J. S. Iwanczyk*, L. Feng*, C. R. Tull*, B. E. Patt*, D. E. Newbury**, J. A. Small**, and N. J. Zaluzec;*** *Radiant Detector Technologies, **National Institute of Standards and Technology, ***Electron Microscopy Center, Argonne National Lab

Broadband CARS Microscopy
Marcus T. Cicerone and Tak W. Kee, National Institute of Standards and Technology

Microwave Processing of Drosophila Tissues for Electron Microscopy
JoAnn Buchanan, Stanford University School of Medicine

Mechanical Polishing Methods for Metal Samples for EBSD
S. Roberts*, D. Flatoff*, B. True;** *South Bay Technology, Inc., **EDAX / TSL

High Pressure Freezing User Group Meeting at M & M 2004

The Microscopy Society Of America Project MICRO
Caroline Schooley, Project MICRO Coordinator

Industry News

MSA 2005 Undergraduate Research Scholarships

NetNotes

Ron Anderson, Editor
Microscopy Today

From MicroscopyL-request-at-ns.microscopy.com Sun Oct 31 23:10:01 2004

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I would like to embed soil in place in the field to compare the
disposition of organic matter, roots, microbes, etc in the soil
among various cropping systems with as little disruption to the soil
as possible so it can be studied on both macro and micro levels.

In western Oklahoma I can find the soil when it is extremely dry of
free water nearly every summer. Of course that is a long way from
free of water but I understand there are some embedding resins that
are very tolerant of water.

Does anyone have a protocol that will work for this. I don't expect
to get very much penetration into the face of the soil. A very few
mm would be great.

Thanks

Gordon

Gordon Couger (retried)
Biosystems & Agricultural Engineering
Oklahoma State University
624 Cheyenne Ave gcc (at) couger.com
Stillwater, OK 74075
405 624 2855 cell 405 269 3588
After 3:00 PM Central Time.

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 05:43:58 2004

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Hello,
We have serious troubles with our EDAX DX4. The system does not boot
neither from HDD nor FDD. Moreover, no BIOS beep codes can be heard at the
start of the system. Please, does anybody had to solve similar problem in
the past? Any responses will be welcomed. Thanking everybody in advance.
Oldrich

-------------------------------------------------------
Oldrich Benada
Laboratory of Electron Microscopy
Institute of Microbiology, Acad. Sci. CR
Prague
Czech Republic
-------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 07:30:56 2004

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Oldrich;

Have you tried to re-install the DX4 program or the platform's operating
system? If the system is connected to the internet and users are
downloading things, I suggest removing it from any internet connection,
provided you get it back up. Also, there should be a "setup" screen that
you can get into when the system boots up. Generally you must hit a key
like "F4" or "Delete" while the system is booting to get into this. You
haven't said whether there are any other applications running on the DX4
computer. You may want to uninstall some of them if you get the system
back up.

If you have a service contract with EDAX, Inc. you should have them
either guide you or fix it themselves.

Regards,

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Oldrich Benada [mailto:benada-at-biomed.cas.cz]
Sent: Monday, November 01, 2004 6:48 AM
To: Microscopy-at-MSA.Microscopy.Com

Hello,
We have serious troubles with our EDAX DX4. The system does not boot
neither from HDD nor FDD. Moreover, no BIOS beep codes can be heard at
the
start of the system. Please, does anybody had to solve similar problem
in
the past? Any responses will be welcomed. Thanking everybody in advance.
Oldrich

-------------------------------------------------------
Oldrich Benada
Laboratory of Electron Microscopy
Institute of Microbiology, Acad. Sci. CR
Prague
Czech Republic
-------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 07:47:33 2004

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Gordon,

Gordon Vrdoljak wrote an article on preparing soil samples for light and
electron microscopy in the September 2003, vol. 11, no. 5, issue of
Microscopy Today. I'll send you a PDF in a separate email.

Ron Anderson, MT Editor
Free subscription to MT in North America at
http://www.microscopy-today.com

-----Original Message-----
} From: Gordon Couger [mailto:gcouger-at-provalue.net]
Sent: Monday, November 01, 2004 12:23 AM
To: MICROSCOPY BB

I would like to embed soil in place in the field to compare the
disposition of organic matter, roots, microbes, etc in the soil
among various cropping systems with as little disruption to the soil
as possible so it can be studied on both macro and micro levels.

In western Oklahoma I can find the soil when it is extremely dry of
free water nearly every summer. Of course that is a long way from
free of water but I understand there are some embedding resins that
are very tolerant of water.

Does anyone have a protocol that will work for this. I don't expect
to get very much penetration into the face of the soil. A very few
mm would be great.

Thanks

Gordon

Gordon Couger (retried)
Biosystems & Agricultural Engineering
Oklahoma State University
624 Cheyenne Ave gcc (at) couger.com
Stillwater, OK 74075
405 624 2855 cell 405 269 3588
After 3:00 PM Central Time.

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 08:35:07 2004

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In a message dated 11/1/04 4:35:56 AM Eastern Standard Time,
gcouger-at-provalue.net writes:
I would like to embed soil in place in the field to compare the
disposition of organic matter, roots, microbes, etc in the soil
among various cropping systems with as little disruption to the soil
as possible so it can be studied on both macro and micro levels.

In western Oklahoma I can find the soil when it is extremely dry of
free water nearly every summer. Of course that is a long way from
free of water but I understand there are some embedding resins that
are very tolerant of water.

Does anyone have a protocol that will work for this. I don't expect
to get very much penetration into the face of the soil. A very few
mm would be great.
Gordon:

You should contact Paul Berg of Boston University paulberg-at-bu.edu. He's
developed some methods for making casts and thinsections of soils at archeological
sites.

Steve Stokowski
President-elect
New England Society for Microscopy

Contact Information:
Stone Products Consultants
10 Clark St., Ste. A
Ashland, Mass. 01721-2145
508-881-6364 (ph. & fax)

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 09:10:26 2004

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Thanks for reply.
I am sorry, I did not mentioned the operation system of DX4: It is based
on DOS 6.22 and Win3.11 (wfw).

Now I know, that it is even impossible to enter the BIOS screen on our
DX4.

Oldrich

On Mon, 1 Nov 2004, Warren E Straszheim wrote:

} I have had other EDS systems but not an EDAX. Was the DX4 based on a PDP-11
} or a Windows computer? I used to consider myself quite knowledgeable about
} the PDP-11 and still have one sitting around with some spare parts. I may
} have to refresh my memory some about its procedures.
}
} Warren

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 09:46:35 2004

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Hi Debby:

A good place to start is "Introduction to the study of insects" by
Borror and DeLong. This is the classic textbook for serious students of
entomology. Your library will have a copy.

Geoff

Debby Sherman wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 11:50:21 2004

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Greetings!
An investigator in my department wishes to have me do TEM on
Haloferax volcanii. I have never worked with an organism that has a
3 M internal salt concentration. Has anyone worked with these? If
so I'd like to know what gives good results or if no good results
have been obtained, please let me know what you tried and did not
work so that I do not make the same mistake.

Thanks for your help,
Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 14:20:19 2004

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Hi
One of the best books on insect structure is: The Insects: Structure and Function, by R.F. Chapman, 4th edition, 1998, Cambridge Univ. Press. As to Ultrastructure, there is: Insect Ultrastructure, Vol. 1 (1982) and Vol. 2 (1984)By R.C. King and H. Akai, Plenum Press. Hope these will be helpful.
El-Desouky Ammar
Dept. Of Entomology,
The Ohio State University,
Wooster, OH 44691.

----- Original Message -----
} From: Debby Sherman {dsherman-at-purdue.edu}

Hello Pat,

the crucial point at the TEM processing of Haloferax (or any other
extremophil for that matter) is a very gradual desalting and pH
increase. After the initial aldehyde protein crosslinking (we use 2.5%
glut made up in the growth medium), the cells should be brought to the
neutral pH before the dehydration. The rule of thumb is that the
previous solution shouldn't be more than 10x more acidic than the
current wash (~factor of 1). A sadly good indicator of going too fast
is a dramatic pellet size decrease - as the cell membranes rupture due
to the osmotic imbalance.

Good luck,
Alice.

Alice Dohnalkova
Research Scientist
Environmental Microbiology
Pacific Northwest National Laboratory
MS P7-50
Richland, WA 99352
(509) 372-0692 office
(509) 376-3654 TEM lab

-----Original Message-----
} From: Pat Connelly [mailto:psconnel-at-sas.upenn.edu]
Sent: Monday, November 01, 2004 10:03 AM
To: Microscopy-at-MSA.Microscopy.com

Greetings!
An investigator in my department wishes to have me do TEM on Haloferax
volcanii. I have never worked with an organism that has a 3 M internal
salt concentration. Has anyone worked with these? If so I'd like to
know what gives good results or if no good results have been obtained,
please let me know what you tried and did not work so that I do not make
the same mistake.

Thanks for your help,
Pat Connelly
The University of Pennsylvania
Department of Biology
Philadelphia, PA 19104-6018
215-898-7145
psconnel-at-sas.upenn.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 1 18:32:56 2004

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For a while now I have had a Nikon Coolpix 4500 interfaced to a petrographic
microscope, leading to much user satisfaction.

However, a student just pointed out that the colors aren't quite correct. Initially I couldn't
understand why this could be, as I routinely set the color balance on the camera, using
either a piece of white paper if reflected light is to be used, or a clean glass microscope
slide for transmitted-light work.

But, of course, this student was using the microscope's built-in crossed polars, that's
why she had any colors at all.

Now if the polarising elements are exactly neutral gray I guess all will be well, but if they
aren't, then a color error could be introduced.

No problem, I thought, I'll just set the white balance with the polars in.

Duh.............. no light gets through when the (crossed) polars are in, no light to set the
white balance!

So should I just uncross the polars to set the white balance, then uncross them again
for the petrologist?

Will this be strictly OK?

Or have I, with my very slight understanding of optical microscopy, missed something
else?

Wise (or at least better-informed) counsel, please!

tia

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 02:04:23 2004

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Hi,

Doing live cell imaging for a long time while maintaining 37 degrees
Celsius and 5-10% CO2 is a bit cumbersome. However agents such as HEPES
which are used as CO2 buffers to get rid of the excess CO2, increase the
sensitivity of media to the phototoxic effects induced by exposure to
(fluorescent) light.

At my previous job, colleagues did long-time (over the weekend)
time-lapse imaging by using a plexi chamber fitted over the microscope
and a "carbogen" bottle slowly releasing its content inside the incubator.

Beware of the need to refocus the system automaticaly, as temperature
fluctuations will cause a shift of the focus level. It is better not to
cover the entire microsope, but only a small part of it around the cell
culture recipient.

References:

HEPES and other organic buffers can be used effectively with many cell
lines (see Shipman, C. (1969) Proc. Soc. Exp. Biol. Med. 130: 305).
However, be aware that the compound can be toxic, especially for some
differentiated cell types, so its effects should be evaluated before
routine use (People, C.A., et al., (1982) In Vitro 18: 755).

HEPES has also been shown to greatly increase the sensitivity of media
to the phototoxic effects induced by exposure to fluorescent light:

Zigler, J.S., et al. (1985) Analysis of the cytotoxic effects of
light-exposed HEPES-containing culture medium. In Vitro 21: 282.

Spierenberg, G.T., et al. (1984) Phototoxicity of
N-2-hydroxyethylpiperazine-N-ethanesulfonic acid-buffered culture media
for human leukemic cell lines. Cancer Research 44:2253.

It has been about 4 years since I was involved in this kind of
experiments, so my knowledge may not be up to date anymore.

Regards,

Peter Van Osta

----------------------------------------------
Peter Van Osta, MD

Director Imaging
MAIA SCIENTIFIC
Cipalstraat 3
B-2440 Geel, Belgium
Tel.: +32 (0)14 570 620
Mobile: +32 (0)497 228 725
Fax.: +32 (0)14 570 621
Email: pvosta-at-maia-scientific.com
Website: www.maia-scientific.com
A Harvard Bioscience Company
----------------------------------------------

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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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}
} I would like to hear what solutions people have come up with for imaging
} cells for long times while maintaining 37C and 5-10% CO2. We have
} managed to get away with using CO2 Independent medium (Invitrogen) and a
} Bioptechs temp controller for everything up until now. We now have a
} situation where the cells die in this medium but are happy in RPMI in a
} CO2 incubator. I presume that means finding a way to maintain the CO2
} on the stage. I have seen some plexiglass boxes with controllers for
} outrageous $$$ which can do this. Is that the best solution? Any
} suggestions for one to go on a Zeiss Axiovert 200? Thanks- Dave

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 04:38:37 2004

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Ritchie Sims writes ...

} For a while now I have had a Nikon Coolpix 4500 interfaced to a
} petrographic microscope, ...
}
} However, a student just pointed out that the colors aren't
} quite correct. ..., as I routinely set the color
} balance on the camera, using either a piece of white paper
} if reflected light is to be used, or a clean glass microscope
} slide for transmitted-light work.
}
} But, of course, this student was using the microscope's built-in
} crossed polars, ...
}
} Now if the polarising elements are exactly neutral gray I guess
} all will be well, but if they
} aren't, then a color error could be introduced.
}
} No problem, I thought, I'll just set the white balance with the polars in.
}
} Duh.............. no light gets through when the (crossed) polars
} are in, no light to set the white balance!

I remember, for a Zeiss (POL) Photomicroscope, we never had any problems
by setting the white balance to "tungsten" (i.e., using tungten film and no
filters).

How well do the 2 following settings compare: (1) setting the WB manually
with white paper, and uncrossing the polars slightly, and (2) using the
Coolpix's "tungsten" WB setting (which may be "incandescent")?

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 09:11:15 2004

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Hello,

I was recommended to ask my question to this address from German Neil of
Zeiss.

I just called my local store to order more TP 120 film for my Zeiss 109
TEM. They said the TP 120 film has been discontinued. So I called Kodak
and they said their plant is down and they are no longer going to be making
the TP 120 film. They recommended the TMAX 100 film in 120 size but said
the quality isn't as good as the TP 120. They didn't have any other
compatible film.

Does anyone have any suggestions on film or what to do as I use this film
on a weekly basis to take biopsy images for our local pathologists?

Thank you for your assistance,

Ginger

Ginger R. Hendricks
Electron Microscopy Laboratory Manager & Adjunct Instructor
OSU Center for Health Sciences
Research Department, 1111 W. 17th St., Tulsa, OK 74107
Phone: (918) 561-8232 or lab x8233; FAX: (918) 699-8629
Email: lizard-at-chs.okstate.edu
Website:
http://www.healthsciences.okstate.edu/research/rsp/electronmicroscopy/electron_microscopy_laboratory.htm

Confidentiality Statement: The information contained in this electronic
transmission is privileged and confidential and is intended only for the
use of the recipient listed above. If you are neither the intended
recipient or the employee or agent of the intended recipient responsible
for the delivery of this information, you are hereby notified that the
disclosure, copying, or use for distribution of this information is
strictly prohibited. Use of privileged or confidential material may result
in prosecution to the fullest extent of the law.

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 09:43:23 2004

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Hello,
I would like to thank to all, who so kindly respond to my request.
The all replies are on following address:

http://www2.biomed.cas.cz/~benada/DX4_troubles.html

Best regards from Prague
Oldrich

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 11:46:23 2004

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Hello Mr. Hendriks,
I would recommend using MACO TP64C. The 120 roll should be available at
around Euro 4 in Germany.
See http://www.mahn.net/PROrth.htm#TP64c
It should be nearly the same quality like Technical Pan.
Sorry but I could not find any data-sheet on the TP64C.
For more information call Mr. Schroeder at Mahn Germany, ++49-40-237008488.

Delivery for the US:
Freestyle Photographic Supplies
5124 Sunset Blvd.
CA 90027 Los Angeles
++1 323 660 3450
++1 323 6663946
info-at-freestylephoto.biz
www.freestylephoto.biz

or
U.S.A. + Canada Gary Bartoloni
1129 Old Sag Harbor Rd.
NY 11932 Bridgehampton
++1 631 7252531
Fax: ++1 631 7258045
gary-at-thelightregistry.com

Best regards,
Stefan Diller

----------------------------------------------------------------------------
-----------------------------------------
Stefan Diller - Photography
Arndtstrasse 22
D - 97072 Wuerzburg Germany
++49 - 931 - 7848700 Phone
++49 - 931 - 7848701 Fax
++49 - 175 - 717 70 51 Cell-Phone

Websites:
http://www.stefan-diller.com
http://www.assisi.de
Anfahrt: http://www.map24.de/map24/mailMap24.php?mlid=stefan.diller
----------------------------------------------------------------------------
-----------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 13:25:13 2004

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Dear Listers,
Does anyone have a manual for an Amray 1000B SEM?
Has anyone successfully upgraded an Amray 1000B to acquire images with a
computer (rather than a Polaroid)?

This model SEM has been donated to us, and I'm looking for information, so
that we may decide how to best use it.
Regards,

Yolande Berta
School of Material Science and Engineering
Georgia Institute of Technology
404-894-2545
404-894-9140 FAX

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 15:01:15 2004

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Me again.

It has been suggested to me that the Coolpix may be intrisically incapable of accurately
recording the colors seen in transmitted light from minerals between crossed polars, as
they result from interference phenomena, as opposed to the 'normal' reflected-light
colors of everyday objects for which the camera was designed.

This has a dreadful ring of plausibility to it, and I would welcome the opinions of those
more knowledgeable than I (that's quite a lot of people) as to whether it is likely to be
so; whether 'proper' microscope digital cameras might have the same problem; and
whether this means that film is still king for this application.

cheers

rtch

} From: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
Organization: Dept of Geology, Univ of Auckland
To: "Listserver" {Microscopy-at-MSA.Microscopy.Com}
Date sent: Tue, 02 Nov 2004 13:45:19 +1300

Colleagues,

Some time ago I received a flyer, which - regrettably - I discarded.
And now I would like the information.

The flyer claimed that one can perceive images in stereo if the two
images making the stereo pair are simply alternated on the screen - with
a period of about a second. Two questions:

Can anyone point me to the company involved (I could not locate them
with a simple web search)?

Can anyone tell me whether this really works?

Alwyn
--
..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 16:58:41 2004

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Rtch
I don't think so. Coolpix may have a hard time trying to interpret
what the colour temperature of such images
is, that is no big surprise, but light is light. Irrespective of the
source, red is red, green is green, etc.
The colour of light transmitted by minerals between crossed polars is
in no way qualitatively different from light of the same intensity and
spectral composition reflected from an "everyday" object, and it would
be surprising if a CCD sensor set to daylight colour balance and a
daylight colour film saw a material difference between them. Having
said that, it is possible that strong polarisation of the
image-forming light is an important issue for CCD imaging. It is
probably irrelevant for film imaging. If your CCD sensor records
different colour-shifts depending on the orientation of the sensor,
then it may be worth experimenting with the insertion of a
quarter-wave plate at 45 degrees to the analyser, or use a circular
polariziing filter as the analyser. (=same thing).

Dr. Chris Jeffree

----- Original Message -----
} From: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
To: "Listserver" {Microscopy-at-MSA.Microscopy.Com}
Sent: Tuesday, November 02, 2004 9:13 PM

Ritchie,

This is indeed a problem with digitals, and, though I'm not in the
minerals-field, a possible solution I came up with now (though I'm not
certain if correct):

Arrange the colours in Photoshop with Hue/Saturation under Image -}
Adjustments -} Hue/Saturation

Here you will change all colours in the same way at the same time by sliding
the spectrum. In other words, if something green has to be red, slide the
first bar over the second one from green to red, all other colours will
follow the same spectrum-shift. Use the spectrum for Master (not seperately
for yellow, green,...). Of course, choosing the new colour depends a lot on
your own observation & interpretation. I'm also a hobby-photographer, and
still prefer the good old negative film...

Best regards,

Sven Terclavers

************************************************
Sven Terclavers
Microscopist - Life Science Imaging
Center for Transgene Technology and Gene Therapy
Campus Gasthuisberg O&N
Herestraat 49
3000 Leuven
Belgium
Tel: +32 (0)16 34 63 71
Fax: +32 (0)16 34 59 90
Email: Sven.Terclaversemed.kuleuven.ac.be
Intranet: http://debian.med.kuleuven.ac.be
Internet: http://www.kuleuven.ac.be/mcm
Internet: http://www.vib.be
************************************************

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Tuesday, November 02, 2004 22:14
To: Listserver

Me again.

It has been suggested to me that the Coolpix may be intrisically incapable
of accurately
recording the colors seen in transmitted light from minerals between crossed
polars, as
they result from interference phenomena, as opposed to the 'normal'
reflected-light
colors of everyday objects for which the camera was designed.

This has a dreadful ring of plausibility to it, and I would welcome the
opinions of those
more knowledgeable than I (that's quite a lot of people) as to whether it is
likely to be
so; whether 'proper' microscope digital cameras might have the same problem;
and
whether this means that film is still king for this application.

cheers

rtch

} From: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
Organization: Dept of Geology, Univ of Auckland
To: "Listserver" {Microscopy-at-MSA.Microscopy.Com}
Date sent: Tue, 02 Nov 2004 13:45:19 +1300

Thanks for your thoughts.

Light is light, but green is not necessarily green, is it?

Aren't there two ways of producing every perceived color?

You can have monochromatic green light, or you can have white light with the
complement of green removed from it, ie there can be (at least) two spectral
compositions that our eyes will perceive as green, red, etc.

And so on for every perceived color.

What I was thinking was that consumer cameras, at least, are made to record the
colors of everyday objects, which are, in general, produced by the latter (subtractive)
process above. But what about the colors in a polarising microscope? Are they
monochromatic or subtractive?

Reminds me a bit of the Asian-printed leaflet that used to come in each packet of those
remarkable 'white' LEDs, which proudly proclaimed the product to produce
"monochromatic white light"!

I think you could well be right about the polarisation affecting a CCD in ways that film
wouldn't be.

cheers

rtch

} From: "Chris Jeffree" {c.jeffree-at-ed.ac.uk}
To: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
Copies to: {microscopy-at-msa.microscopy.com}

On Oct 27, 2004, at 12:24 AM, Sim Kok Swee wrote:

} does anyone know the bethe range and Kanaya Okayama range of carbon
} from
} 20kev to 30kev. Let me know.
}
Dear Sim Kok Swee,
I do have that information in a box in storage--I just moved my stuff
from my old lab in Albany, NY--and I will unpack in due course and give
you the info. Please be patient, and let me know if anyone else has
been able to respond.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 18:05:16 2004

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Alwyn,

I too would be very interested in this and I've heard about it also. I
wonder if this would work for someone who does not see stereo, i.e. a person
who uses one eye or the other but cannot fuse the two images.

Damian

-----Original Message-----
} From: Alwyn Eades [mailto:jae5-at-lehigh.edu]
Sent: Tuesday, November 02, 2004 5:02 PM
To: Microscopy-at-MSA.Microscopy.Com

Colleagues,

Some time ago I received a flyer, which - regrettably - I discarded.
And now I would like the information.

The flyer claimed that one can perceive images in stereo if the two
images making the stereo pair are simply alternated on the screen - with
a period of about a second. Two questions:

Can anyone point me to the company involved (I could not locate them
with a simple web search)?

Can anyone tell me whether this really works?

Alwyn
--
.........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 18:35:21 2004

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Alwyn: there was an article on that subject in the September 2004
"Microscopy Today". It's probably out in the archives. The authors
were Nathan and Victor Greenhut, out of Rutgers University. Victor can
be reached at flickerstereo-at-comcast.net, according to the article. I
have no clue whether it works or not, but it would be cool if it did.

Alwyn Eades wrote:

}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Colleagues,
}
} Some time ago I received a flyer, which - regrettably - I discarded.
} And now I would like the information.
}
} The flyer claimed that one can perceive images in stereo if the two
} images making the stereo pair are simply alternated on the screen -
} with a period of about a second. Two questions:
}
} Can anyone point me to the company involved (I could not locate them
} with a simple web search)?
}
} Can anyone tell me whether this really works?
}
} Alwyn

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 18:35:26 2004

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When did color film become capable of that?

John Twilley

Ritchie Sims wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Me again.
}
} It has been suggested to me that the Coolpix may be intrisically incapable of accurately
} recording the colors seen in transmitted light from minerals between crossed polars, as
} they result from interference phenomena, as opposed to the 'normal' reflected-light
} colors of everyday objects for which the camera was designed.
}
} This has a dreadful ring of plausibility to it, and I would welcome the opinions of those
} more knowledgeable than I (that's quite a lot of people) as to whether it is likely to be
} so; whether 'proper' microscope digital cameras might have the same problem; and
} whether this means that film is still king for this application.
}
} cheers
}
} rtch
}
} } From: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
} Organization: Dept of Geology, Univ of Auckland
} To: "Listserver" {Microscopy-at-MSA.Microscopy.Com}
} Date sent: Tue, 02 Nov 2004 13:45:19 +1300
} Subject: [Microscopy] White Balance
} Priority: normal
}
} }
} }
} } ----------------------------------------------------------------------
} } -------- The Microscopy ListServer -- Sponsor: The Microscopy Society
} } of America To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------
} } ---------
} }
} }
} } For a while now I have had a Nikon Coolpix 4500 interfaced to a
} } petrographic microscope, leading to much user satisfaction.
} }
} } However, a student just pointed out that the colors aren't quite
} } correct. Initially I couldn't understand why this could be, as I
} } routinely set the color balance on the camera, using either a piece of
} } white paper if reflected light is to be used, or a clean glass
} } microscope slide for transmitted-light work.
} }
} } But, of course, this student was using the microscope's built-in
} } crossed polars, that's why she had any colors at all.
} }
} } Now if the polarising elements are exactly neutral gray I guess all
} } will be well, but if they aren't, then a color error could be
} } introduced.
} }
} } No problem, I thought, I'll just set the white balance with the polars
} } in.
} }
} } Duh.............. no light gets through when the (crossed) polars are
} } in, no light to set the white balance!
} }
} } So should I just uncross the polars to set the white balance, then
} } uncross them again for the petrologist?
} }
} } Will this be strictly OK?
} }
} } Or have I, with my very slight understanding of optical microscopy,
} } missed something else?
} }
} } Wise (or at least better-informed) counsel, please!
} }
} } tia
} }
} } rtch
} }
} } --
} } Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
} } Microanalyst Fax : 64 9 3737435
} } Department of Geology email : r.sims-at-auckland.ac.nz
} } The University of Auckland
} } Private Bag 92019
} } Auckland
} } New Zealand
} }
} }

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 18:33:53 2004

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Ritchie,

I find it more effective to set the Coolpix' white balance with a neutral grey card rather than a
white surface. Accordingly, for routine transmitted light work, I use partially crossed polars to

set the white balance. For more critical transmitted light, crossed polar work does get
difficult, because the color imbalance seems to be a function of the degree to which the polars
are crossed. I would find a petro slide with minerals at first order grey or ones that are
clouded by inclusions (sercitized feldspars might do, chert, or very fine-grained gypsum with
random orientation. You might also use evenly dispersed particulates of clay or gypsum in
immersion oil), set the polarizers to their crossed position and then rack the stage away to
defocus the subject so that the field is evenly iluminated - then set the white balance.

The final difficulty may be that the CCD doesn't render the monochromatic interference colors
exactly as the eye sees them. For that there is probably no simple solution.

John Twilley

Ritchie Sims wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} For a while now I have had a Nikon Coolpix 4500 interfaced to a petrographic
} microscope, leading to much user satisfaction.
}
} However, a student just pointed out that the colors aren't quite correct. Initially I couldn't
} understand why this could be, as I routinely set the color balance on the camera, using
} either a piece of white paper if reflected light is to be used, or a clean glass microscope
} slide for transmitted-light work.
}
} But, of course, this student was using the microscope's built-in crossed polars, that's
} why she had any colors at all.
}
} Now if the polarising elements are exactly neutral gray I guess all will be well, but if they
} aren't, then a color error could be introduced.
}
} No problem, I thought, I'll just set the white balance with the polars in.
}
} Duh.............. no light gets through when the (crossed) polars are in, no light to set the
} white balance!
}
} So should I just uncross the polars to set the white balance, then uncross them again
} for the petrologist?
}
} Will this be strictly OK?
}
} Or have I, with my very slight understanding of optical microscopy, missed something
} else?
}
} Wise (or at least better-informed) counsel, please!
}
} tia
}
} rtch
}
} --
} Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
} Microanalyst Fax : 64 9 3737435
} Department of Geology email : r.sims-at-auckland.ac.nz
} The University of Auckland
} Private Bag 92019
} Auckland
} New Zealand

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 18:51:58 2004

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On Oct 29, 2004, at 2:48 PM, Tindall, Randy D. wrote:

} We have a client looking at various incarnations of carbon (nanotubes,
} etc.) in the TEM and he is very curious about a phenomenon he is
} seeing.
} This involves dark bands traveling rapidly down lengths of carbon
} during
} viewing and is very similar to an effect I have seen commonly when
} looking at crystalline structures. I bet most, if not all, TEM users
} have noted something similar at some point, such as when looking at
} negatively stained specimens when part of the stain has crystallized.
} When the beam hits a new area, there appears to be almost a liquid flow
} within the crystal which stabilizes in a few seconds.
}
} I have never given this much thought, assuming that this is just
} electron flow within the particles somehow affecting the beam to give
} this visual result. Can someone describe the physics, and possibly
} significance, of this?
}
} I know I have probably described this effect very poorly, but if anyone
} wants to take a stab at it, let me know and I will forward a couple
} images to you showing the movement of these bands.
}
} Thanks for any help. Our client seriously wants to understand this,
} and
} I don't have a clue where to start researching it (except to ask you
} guys!).
}
} Happy Halloween,
}
Dear Randy,
I guess this phenomenon can be spooky enough for Halloween.
Diffraction contrast is very dependent on alignment, so when the
lattice is oriented such that many reflections are excited--which
occurs, e.g., along a zone axis--many electrons are scattered and the
image looks dark. Alternatively, for orientations differing by only a
few degrees, few reflections are at the Bragg angle, so there is little
scattering, and the image looks light. Since the beam will heat the
crystal locally and deform it--especially if there are stresses that
have been incorporated into the crystal during its formation--the
orientation can change from one that is strongly scattering to one that
is weakly scattering and vice versa, so dark and light bands will shift
as the local orientations change, then stabilize as these orientations
cease to change. These stripes are called bend contours, and they are
discussed in many EM books. I am still in the process of unpacking my
reference material from Albany or I would be able to give you a few
titles. Without any guarantees, I guess that Electron Microscopy of
Thin Crystals, by several authors of whom Howie and Whelan are two (I
think), and Cowley's Diffraction Physics would discuss this and other
topics of interest to your client.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 19:02:48 2004

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} From: "Ritchie Sims" {r.sims-at-auckland.ac.nz}
: Me again.
:
: It has been suggested to me that the Coolpix may be intrisically
incapable of accurately
: recording the colors seen in transmitted light from minerals
between crossed polars, as
: they result from interference phenomena, as opposed to the
'normal' reflected-light
: colors of everyday objects for which the camera was designed.
:
: This has a dreadful ring of plausibility to it, and I would
welcome the opinions of those
: more knowledgeable than I (that's quite a lot of people) as to
whether it is likely to be
: so; whether 'proper' microscope digital cameras might have the
same problem; and
: whether this means that film is still king for this application.
:

No film or system renders colors exactly as the eye perceives them.
I even have some question if everyone perceives colors the same. It
is well known that some people hear color and see sounds and words
as having color. So there is a lot of room for what perception of
color is. Every part of the system that displays the color has an
effect on the color so it makes things real complicated.

But with digital images if you standardize your lighting, white
balance and lenses, objectives and filters you can apply an
adjustment to all the images as long as it is not too great and
resolve the differences.

You have the same problem with differnet emulsion of color film with
each one giving different results. Doing a 3 negatives set with
filters for yellow, cyan and magenta or red, blue and green and
black and white film are more trouble that most of use are willing
to take. And that still has problems with the chartieriscics of the
filters and inks.

I clearly remember a friend of mine trying to print the cover of a
magazine that was an oil painting and it was impossible to match the
colors with the separation process and inks available to the 4 color
process.

If you can find a fool proof system a better fool is sure to break
it.

Gordon
Gordon Couger gcc-at-couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 2 20:02:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Joan.Sempf-at-med.va.gov) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, November 2, 2004 at 12:00:32
---------------------------------------------------------------------------

Email: Joan.Sempf-at-med.va.gov
Name: Joan Sempf

Title-Subject: [Microscopy] [Filtered] MListserver:Sorvall TC-2 Tissue Sectioner

Question: To all on the Listserver:

We are interested in doing some preembedding immunogold and do not have a vibratome. We do have a Sorvall TC-2 tissue Sectioner. The problem is we have no instruction manual for it. Is it worth trying to operate this machine? Thanks for your advice in advance.

Joan

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 03:32:20 2004

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Hello,

I've been having problems with water marks being left on my micrographs once they have dried. Does anyone know of any way I can minimise this?

Thanks,
Anna Young

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 05:55:06 2004

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Dear Anna,
most of the watermarks on negatives are a problem of too fast drying of the
film or use of too less wetting agent (like PhotoFlo from Kodak) in
coherence with calcareous washing water..
Normally - if thegelatine of the film is not disturbed with too hot drying -
you can soak the film again rub it cautiously and do a new drying cycle,
best not above 100° F.

If you are talking about watermarks on the prints the problem is the same.
Use wetting agent as last bath; use a infrared dryer or use a windscreen
wiper blade to get rid of the water on both sides of the prints...

Best regards,
Stefan Diller

----------------------------------------------------------------------------
-----------------------------------------
Stefan Diller - Photography
Arndtstrasse 22
D - 97072 Wuerzburg Germany
++49 - 931 - 7848700 Phone
++49 - 931 - 7848701 Fax
++49 - 175 - 717 70 51 Cell-Phone

Websites:
http://www.stefan-diller.com
http://www.assisi.de
Anfahrt: http://www.map24.de/map24/mailMap24.php?mlid=stefan.diller
----------------------------------------------------------------------------
-----------------------------------------

----- Original Message -----
} From: "Anna Young" {Anna.Young-at-warwick.ac.uk}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, November 03, 2004 10:45 AM

Becky Holdford writes ...

} Alwyn: there was an article on that subject in the September 2004
} "Microscopy Today". It's probably out in the archives. The authors
} were Nathan and Victor Greenhut, out of Rutgers University. Victor can
} be reached at flickerstereo-at-comcast.net, according to the article. I
} have no clue whether it works or not, but it would be cool if it did.

I believe I also found a reference to a similar e-mail, but as
"flicker_stereo-at-comcast.net". I wrote both and haven't yet heard back.
Perhaps the editors of MT can clear this up(?)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

} Alwyn Eades wrote:
}
} }
} }
} }
} --------------------------------------------------------------------------
} ----
} }
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------------------
} -----
} }
} }
} } Colleagues,
} }
} } Some time ago I received a flyer, which - regrettably - I discarded.
} } And now I would like the information.
} }
} } The flyer claimed that one can perceive images in stereo if the two
} } images making the stereo pair are simply alternated on the screen -
} } with a period of about a second. Two questions:
} }
} } Can anyone point me to the company involved (I could not locate them
} } with a simple web search)?
} }
} } Can anyone tell me whether this really works?
} }
} } Alwyn
}
}
} --
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} Becky Holdford (r-holdford-at-ti.com)
} 972-995-2360
} 972-648-8743 (pager)
} SC Packaging FA Development
} Texas Instruments, Inc.
} Dallas, TX
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 06:30:25 2004

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After seeing this article, I sent an email to this address about three
weeks ago in hopes of learning more about stereo viewing. I have not yet
received a reply. Possibly a more direct mode of contact (i.e. not email)
would be more effective. If I hear something, I'll pass it on.

Kirk

Brian (Kirk) Kirkmeyer, Ph.D.
Research Scientist, Microscopy International
Flavors and Fragrances
732-335-2426 / 732-335-2350 FAX 1515 State Highway
36
brian.kirkmeyer-at-iff.com Union Beach,
NJ 07735-3542

Becky Holdford {r-holdford-at-ti.com}
11/02/2004 07:47 PM

To: Alwyn Eades {jae5-at-lehigh.edu}
cc: Microscopy-at-MSA.Microscopy.Com
Subject: [Microscopy] Re: Stereo viewing

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Alwyn: there was an article on that subject in the September 2004
"Microscopy Today". It's probably out in the archives. The authors
were Nathan and Victor Greenhut, out of Rutgers University. Victor can
be reached at flickerstereo-at-comcast.net, according to the article. I
have no clue whether it works or not, but it would be cool if it did.

Alwyn Eades wrote:

}
}
}
------------------------------------------------------------------------------

}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
-------------------------------------------------------------------------------

}
}
} Colleagues,
}
} Some time ago I received a flyer, which - regrettably - I discarded.
} And now I would like the information.
}
} The flyer claimed that one can perceive images in stereo if the two
} images making the stereo pair are simply alternated on the screen -
} with a period of about a second. Two questions:
}
} Can anyone point me to the company involved (I could not locate them
} with a simple web search)?
}
} Can anyone tell me whether this really works?
}
} Alwyn

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 06:38:46 2004

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It has been a while since I processed negatives, but...
We used to use a wetting agent called "Photoflo" in the final soak/rinse. I
believe it was a Kodak product. Have not tried, but suspect a tiny dose of
(dishwashing) liquid detergent would do the same thing. Use just enough to
cause "sheeting" rather than "beading" of the rinse water. Hang to dry.

Woody

-----Original Message-----
} From: Anna Young [mailto:Anna.Young-at-warwick.ac.uk]
Sent: Wednesday, November 03, 2004 4:45 AM
To: microscopy-at-microscopy.com

Hello,

I've been having problems with water marks being left on my micrographs once
they have dried. Does anyone know of any way I can minimise this?

Thanks,
Anna Young

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 06:54:59 2004

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Hi all,

I have here a Sony CCD-camera which is connected to a Matrox Meteor II
framegrabber card. Both in good conditions, no doubt, but is there some
software I can use for live imaging and acquisition? Analysis is a nice
extra, but is not necessary!

I tried to connect to ImageJ, but this did not work out. I need to make it
TWAIN. How does this works/is this possible?

Thanks in advance,

Sven Terclavers

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 07:07:28 2004

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Dear Anna,

The books on developing films always recommend using a
rinse agent such as 'Photoflow' to prevent drying marks.

However, in my experience very few people do and very few
have drying problems. It mainly comes down to how you wash
and your water supply. Assuming you are washing in flowing
water for 20-30 minutes with several changes of water during
that time then it is probably 'dirty water'. I assume you
have cleaned the wash tank. Is the water coming from mains
or is it from storage tanks? If the latter try mains water.
Try putting a filter on the tap to remove particulates.

If you really cannot get rid of the problem you may need to
dip the films into a bath of rinse agent before drying.

Good luck,
Ron

On Wed, 03 Nov 2004 09:45:01 +0000 Anna Young
{Anna.Young-at-warwick.ac.uk} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Hello,
}
} I've been having problems with water marks being left on my micrographs once they have dried. Does anyone know of any way I can minimise this?
}
} Thanks,
} Anna Young
}
}
}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 07:29:38 2004

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Have you tried adding Photoflo to the final rinse
solution? I believe it is made for the purpose of
precluding water marks on film. It's not expensive.
I also use it in the lab as a general wetting agent.

Stu Smalinskas
SKF
Plymouth, Michigan

~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

Anna wrote:

Hello,

I've been having problems with water marks being left
on my micrographs once they have dried. Does anyone
know of any way I can minimise this?

Thanks,
Anna Young

__________________________________
Do you Yahoo!?
Check out the new Yahoo! Front Page.
www.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 08:03:42 2004

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Alwyn,
Its called Flicker stereo. There was an articla about it the
September issue of Microscopy Today (Nathan & Victor Greenhut). YOu
can download it for free (for non-for-profit private use) from
flickerstereo-at-comcast.net.
haven't tried it myself, but it sounds fun and intriguing.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 08:04:03 2004

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Hi

I used the Agfa APX 100-120 for our old SEM. I bought last batch 3 or 4
years ago, but, with the changes on the BW photo market, I don't know if
it will be longer avaible... On the web int seems to exist, but how long ?
Good quality for SEM work, better and cheaper than the T-max. I never
compared it with TP. Before, I used the Kodak VP, but since years
discontinued !

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

On Tue, 2 Nov 2004 lizard-at-osu-com.okstate.edu wrote:

}
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} Hello,
}
} I was recommended to ask my question to this address from German Neil of
} Zeiss.
}
} I just called my local store to order more TP 120 film for my Zeiss 109
} TEM. They said the TP 120 film has been discontinued. So I called Kodak
} and they said their plant is down and they are no longer going to be making
} the TP 120 film. They recommended the TMAX 100 film in 120 size but said
} the quality isn't as good as the TP 120. They didn't have any other
} compatible film.
}
} Does anyone have any suggestions on film or what to do as I use this film
} on a weekly basis to take biopsy images for our local pathologists?
}
} Thank you for your assistance,
}
} Ginger
}
} Ginger R. Hendricks
} Electron Microscopy Laboratory Manager & Adjunct Instructor
} OSU Center for Health Sciences
} Research Department, 1111 W. 17th St., Tulsa, OK 74107
} Phone: (918) 561-8232 or lab x8233; FAX: (918) 699-8629
} Email: lizard-at-chs.okstate.edu
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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 08:14:46 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Stacey.Andringa-at-uc.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, November 3, 2004 at 07:55:04
---------------------------------------------------------------------------

Email: Stacey.Andringa-at-uc.edu
Name: Stacey Andringa

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I was given some mouse eyes in a paraformaldehyde/glutaraldehyde phosphate buffered fix. This is called this "chick fix" because it was used to fix chick embryos. I have used this for over 30 years as our standard fix. The researcher is interested in the cornea. Any suggestions about how to proceed. I would normally post-osmicate in 1% osmium tetroxide in Millonig's phosphate buffer, ethanol dehydrate, propylene oxide/Spurr infuse and embed in Spurr resin.
Will this work or not? What should have been done differently? We do not do paraffin embedding in our lab. Would that have been better? I am not sure if the researcher wants TEM.
Thanks for any help.

Stacey Andringa

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 08:34:12 2004

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Anna

I assume that you are washing your film in tap water and then drying. You need to give your film a final rinse with a few drops of detergent to act as a wetting agent. You can use ordinary washing liquid but given the cost of film and time it's probably better just to stick with a commercial film wetting agent such as Kodak Photoflo or Ilford Ilfotol (if it's still available). I generally make up a tank of distilled water (rather than tap water) with a few drops of wetting agent for each film. Agar Scientific or any decent photographic shop should supply a range of wetting agents.

It's also possible to use special squeegee tongs to remove most of the water from film (especially 35mm) and further reduce drying marks but if any grit ever gets onto the rubber pads it would cause more damage than drying marks.

If you have old drying marks it may be possible to remove them from film provided that they aren't on the emulsion side. A nice long soak in distilled water and wetting agent can help, although I'm sure other microscopists may have some magic techniques of their own.

Good luck

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
tel no: 0191 515 2872 / 3468
e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Anna Young {Anna.Young-at-warwick.ac.uk}

Anna,

Wetting agent(usually about a 1 to 2% solution), and proper constant clean
water flow in rinse tank and sufficient duration of rinse are all going to
prevent marks (from water and residual processing chemicals left on
photos). You could also add to that........use of special squeegee tongs.
These are just tongs with soft, inward facing wiper blade areas, which you
pull down along the film surface to remove any excess water.

Sheet film/photos should be hung from one corner of the film to prevent
drying streaks.

One other comment. When using wetting agent such as PhotoFlo (or
whatever).........you should probably NOT use hard water because it may
still leave drying marks. Use distilled water, or bottled
water.........or any other source of SOFT water is preferred.

Kelly A. Ramos
Metallurgical Engineer / Supervisor
Argo-Tech Materials Laboratories
23555 Euclid Avenue
Cleveland, OH 44117
216-692-5904 or 216-692-5446
(fax) 216-692-5816
http://www.atclabs.com

-----Original Message-----
} From: Anna Young [mailto:Anna.Young-at-warwick.ac.uk]
Sent: Wednesday, November 03, 2004 4:45 AM
To: microscopy-at-microscopy.com

---

Hello,

I've been having problems with water marks being left on my micrographs
once
they have dried. Does anyone know of any way I can minimise this?

Thanks,
Anna Young

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:00:46 2004

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The final rinse of your film should be in distilled water for a few
minutes, followed by a distilled water rinse containing Kodak's
"photo-flo" wetting agent or a similar product. If the water marks are
on prints, a final rinse in distilled water should solve the problem
(assuming of course that the negatives are not water-marked).

Geoff

Anna Young wrote:

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--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:03:58 2004

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Hello Alwyn,

it is indeed possible to get a 3D-effect from alternating between two stereo
images. The frequency of 1 Hz or so seems to be right. We use that in our
software, but it is only for getting a 3D impression. As you are changing
between two images, it is very hard to make any measurements or get
quantitative results. For that anaglyphic (red-green or red-blue) images are
better or a full stereo reconstruction.

The images have to be aligned so that they tilt around a common pivot point,
otherwise you will get lateral movement as well, which can destroy the 3D
impression.

I just tried it with one eye closed. I did get a 3D impression. So this
would also probably work for people who cannot fuse stereo images.

Alwyn, let me know if you want to try this. I can send you our software as a
demo and you can see for yourself if it works for you. Please contact me
offline to set this up.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Alwyn Eades [mailto:jae5-at-lehigh.edu]
Sent: Tuesday, November 02, 2004 16:02
To: Microscopy-at-MSA.Microscopy.Com

Colleagues,

Some time ago I received a flyer, which - regrettably - I discarded.
And now I would like the information.

The flyer claimed that one can perceive images in stereo if the two
images making the stereo pair are simply alternated on the screen - with
a period of about a second. Two questions:

Can anyone point me to the company involved (I could not locate them
with a simple web search)?

Can anyone tell me whether this really works?

Alwyn
--
.........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:10:37 2004

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Look into StreamPix - http://www.norpix.com/streampix.htm

if they have a driver for your capture board it should work ..

Bill Miller

At 08:10 AM 11/3/2004, Sven Terclavers wrote:

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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:09:51 2004

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Alwyn,
Our old Kevex Delta 8000 x-ray/imaging system did this. Basically, you
would aquire two images at different tilts and put them in two different
pages, then alternate between the two pages. The system would then page
between the images and you could adjust the speed between alternations.
The only caveate is that you need to get the right speed for your
viewing, too fast or too slow and the stereo effect is lost. It wasn't
bad at the "right" paging speed although this speed could be a little
different for different people.

Greg

--
--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:21:20 2004

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Anna,
We use Kodak Photo-flo just before hanging the negative to dry. It is a
wetting agent that helps to prevent water spots during drying.
Alternatively, you can do a final wash in distilled or RO water before
hanging the negs to dry.
Greg

Anna Young wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
==================================================================
Greg Strout
Electron Microscopist, University of Oklahoma
WWW Virtual Library for Microscopy:
http://www.ou.edu/research/electron/www-vl/
e-mail: gstrout-at-ou.edu
Opinions expressed herein are mine and not necessarily those of
the University of Oklahoma
==================================================================

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:26:41 2004

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Dr. Greenhut is at Rutgers greenhut-at-alumina.rutgers.edu

At 10:12 PM 11/2/2004, Brian.Kirkmeyer-at-iff.com wrote:

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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:46:29 2004

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Anna, and others who have responded,

I gave up on Photoflo and other drying aids a long time ago. Seems like no
matter what you do, they all leave water beading up somewhehere on the film
and all those dissolved minerals in the water leave drying marks. Plus,
stuff starts to grow in a stored working solution after awhile, so if you
still want to use Photoflo, mix it fresh from the concentrate every time you
use it.

So after my final water wash of film, I drain excess water off for 15
seconds, then I use a DISTILLED water rinse (not deionized) and get clear
negs everytime with no water marks at all. I keep a plastic tray with cover
filled deep enough with distilled water so that the TEM negs in rack will be
submerged. Just dip in an out a few times and then dry as usual. I change
the distilled water in the tray periodically, depending on number of negs
processed, as some tap water remains in there as a result of rinsing, tho of
course its much diluted compared to tap water.

Gib
--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra

} Hello,
}
} I've been having problems with water marks being left on my micrographs once
} they have dried. Does anyone know of any way I can minimise this?
}
} Thanks,
} Anna Young

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:46:00 2004

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Hello Sven,

Frame grabbers are like most cards you put into a computer, they need
drivers. Most imaging acquisition packages support frame grabber cards, but
not all packages support all cards. So you need to find a program that
supports your card. The Meteor II was or is sold in different flavors. Our
software, analySIS, does support some of the flavors. Let me know exactly
what card you have and I can tell you if we support it.

There is, however, a "general" driver that is supported by many software
packages. It's called "TWAIN" ("Thing without an interesting name"). If your
card comes with a TWAIN driver and the software has a TWAIN interface, you
can use that to communicate with the card. Apparently ImageJ has a TWAIN
interface. You should go to the Matrox web site (www.matrox.com) and find
out if they have a TWAIN driver for the card.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Sven Terclavers [mailto:Sven.Terclavers-at-med.kuleuven.ac.be]
Sent: Wednesday, November 03, 2004 06:10
To: Microscopy

Hi all,

I have here a Sony CCD-camera which is connected to a Matrox Meteor II
framegrabber card. Both in good conditions, no doubt, but is there some
software I can use for live imaging and acquisition? Analysis is a nice
extra, but is not necessary!

I tried to connect to ImageJ, but this did not work out. I need to make it
TWAIN. How does this works/is this possible?

Thanks in advance,

Sven Terclavers

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 09:52:26 2004

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The Microscopy Today article is:
Greenhut and Greenhut Flicker Stereo: Digital 3D Viewing for PC & Presentation
The article isn't available on line yet, but I've got the issue at
home and could send a photocopy if needed. I think Ron can provide a
pdf file. HIs email is: microscopytoday-at-tampabay.rr.com

Phil

} Becky Holdford writes ...
}
} } Alwyn: there was an article on that subject in the September 2004
} } "Microscopy Today". It's probably out in the archives. The authors
} } were Nathan and Victor Greenhut, out of Rutgers University. Victor can
} } be reached at flickerstereo-at-comcast.net, according to the article. I
} } have no clue whether it works or not, but it would be cool if it did.
}
} I believe I also found a reference to a similar e-mail, but as
} "flicker_stereo-at-comcast.net". I wrote both and haven't yet heard back.
} Perhaps the editors of MT can clear this up(?)
}
} cheerios ... shAf :o)
} Avalon Peninsula, Newfoundland
} {www.micro-investigations.com}
}
}
}
} } Alwyn Eades wrote:
} }
} } }
} } }
} } }
} } --------------------------------------------------------------------------
} } ----
} } }
} } } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } } To Subscribe/Unsubscribe --
} } } http://www.msa.microscopy.com/MicroscopyListserver
} } } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } }
} } --------------------------------------------------------------------------
} } -----
} } }
} } }
} } } Colleagues,
} } }
} } } Some time ago I received a flyer, which - regrettably - I discarded.
} } } And now I would like the information.
} } }
} } } The flyer claimed that one can perceive images in stereo if the two
} } } images making the stereo pair are simply alternated on the screen -
} } } with a period of about a second. Two questions:
} } }
} } } Can anyone point me to the company involved (I could not locate them
} } } with a simple web search)?
} } }
} } } Can anyone tell me whether this really works?
} } }
} } } Alwyn
} }
} }
} } --
} } ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} } Becky Holdford (r-holdford-at-ti.com)
} } 972-995-2360
} } 972-648-8743 (pager)
} } SC Packaging FA Development
} } Texas Instruments, Inc.
} } Dallas, TX
} } ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} }
} }
} }

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 10:12:25 2004

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Sven:

The Matrox board should have come with the MIL or MIL-lite software.
Both of which allow for live imaging and basic image capture. If it did not you
need to contact the sales person or Matrox and get a copy.

}
} Hi all,
}
} I have here a Sony CCD-camera which is connected to a Matrox Meteor II
} framegrabber card. Both in good conditions, no doubt, but is there some
} software I can use for live imaging and acquisition? Analysis is a nice
} extra, but is not necessary!
}
} I tried to connect to ImageJ, but this did not work out. I need to make it
} TWAIN. How does this works/is this possible?
}
} Thanks in advance,
}
} Sven Terclavers
}
}

Richard E. Edelmann, Ph.D.
Electron Microscopy Facility Director
350 Pearson Hall
Miami University, Oxford, OH 45056
Ph: 513.529.5712 Fax: 513.529.4243
E-mail: edelmare-at-muohio.edu
http://www.emf.muohio.edu

"RAM disk is NOT an installation procedure."

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 10:09:58 2004

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I've read the replies on this topic. I assume that you are using some kind of rack that holds your negative in a vertical position. I agree with the use of photoflo. However, make sure that you don't use too much of it and don't stir it so that it froths when you put it in. I almost cut the recommend amount in half. Wait a little time for it to mix with the water. Too much photoflo will also put marks on the negatives. Pour out the water in the washing tank and let it dry in between use. You should also use a filter on your wash water, especially if you mix it with warm water to keep the temperature constant. Check and change the filters.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

Anna wrote:

Hello,

I've been having problems with water marks being left
on my micrographs once they have dried. Does anyone
know of any way I can minimise this?

Thanks,
Anna Young

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 12:25:07 2004

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Hi Stacey,
I have done a fair amount of rat eye preps and have found that
Epon-Araldite i a medium to soft composition works well with eyes,
especially if you'll be cutting for LM. You also need to draw out
the infiltration: 2:1 PO to resin , then 1:1 then 1:2. do each step
overnight (8 hours) on a rotator then 24 hours in a two changes of
resin without accelerator, then one change with accelerator. Its
long, but it works. Its a method given to me by someone who works
with nothing but eyes.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 12:48:22 2004

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There's the pricy glasses-free stereo LCD monitor from Stereographics (www.stereographics.com/), or the much less expensive Crystal Eyes system (uses shuttered glasses to view alternated images) from the same company. Viewing alternated images with both eyes isn't stereo in the sense of binocular depth perception, but could give the sense of depth perception available to one-eyed observers. Alternating multiple images in a suitably aligned tilt series of photos, or just riffling through a stack of these images might be better. Readers intrigued by stereo vision might check out "Foundations of Cyclopean Perception" (U. of Chicago Press, 1971) by B. Julesz.

I often view side-by-side displayed stereo images by putting a simple plastic of glass wedge in front of one eye to overlap images in the visual field. The wedges are easy to make and avoid the eye muscle work that unaided viewing requires.

Larry Thomas
Pacific Northwest National Laboratory
P.O. Box 999
Mail Stop P8-16
Richland, WA, USA

email: Larry.Thomas-at-pnl.gov
phone: (509) 372-0793
fax; (509) 376-6308

} ----------
} From: Leona Cohen-Gould
} Sent: Wednesday, November 3, 2004 6:15 AM
} To: Alwyn Eades; Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] Re: Stereo viewing
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
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} -------------------------------------------------------------------------------
}
}
} Alwyn,
} Its called Flicker stereo. There was an articla about it the
} September issue of Microscopy Today (Nathan & Victor Greenhut). YOu
} can download it for free (for non-for-profit private use) from
} flickerstereo-at-comcast.net.
} haven't tried it myself, but it sounds fun and intriguing.
} Lee
} --
} Leona Cohen-Gould, M.S.
} Sr. Staff Associate
} Director, Electron Microscopy Core Facility
} Manager, Optical Microscopy Core Facility
} Joan & Sanford I. Weill Medical College
} of Cornell University
} voice (212)746-6146
} fax (212)746-8175
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 13:15:42 2004

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You probably saw the "Flicker Stereo" article in the September Microscopy
Today. By the Greenhuts on pg 46.

Ron Anderson

-----Original Message-----
} From: Alwyn Eades [mailto:jae5-at-lehigh.edu]
Sent: Tuesday, November 02, 2004 6:02 PM
To: Microscopy-at-MSA.Microscopy.Com

Colleagues,

Some time ago I received a flyer, which - regrettably - I discarded.
And now I would like the information.

The flyer claimed that one can perceive images in stereo if the two
images making the stereo pair are simply alternated on the screen - with
a period of about a second. Two questions:

Can anyone point me to the company involved (I could not locate them
with a simple web search)?

Can anyone tell me whether this really works?

Alwyn
--
.........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 13:25:48 2004

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Hi Mike

This seems to, to me, quite incredible.

Isn't the basis of 3D perception that different images are seen by each eye?

Do you have any idea how you could have gotten a 3D perception with one eye closed?

cheers

rtch

} From: Mike Bode {mb-at-soft-imaging.com}
To: Microscopy-at-MSA.Microscopy.Com
Copies to: "'Alwyn Eades'" {jae5-at-lehigh.edu}

Relative motion is quite useful for generating stereoscopic perception
from your images. I've done this with view pairs, as well as with
multiple views or movies generated from 3D data. As mentioned, playback
or flicker rate can be adjusted to provide the best perception. The
viewing angle between the two (or more) views is also important. I've
found success with about 4 to 8 degrees, depending on the sample. Both
angle and speed for best perception vary from person to person.

What is happening is that you perceive motion cues on portions of your
object, translating those into depth based on that relative motion. I
personally get a better depth perception from motion than I do from
stereo fusion (as with the colored glasses); of course, everyones
mileage will vary.

I seem to recall that ~10% of the population uses primarily motion cues
for depth perception, and find stereo fusion of static images rather
difficult. Motion cueing is very useful for these folks, and doesn't
require glasses or a special monitor.

-- Kevin Ryan

kevin-at-mediacy.com
Media Cybernetics, Inc.
Image-Pro
www.mediacy.com

} From: Leona Cohen-Gould
} Sent: Wednesday, November 3, 2004 6:15 AM
} To: Alwyn Eades; Microscopy-at-MSA.Microscopy.Com
} Subject: [Microscopy] Re: Stereo viewing
}
}
} Alwyn,
} Its called Flicker stereo. There was an articla about it the
} September issue of Microscopy Today (Nathan & Victor Greenhut). YOu
} can download it for free (for non-for-profit private use) from
} flickerstereo-at-comcast.net.
} haven't tried it myself, but it sounds fun and intriguing.
} Lee
} --
} Leona Cohen-Gould, M.S.
} Sr. Staff Associate
} Director, Electron Microscopy Core Facility
} Manager, Optical Microscopy Core Facility
} Joan & Sanford I. Weill Medical College
} of Cornell University
} voice (212)746-6146
} fax (212)746-8175

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There is another effect that produces the perception of depth even when
viewed with only one eye. Check out the "rotoreliefs" at
http://www.aqualoop.com/aqua_sound/delia/Duchamp.html.
--
Lew Rabenberg
University of Texas at Austin

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 15:33:11 2004

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On Nov 3, 2004, at 1:45 AM, Anna Young wrote:

} I've been having problems with water marks being left on my
} micrographs once they have dried. Does anyone know of any way I can
} minimise this?
}
Dear Anna,
Have you made up fresh photoflo recently? I had best results by
air-drying overnight at room temp, rather than using a hot air drier.
You could also have problems if your rinse water contains something
that does not wash off during the dip in photoflo, such as high mineral
content. In that case, use the house distilled water to rinse the
negs.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

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On Nov 3, 2004, at 4:45 AM, White, Woody N. wrote:

} Have not tried, but suspect a tiny dose of
} (dishwashing) liquid detergent would do the same thing.

Dear Woody,
Photoflo is a polyethylene glycol, which does not damage the gel and
is clear. I would be concerned that the detergent might detach the gel
from the plastic backing--especially since that's what happens when you
wash dishes.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

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kineopsis - see http://www.hirox-usa.com for many examples

Bill Miller

At 02:37 PM 11/3/2004, Ritchie Sims wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

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I've seen/used the alternating image method very effectively on a
system where you wear 'goggles' with LCD eye-pieces. Left and right
eye-pieces are alternately blanked, synchronised with the images on
the screen. The visualisation software included an 'overlay' which
allowed measurements to be taken. Not sure if this is the same sort
of system that Mike Bode is describing - I seem to remember the
frequency was a lot higher, 25 Hz? I don't recall the details of the
software/hardware but the SPM group in Pharmaceutical Sciences at
Nottingham University, UK use the system extensively.

Stereo vision does require two eyes so that each eye 'sees' the same
field from slightly different angles. In viewing stereo pair images,
traditional stereo viewers just ensure each eye is separately
presented with an image that has already be obtained from different
viewpoints - the brain then parallel processes and puts then together
so that you seem to be seeing a single image, rather than two
different images. I guess the brain can manage a similar trick if the
same date is presented in serial.

The interesting question is whether you could get stereo perception
through one eye if your brain had never learnt to process stereo i.e.
if you were born with vision in only in one eye?
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

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Hi Anna,

This may have been addressed in the other responses but...there are two type of water spots. 1. is
mineral or soap residue and can be washed off. 2. Is permanent due to the water molecules lining up
around the edge of the droplet of water creating a charge that causes the silver to migrate through the
emulsion and form a ring of extra density where the edge of the droplet was. So use a small amoant of
Photoflo diluted in distilled water, agitate the film in this solution for 30 sec. and hang to dry.

Bob

On Wed, 3 Nov 2004, Anna Young wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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} -------------------------------------------------------------------------------
}
} Hello,
}
} I've been having problems with water marks being left on my micrographs once they have dried.
Does anyone know of any way I can minimise this?
}
} Thanks,
} Anna Young
}
}
}
}

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{snip}

} Stereo vision does require two eyes so that each eye 'sees' the same
} field from slightly different angles. In viewing stereo pair images,
} traditional stereo viewers just ensure each eye is separately
} presented with an image that has already be obtained from different
} viewpoints - the brain then parallel processes and puts then together
} so that you seem to be seeing a single image, rather than two
} different images. I guess the brain can manage a similar trick if the
} same date is presented in serial.
}
} The interesting question is whether you could get stereo perception
} through one eye if your brain had never learnt to process stereo i.e.
} if you were born with vision in only in one eye?

3D information is also gained from visual clues as shading (the brain is
assuming light comes from above) and movement (switching between two
pictures).
Stereo perception is only the brains capability to create a 3D model of
the world. Movement and shading is at work at a deep level in the brain,
if there is only one eye working we still process theese clues. So I
believe that a one eyed person would have stereo perception of the world
around him.

There were an interesting story in Scientific American about ten years
ago on this subject.
/Göran

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Hello Ritchie,

Of course you can't have binocular vision with only one eye. The normal
depth perception is based on stereo vision. However, in this case we add
movement to the equation. Let's say that you have an object sticking out at
you. When you start tilting the image, the top (the part that is closest to
you) moves with a larger amplitude than parts that are further away.
Apparently our brain is clever enough to interpret this as a change in a
parallax and fills in the missing information.

I am not saying that this is quantitative in any way, but it works.

You can test it for yourself. Close one eye and look at an object. You'll
find that the object appears flat - no 3D information. Now move your head to
the left and right (still one eye closed). You'll immediately see that you
get an impression of the 3-dimensionality of the object from the changes.

I have no problem fusing stereo images. I don't know what happens to people
with neurological problems that can't fuse stereo images. Whether they can
use the oscillation method remains to be seen.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: Ritchie Sims [mailto:r.sims-at-auckland.ac.nz]
Sent: Wednesday, November 03, 2004 12:37
To: Mike Bode; Microscopy-at-MSA.Microscopy.Com

Check out the review of a Sharp monitor in the recent issue of PC
Magazine:
http://www.pcmag.com/article2/0,1759,1647635,00.asp

John Mardinly
Intel

-----Original Message-----
} From: Leona Cohen-Gould [mailto:lcgould-at-med.cornell.edu]
Sent: Wednesday, November 03, 2004 6:16 AM
To: Alwyn Eades; Microscopy-at-MSA.Microscopy.Com

Alwyn,
Its called Flicker stereo. There was an articla about it the
September issue of Microscopy Today (Nathan & Victor Greenhut). YOu
can download it for free (for non-for-profit private use) from
flickerstereo-at-comcast.net.
haven't tried it myself, but it sounds fun and intriguing.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

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Is the concept of paralax lost on everyone.
what do you think causes the depth of field?
so a one eyed person, no matter what the software and
not see in depth.
john

__________________________________
Do you Yahoo!?
Check out the new Yahoo! Front Page.
www.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 3 20:20:49 2004

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I'm going to jump in here and add my two cents worth. I was born with
strabismus or crossed eyes and as such, as was explained to me, the neural
pathways could not develop so that the two images could be fused in the
brain to form a 3-D view. Although my eyes were straightened at 2, it was
too late for the stereopsis to develop. Consequently I see or I should say
I focus with one eye or the other but not both simultaneously. I can switch
back and forth between the two eyes and see the parallax or shift in the
position of two objects with respect to one another but don't see 3-D. In
this I am not like someone who has only one eye. Another consequence of
this brain damage :-) is that I have learned to compensate using visual cues
to place objects but that requires a multitude of variables including
lighting, shadows, my position and orientation, and probably others that I
don't know about. There are some situations where I am totally unable to
determine positions. That is why I spend a number of years working at a
1MeV TEM lab where stereo was a capability due to the thick sections used
and specimen rotation then I went on to confocal (among other things). At
least I could get the perception of depth using a rotation software package.
I do recall once visiting a ophthalmologist quite a number of years ago who
used a prism system that gave me the impression of 3-D and it was a very
strange sensation.

Damian Neuberger, PhD

Hello Ritchie,

Of course you can't have binocular vision with only one eye. The normal
depth perception is based on stereo vision. However, in this case we add
movement to the equation. Let's say that you have an object sticking out at
you. When you start tilting the image, the top (the part that is closest to
you) moves with a larger amplitude than parts that are further away.
Apparently our brain is clever enough to interpret this as a change in a
parallax and fills in the missing information.

I am not saying that this is quantitative in any way, but it works.

You can test it for yourself. Close one eye and look at an object. You'll
find that the object appears flat - no 3D information. Now move your head to
the left and right (still one eye closed). You'll immediately see that you
get an impression of the 3-dimensionality of the object from the changes.

I have no problem fusing stereo images. I don't know what happens to people
with neurological problems that can't fuse stereo images. Whether they can
use the oscillation method remains to be seen.

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

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I haven't done any developing in long time but re-washing the
negatives won't hurt them and may solve the problem it won't make it
worse.

Test any rubbing on an unimportant area of the negative first. Some
emulsions will take a lot more abuse than others. Kodak T-Max is
really tough compared to Agfa Pan. I accidentally washed some T-Max
in 140 f. water and plunge in 70 f. water with no detectable damage.
I think it is designed to be deviled at 100 f. along with color
film. Don't try that with anything else.

As a final wash I used distilled water or deionized water with a
very little bit of photo flow for 1 or two minutes when I lived in a
hard water area. Make sure there are no drops of water left on the
negative and hang it in a dust free environment to dry at normal
temperature. If you are doing a lot of negatives a cabinet with a
HEPA filter is a very good investment. Getting the water off the
film can be done with your fingers, a chamois, sponge, pair of
windshield wipers or any number of ways but they all run some risk
of scratching the negative. With Distilled water and the right
amount of photo flo the water should run off without the need of any
help. But don't leave any drops of water on the film to dry or you
are very likely to find deposits of stuff in the edges of the drops.

I often used very rapid drying methods that include a substitute sea
water to rapidly remove the fixer followed by a 30 second rinse in
water into to similar rinse in alcohol with a bit of photo flow then
forced drying with hot air. before printing then a proper wash the
next day. Having to make a dead line on a newspaper could be
difficult. But I could print a picture in less than 15 minutes of
taking it every time, 10 minutes if I used a press camera and the
negatives are still good 30 years later.

Gordon
Gordon Couger gcc at couger.com

I collect links on information related to light microscopes.
http://www.couger.com/microscope/links/gclinks.html
Please forward any links or information you think might be useful to
others.
Microscope Manual at www.science-info.org

} From: "Ron Doole" {ron.doole-at-materials.oxford.ac.uk}

:
: Dear Anna,
:
: The books on developing films always recommend using a
: rinse agent such as 'Photoflow' to prevent drying marks.
:
: However, in my experience very few people do and very few
: have drying problems. It mainly comes down to how you wash
: and your water supply. Assuming you are washing in flowing
: water for 20-30 minutes with several changes of water during
: that time then it is probably 'dirty water'. I assume you
: have cleaned the wash tank. Is the water coming from mains
: or is it from storage tanks? If the latter try mains water.
: Try putting a filter on the tap to remove particulates.
:
: If you really cannot get rid of the problem you may need to
: dip the films into a bath of rinse agent before drying.
:
: Good luck,
: Ron
:
:
: On Wed, 03 Nov 2004 09:45:01 +0000 Anna Young
: {Anna.Young-at-warwick.ac.uk} wrote:
:
: }
: }
:
} ------------------------------------------------------------------
------------
: } The Microscopy ListServer -- Sponsor: The Microscopy Society of
America
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: }
: } Hello,
: }
: } I've been having problems with water marks being left on my
micrographs once they have dried. Does anyone know of any way I can
minimise this?
: }
: } Thanks,
: } Anna Young
: }
: }
: }
: }
:
: ----------------------
: Mr. R.C. Doole
: Department of Materials,
: University of Oxford.
: Parks Road, Oxford. OX1 3PH. UK.
: Phone +44 (0) 1865 273701
: Fax +44 (0) 1865 283333
: ron.doole-at-materials.ox.ac.uk
: http://www-em.materials.ox.ac.uk/
: *********************************
:
:
:
:

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Metropolitan Microscopy Society Fall Meeting 2004
=====================================================

The thread seems long enough already. Maybe I can help summarize.

At 01:37 PM 11/03/04, Ritchie Sims wrote:

} This seems to, to me, quite incredible.
} Isn't the basis of 3D perception that different images are seen by each eye?
} Do you have any idea how you could have gotten a 3D perception with one
} eye closed?
} cheers

Depth perception can sometimes be attained with a single view. Shading cues
can help determine relative position. However, that does require many
assumptions and it is not foolproof. Some may remember some planetary
images that were referenced in this forum some months ago. It was unclear
whether features were bumps or depressions. It depended on the
interpretation and relied on knowledge of the lighting.

Depth perception is usually done via "stereo" imaging. Much of this
discussion has equated stereo with binocular vision. That is not strictly
necessary. _What IS needed are two (or more) images for the brain to
process._ In binocular vision, those images are provided simultaneously
through two different channels. However, the same effect can be achieved
through sequential viewing. That can be done via flicker stereo or by
(closing one eye and) moving one's head back and forth, or by taking
sequential EM images.

Mike Bode had said:
} Of course you can't have binocular vision with only one eye. The normal
} depth perception is based on stereo vision. However, in this case we add
} movement to the equation. Let's say that you have an object sticking out at
} you. When you start tilting the image, the top (the part that is closest to
} you) moves with a larger amplitude than parts that are further away.
} Apparently our brain is clever enough to interpret this as a change in a
} parallax and fills in the missing information.
}
} I am not saying that this is quantitative in any way, but it works.

I don't know why Mike thought that disclaimer necessary. I understand that
stereo depth perception can always be quantitative even though it is often
left as qualitative. Our brains normally learn the spatial relationships
(i.e., trigonometry) that allow us to extend our hand some distance to
grasp an object. (Granted, we often update our estimates via continuous
monitoring of the progress.) Even though it seems "intuitive" to our human
systems, with appropriate measurements, any two images taken at known
angles should be able to lead to quantitative measurements of relative
distance or height. If there is a restriction besides incomplete
information (i.e., unknown angles) that limits it to qualitative
perception, I am not aware of it.

Meanwhile, I have found the various approaches to sensing or achieving the
stereo effect to be interesting.

Warren Straszheim
involved in qualitative and quantitative stereo image for many years

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I'm reviewing marketing literature for SEMs and I can't seem to find Hitachi
or Amray. Did I miss something? Did they get absorbed into another
company, get out of the SEM business, or am I just using a bad search
engine?

Thanks for any help,

Diane Ciaburri

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A few additional notes may be helpful.

Certainly it is possible to apply simple trigonometry to determine the
absolute distances of features using a pair of images taken with a known view angle
or spacing between them. But while that is how stereoscopic measurements are
made, it isn't how humans use two-eye views. That process functions by rotating
the eyes in their sockets so that the same feature is brought to the fovea
(the high resolution center of the retina where the highest density of cones
resides). As the center of attention is shifted from one feature in a scene to
another, the rotation of the eyes in their sockets - in or out - provides a
relative signal as to which feature is closer. Only by sequentially treating a
number of points in the scene and building up a mental list of relative distance
order does our brain construct an overall sense of relative depth. And it is
definitely relative, not absolute. We have no transits or even protractors in
our eye sockets, and there is no evidence that anything in human vision is
quantitative as opposed to relative (comparisons). Indeed, in terms of reaching a
finger out to touch something, or judging the approach of an object, there is
evidence that other cues such as relative size, shadows and precedence (if one
object blocks another, it is closer) are more important than stereo vision.

The use of "sequential stereo" by moving the eye point back and forth - or
flipping between two images - is not quite the same as using vergence (the
rotating of the eyes in their sockets). In the sequential case, the more an object
shifts from one scene to the other (or the more it shifts as our head is
bobbed back and forth) provides a measure of relative distance. Many researchers
believe that snakes "weave" back and forth to judge striking distance in this
way, and the many animals that do not have significantly overlapping visual
fields from eyes placed on the sides of their heads probably use similar
techniques for judging close distances. But again, this provides a relative rather than
an absolute measure, and the visual impression has to be built up
sequentially by viewing many points, which is why the flipping back and forth has to be
repeated.

All of this isn't to say that sequential displays of "stereo" images may not
be useful in some situations. The method has the advantages that 1) it can be
used for color images, which red/blue glasses cannot (although polarized
lenses or side by side viewing can); 2) it works for the significant fraction of
people who don't use both eyes equally and can't fuse stereo; and 3) it is
trivially easy to accomplish with any computer display system (you can do it in
Photoshop by putting the two images in layers, and writing an action to turn the
top layer on and off, and the use of layers makes it easy to align the images
properly as well). My own experience with it suggests that the speed of the
flipping has to be individually adjusted for different viewers, and that a
significant fraction of people find the process more distracting than helpful.

John Russ
=======

In a message dated 11/4/04 2:57:02 PM, wesaia-at-iastate.edu writes:

} I don't know why Mike thought that disclaimer necessary. I understand that
}
} stereo depth perception can always be quantitative even though it is often
}
} left as qualitative. Our brains normally learn the spatial relationships
}
} (i.e., trigonometry) that allow us to extend our hand some distance to
}
} grasp an object. (Granted, we often update our estimates via continuous
}
} monitoring of the progress.) Even though it seems "intuitive" to our human
}
} systems, with appropriate measurements, any two images taken at known
} angles should be able to lead to quantitative measurements of relative
}
} distance or height. If there is a restriction besides incomplete
} information (i.e., unknown angles) that limits it to qualitative
} perception, I am not aware of it.

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Diane: Hitachi can be found at http://www.hitachi-hhta.com/. Amray was
bought by someone but I can't remember who. I'm not even sure there
still in the SEM business. Surely someone on the list will know their
fate.

Diane.Ciaburri-at-gd-ais.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
Becky Holdford (r-holdford-at-ti.com)
972-995-2360
972-648-8743 (pager)
SC Packaging FA Development
Texas Instruments, Inc.
Dallas, TX
~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~

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Diane
Hitachi very definitely alive.
British and American contacts for Hitachi below:

http://www.hitachi-hitec-uk.com/elecmicro/index.php
http://www.hitachi-hta.com/pageloader.aspx?type=product&id=62&orgid=42

Amray? no idea, sorry.

Chris

Dr. Chris Jeffree

----- Original Message -----
} From: {Diane.Ciaburri-at-gd-ais.com}
To: {Microscopy-at-msa.microscopy.com}
Sent: Thursday, November 04, 2004 9:07 PM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (pgrover-at-bilbo.bio.purdue.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, November 4, 2004 at 09:05:34
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Email: pgrover-at-bilbo.bio.purdue.edu
Name: Paul Grover

Organization: Purdue University

Title-Subject: [Microscopy] [Filtered] stereo scope collimation

Question: A colleague of mine who works at a stereo dissecting scope much of the day complained of fatigue resulting from his use of the microscope. I did the test I had learned to check the collimation of binoculars, and found the scope significantly out of whack. Can anyone direct me to an article or other resource on this problem/associated dangers/repair?

Paul

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From MicroscopyL-request-at-ns.microscopy.com Thu Nov 4 18:46:00 2004

Contents Retrieved from Microscopy Listserver Archives
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Thanks, John.

Couldn't have said it better :-)

mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Thursday, November 04, 2004 14:26
To: wesaia-at-iastate.edu; Microscopy-at-msa.microscopy.com

As noted, Hitachi is still around. Amray was bought for their FE gun
technology by KLA-Tencor, an American manufacturer of semiconductor
manufacturing equipment. As soon as they bought Amray (around 3 years
ago), KLA let non-FE customers know that they weren't going to provide
service for their instruments anymore. They claimed that they would still
support the FE instruments, I don't know if they still do. They may have
continued producing laboratory SEMs for awhile as Amray's stock was
depleted, but I'm sure they are out of that business now. They do make
specialized SEMs for wafer inspection.

Allen R. Sampson
Advanced Research Systems
317 North 4th. Street
St. Charles, Illinois 60174

phone (630) 513-7093 fax (630) 513-7092 http://www.sem.com

On Thursday, November 04, 2004 5:15 PM, Becky Holdford
[SMTP:r-holdford-at-ti.com] wrote:
}
}
}
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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}
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-------
}
} Diane: Hitachi can be found at http://www.hitachi-hhta.com/. Amray was
} bought by someone but I can't remember who. I'm not even sure there
} still in the SEM business. Surely someone on the list will know their
} fate.
}
} Diane.Ciaburri-at-gd-ais.com wrote:
}
}
} -----------------------------------------------------------------------
-------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe --
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} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
} -----------------------------------------------------------------------
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} }
} } I'm reviewing marketing literature for SEMs and I can't seem to find
Hitachi
} } or Amray. Did I miss something? Did they get absorbed into another
} } company, get out of the SEM business, or am I just using a bad search
} } engine?
} }
} } Thanks for any help,
} }
} } Diane Ciaburri
} }
} }
} }
} }
}
} --
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
} Becky Holdford (r-holdford-at-ti.com)
} 972-995-2360
} 972-648-8743 (pager)
} SC Packaging FA Development
} Texas Instruments, Inc.
} Dallas, TX
} ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 4 22:23:04 2004

Contents Retrieved from Microscopy Listserver Archives
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1st International Conference on Environmental, Industrial and Applied
Microbiology (BioMicroWorld-2005)
"Fostering Cross-disciplinary Applied Research in Microbiology and Microbial
Biotechnology"
Badajoz, Spain, March 15-18th, 2005
http://www.formatex.org/biomicroworld2005

Dear colleague,

On behalf of the organizers, you are cordially invited to send abstracts of
your best research for presentation at the forthcoming 1st International
Conference on
Environmental, Industrial and Applied Microbiology (BioMicroWorld-2005),
that will take place in March 2005 in Badajoz (Spain).

Modern microbiology includes a broad variety of scholarly approaches leading
to a better understanding of all living things at the macroscopic,
microscopic/single-cell and nanoscopic/molecular level, producing beneficial
applications in medicine, agriculture, industry, and ecology. Therefore, the
Conference will specially welcome papers reporting interdisciplinary
researchers, relating Microbiology with other Sciences as Physico/chemistry,
Materials Science, Polymer Science, Environmental Sciences, Genetics,
Pharmacology, Microscopy/Imaging Science, Nanoscience and Nanotechnology,
etc. In other words, we are specially (but not exclusivelly) interested in
reports applying the techniques, the training, and the culture of
Microbiology to research areas usually associated with other scientific and
engineering disciplines, from an applied perspective.

Main topics of the Conference are

- Environmental Microbiology, Marine Microbiology, Water/Aquatic
Microbiology, Geomicrobiology
- Industrial Microbiology - Future Bioindustries
- Food Microbiology
- Cell Engineering
- Pharmaceutical Microbiology
- Agriculture, Soil, Forest Microbiology
- Structure and Morphogenesis
- Analytical Techniques, Imaging Techniques, Microscopy
- Microbial Physiology, Metabolism and Gene Expression
- Microbial Biotechnology
- Aerospace Microbiology, Astro(micro)biology
- Quantitative Models and Bioinformatics in Microbiology
- Methods in Basic and Applied Microbiology
- Medical Microbiology
- Microbiology Education

IMPORTANT DEADLINES

Submission of abstracts: November 22th, 2004 (at least for oral
presentations; some more time will be given to abstracts for posters)
Submission of Full Papers for publication: On site

CONFERENCE PUBLICATION - PROCEEDINGS

1. Proceedings Book
A multi-volume book entitled "Recent Advances in Multidisciplinary Applied
Microbiology. Biological, Physical, Chemical and Engineering Aspects" will
be published
including Full papers of works (oral, posters) presented at the conference.
The book will be published by an international publisher (now in
negotiations with Elsevier Science), in order to give it a broad
international distribution.

2. Abstracts Book
A separate Abstracts Booklet will be published with abstracts of works
presented at the Conference. It will be distributed at the beginning of the
conference.

3. International Journals special issues
Agreements are being arranged with several international journals, in order
to produce special issues based on very good papers presented at the
Conference.
Manuscripts must be delivered during the Conference, according to the
instructions we will give in due course for each journal. All papers will be
strictly reviewed and treated as regular papers. High quality and high
impact special issues should be produced. Please refer to the conference
website for details.

4. 2005 Current Reviews on Applied Microbiology
A call for mini-reviews on topics covered by the conference will be made by
the end of October. Accepted reviews will be collected in a comprehensive
publication. Authors will receive a free copy of the publication, and its
content will be made freely available shortly after the conference.
Proposals for mini-reviews are welcome from qualified researchers,
irrespective they attend the conference or not.

SPECIAL SESSIONS - WORKSHOPS

- Workshop on Modern Microscopy Techniques in Applied Microbiology
- MICROFACTORIES - Microbial Production of Chemicals and Pharmaceuticals
- Workshop on Biotechnologically Relevant Enzymes and Proteins
- Workshop on Studies on Extracellular Matrix: Biology and Physico/chemistry
- Workshop on Biosurfactants: Purification, Mass production, Applications
- Workshop on Yeast and Bacterial Flocculation: Fundamentals and Industrial
interest
- Worskhop on Microbial Biosensors
- Methods in Cell, Proteins, Enzymes and other Biomolecules Immobilisation
- Workshop on Biohydrogen - Hydrogen production by Microorganisms, as a
Novel Source of Renewable Energy
- Workshop on Bioremediation
- Workshop on Microbial Biopolymers: Synthesis, Characterization and
Applications
- Methods in Cell Adhesion: Classical and Novel Methods, from Macroscopic to
Nanometer scale, from Biochemistry to Nano(bio)technology

PLENARY LECTURES

Plenary talks include:

"Biomarkers to define interactions in the environment and health"
David C. White, Director of the Center for Biomarker Analysis, University of
Tennessee, USA

"Novel time-resolved Fluoresecence based Immunoassays and Real-time PCR
assays in Microbiological Applications"
Timo Lövgren, Department of Biochemistry and Food Chemistry/Biotechnology,
University of Turku, Finland

"The genetics and biochemistry of malonate and 2,4-D biodegradation by
Burkholderia cepacia strain 2a"
Ian James Bruce, Nanobiotechnology Research Group, Istituto di Scienze
Chimiche, Universita degli Studi di Urbino, ITALY / School of Science,
University of
Greenwich, UK

Alexander Steinbuchel, Institut fur Molekulare Mikrobiologie und
Biotechnologie, Munster, GERMANY
[titletobeannounced]

SEARCHING FOR PARTNERS FOR TRANSNATIONAL COLLABORATION PROJECTS?

One of the major goals of this International Meeting is promoting contacts
among researchers and research groups for the creation of Multinational
Thematic and
Research Networks, as well as promoting the future presentation of
collaborative joint projects within some of the EU Operational Programs and
Iniciatives (for
example, the EC Sixth Framework Program). Presentation of results of already
executed or under developement European Projects are highly encouraged,
specially in the case of Interdisciplinary projects. Also initial proposals
for future EU projects are welcome. All ideas/proposals for collaboration
will be included in a booklet entitled "Scientific/Tecnological Offer for
Collaborative Projects", to be distributed at the beginning of the
Conference. If your group wants to be included, please download the form
available at the conference website and send it to the conference
secretariat.

If you have any question or suggestion, please do not hesitate to contact
us.

We hope you find it interesting to present your work(s) at the Conference,
and we certainly hope to receive your abstract(s) by November 22th!

Best regards,

Fatima Penya
BioMicroWorld-2005 Secretariat
Formatex Research Centre
C/Zurbaran, 1 2ş Office 1
06001 Badajoz, SPAIN
Phone/Fax: +34 924258615
E-mail: applmicro-at-formatex.org
http://www.formatex.org/biomicroworld2005

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 08:05:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jose.maria.manero-at-upc.es) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, November 5, 2004 at 07:34:24
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Email: jose.maria.manero-at-upc.es
Name: Jose M Manero

Organization: UPC

Title-Subject: [Microscopy] [Filtered] How to prepare samples to see barcteria?

Question: Dear Colleagues

I have samples of tooth decay. My goal would be to have a look on the existing bacteria in the caries through an electron microscopy. Samples were observed by me by means of an ESEM (without any kind of preparation), as well as I have observed them by a SEM (just gold coated samples) and I have never been able to see them. Has anyone experience in how to prepare samples to see the bacteria? Do I have to use conventional methods: deshydratation, fixation, critical points, conductive coatingsÖ?

Than you in advance for your co-operation!

Dr. Jose M Manero
Electron Microscopy Laboratory
Departament of Materials Science
UPC. Av Diagonal 647. Barcelona. Spain

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From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 08:04:53 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (steven.obenour-at-unison.ae.ge.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, November 5, 2004 at 07:19:48
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Email: steven.obenour-at-unison.ae.ge.com
Name: Steven Obenour

Organization: GE Aircraft Engines

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for metallographic etchants for Ruthenium and Kovar.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 08:30:53 2004

Contents Retrieved from Microscopy Listserver Archives
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Colleagues

The October Archives are now on-line at:

http://www.microscopy.com/MicroscopyListserver

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 08:40:24 2004

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Hi Diane,

As you have already learned via the list, Hitachi is alive and well and
still very much manufacturing Microscopes. Amray however, was purchased
by KLA-Tencor a number of years ago and has not been in the Lab SEM
business since. There are several Companies around the country who
specialize in retrofitting and re-selling used Amray Microscopes. If
you are interested in them please contact me off-list.

Michael R. Nesta
General Manager
Energy Beam Sciences, Inc.
800 992-9037
mnesta-at-ebsciences.com
www.ebsciences.com
"Adding Brilliance to Your Vision"

Diane.Ciaburri-at-gd-ais.com wrote:

}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} I'm reviewing marketing literature for SEMs and I can't seem to find Hitachi
} or Amray. Did I miss something? Did they get absorbed into another
} company, get out of the SEM business, or am I just using a bad search
} engine?
}
} Thanks for any help,
}
} Diane Ciaburri
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 09:54:35 2004

Contents Retrieved from Microscopy Listserver Archives
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Thanks for all your responses!

Summary of SEM Manufacturers:

Amray was absorbed by KLA -Tencor and only makes SEM's for the Semiconductor
industry.
Hitachi SEMs can be found under http://www.hitachi-hta.com/
Leo is back to being Zeiss - http://www.smt.zeiss.com/
Jeol is still http://www.jeol.com/
CamScan now includes Tescan - - http://www.camscan-usa.com
RJ Lee is now Aspex - http://www.aspexllc.com
FEI (was Philips, Electroscan)- http://www.feicompany.com

I have to admit, JEOL gets a gold star in my book. I still love my old 35C
(vintage 1978), and the best part is that JEOL service has kept it up and
running all these years. (No financial interest - just a satisfied
customer.) If anyone has had good or poor service on other brands of SEM,
I'd be interested in hearing about it.

Thanks!

Diane Ciaburri

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 11:39:55 2004

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I'm in the funny position of suddenly and quickly needing to purchase a EDS
system. I have a detector from Thermo Noran and I am considering both the
Noran System 6 and PGT's Avalon 8000. I need imput!

Has anyone experence difficult with either system? Any horror stories I
should know about? Anyone in love with their EDS system? Should I look at
another vendor?

Here's the catch.... I gotta place the order by Dec 1 2004....

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

330-668-2235 Ext. 238

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 12:06:03 2004

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Dear Steven:

I can offer the following suggestions:

Material: Ruthenium (Ru)
Type: Microetching
Method: Chemical etching
Etchant (electrolyte): 80 ml distilled water, 20 ml hydrochloric acid, 1
ml hydrogen peroxide (3 %).
Procedure: Few minutes.
Remarks: Ru rich alloys and Ru-Mo alloys.
Reference: G. Petzow, Metallographic Etching, ASM (American Society for
Metals), 1978, p. 45.

Material: Ruthenium and alloys (Ru), osmium and alloys (Os), rhodium and
alloys (Rh)
Type: Macroetchant
Method: Chemical etching
Etchant (Electrolyte): 50 ml lactic acid, 20 ml HNO3, 30 ml HF.
Procedure: Few minutes.
Remarks: Grain contrast.
Reference: Practical Metallography, Vol. 7, No. 6, 1970, p. 314-324.

Material: Kovar, cemented carbides (Fe)
Type: Microetchant
Method: Chemical etching
Etchant (Electrolyte): 100 ml distilled water, 20 g ammonium persulfate.
Procedure: No data.
Remarks: Kovar, Cemented carbides with Co base.
Reference: Practical Metallography, Vol. 10, No. 7, 1973, p. 407-413.

Material: Kovar alloy (Fe)
Type: Microetchant
Method: Electrolytic etching
Etchant (Electrolyte): 10 ml HCl (conc.), 90 ml alcohol.
Procedure: 6-10 V.
Remarks: Kovar alloy.
Reference: Practical Metallography, Vol. 10, No. 7, 1973, p. 407-413.

This data was extracted from a Metallographic Etch Database that we
offer. You can get more details on it by typing in the search term
"MED" on our website at www.southbaytech.com. Alternatively, contact me
off-line and I can email the information to you.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

by way of MicroscopyListserver wrote:

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (steven.obenour-at-unison.ae.ge.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, November 5, 2004 at 07:19:48
---------------------------------------------------------------------------

Email: steven.obenour-at-unison.ae.ge.com
Name: Steven Obenour

Organization: GE Aircraft Engines

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for metallographic etchants for Ruthenium and Kovar.

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 12:50:26 2004

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Hopefully this isn't 'the last word' because experience suggests that the notion of eye convergence being vital to stereoscopic depth perception is mistaken. Stereo viewing of side-by-side photos with the eyes unconverged (i.e., pointed straight ahead) and essentially kept in fixed positions is easily learned and is practiced by many microscopists and other photointerpreters. Maybe there's research showing that the brain also processes eyeball rotation information, but simply presenting the appropriate (suitably matched and aligned) images containing horizontal parallax to each eye seems sufficient. The essential information is parallax, as is easily demonstrated with stereo imagery that lacks any secondary depth cues such as shadows, occlusion or familiar subjects that we associate with size. Stereo images taken of thin-slice or foil samples in TEM are good examples.

On the subject of depth measurements from stereo images, these can of course be absolute if the projection geometry and magnification are known. The relative depth sense of stereoviewing is not essential for measuring the parallax shifts in stereo images, but it helps a lot for correctly matching corresponding image features in relation to their heights in the perceived stereo model.

Larry

Larry Thomas
Pacific Northwest National Laboratory
P.O. Box 999
Mail Stop P8-16
Richland, WA, USA

email: Larry.Thomas-at-pnl.gov
phone: (509) 372-0793
fax: (509) 376-6308

} ----------
} From: Mike Bode
} Sent: Thursday, November 4, 2004 4:57 PM
} To: 'DrJohnRuss-at-aol.com'
} Cc: Microscopy-at-msa.microscopy.com
} Subject: [Microscopy] RE: Re: Summary of stereo viewing
}
}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Thanks, John.
}
} Couldn't have said it better :-)
}
} mike
}
}
} Michael Bode, Ph.D.
} Soft Imaging System Corp.
} 12596 West Bayaud Avenue
} Suite 300
} Lakewood, CO 80228
} ===================================
} phone: (888) FIND SIS
} (303) 234-9270
} fax: (303) 234-9271
} email: mailto:info-at-soft-imaging.com
} web: http://www.soft-imaging.com
} ===================================
}
}
}
} -----Original Message-----
} } From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
} Sent: Thursday, November 04, 2004 14:26
} To: wesaia-at-iastate.edu; Microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Re: Summary of stereo viewing
}
}
}
}
} ----------------------------------------------------------------------------
} --
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America To

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 13:25:49 2004

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Viewing side-by-side images with eyes pointed "straight ahead" turns out not
to be a counter-example. Your eyes don't stay "straight ahead." They move. If
they didn't, your brain wouldn't get any information about most of the scene.
In fact, when looking at any scene your "fovea point" or point of interest
jumps around all the time, very rapidly (and short of using drugs, you can't
suppress this motion). Tests that track eye motion by bouncing a light off the eye
while a scene is being viewed study the "interesting points" that are
selected, and confirm that the consciously remembered information in the scene only
comes from the places that your vision "visited." Even by trying very hard, it
is difficult to get very much information from portions of a scene that appear
only in your peripheral vision. The "jumping around" process also fills in
the blind spot in your retina, where the optic nerve connects, and where there
are no light sensors. So the point-by-point sequential comparison of depths
determined by vergence of the eyes (even if the motion is slight, and even if the
nominal viewpoint of the eyes is straight ahead towards two side-by-side
images) is in fact the way human vision uses stereo. It is fundamentally different
than the measurement of parallax from a set of stereo images as performed by
a computer.

In a message dated 11/5/04 2:02:06 PM, Larry.Thomas-at-pnl.gov writes:

} Hopefully this isn't 'the last word' because experience suggests that the
} notion
} of eye convergence being vital to stereoscopic depth perception is mistaken.
} Stereo viewing of side-by-side photos with the eyes unconverged (i.e.,
} pointed
} straight ahead) and essentially kept in fixed positions is easily learned
} and is
} practiced by many microscopists and other photointerpreters

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 13:38:02 2004

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On Friday, November 5, 2004, at 01:06 PM, Frank.Karl-at-degussa.com wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
}
}
}
}
} I'm in the funny position of suddenly and quickly needing to purchase
} a EDS
} system. I have a detector from Thermo Noran and I am considering both
} the
} Noran System 6 and PGT's Avalon 8000. I need imput!
}
} Has anyone experence difficult with either system? Any horror stories
} I
} should know about? Anyone in love with their EDS system? Should I
} look at
} another vendor?
}
} Here's the catch.... I gotta place the order by Dec 1 2004....
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}
}
} 330-668-2235 Ext. 238
}
}

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 5 14:09:47 2004

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I looked this up in #5 of the Edington Monograph series

Ru:
electropolish
78g CaCl2.2H2O
200 ml water
6ml conc hydrochloric acid
10V reduced to 7V, 0C (200 and 100 mA/mm^2, respectively)

Since this is a chloride, you might want to check with South Bay Technology and looked up Bernie Kestel's acid free electrolyte for polishing.

Kovar is approximately 53%Fe-29%Ni-17%Co.
I can't find one specifically for Kovar. I would look to the literature. there is one for 18%Ni-Co-Mo maraging steels which is 10% perchloric and 90% ascetic.

I would try some of the perchloric-acetic acid etches, for Fe-Ni alloys or perhaps the chromium trioxide-acetic acid ones for steels. Again, the acid-free electrolyte might work.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: steven.obenour-at-unison.ae.ge.com
[mailto:steven.obenour-at-unison.ae.ge.com]
Sent: Friday, November 05, 2004 9:18 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (steven.obenour-at-unison.ae.ge.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, November 5, 2004 at 07:19:48
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Email: steven.obenour-at-unison.ae.ge.com
Name: Steven Obenour

Organization: GE Aircraft Engines

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for metallographic etchants for Ruthenium and Kovar.

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 05:29:52 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear All,

I would like to know what mounting medium is used for araldite or epon
semithick sections (2-5 micrometer).
We have used canadian balsam so far but this causes wrinkles of sections
under the cover glasses.
So, my question is:
Is there known anything else beside canadian balsam for mounting semithick
epon/araldite sections to study with LM?

Kärt Padari
kartp-at-ut.ee
University of Tartu
Estonia

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 07:26:15 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (somayyeh_kheiri-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, November 8, 2004 at 02:26:04
---------------------------------------------------------------------------

Email: somayyeh_kheiri-at-yahoo.com
Name: kheiri

Title-Subject: [Microscopy] [Filtered] break seed dormancy

Question: I am doing experiments on seed growth on verbascum.
does anybody know how to break the dormancy of the seeds?
many thanks
Somayyeh

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 07:54:00 2004

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Why not use the same resin?
We do. Put some left-over resin from an embedding run into a 1ml syringe.
Ideal for controlled dropwise delivery.
You can seal with Parafilm and keep a stock syringe or two in the freezer
for future use.

Chris

----- Original Message -----
} From: "Kart Padari" {kartp-at-ut.ee}
To: {Microscopy-at-MSA.Microscopy.Com}
Sent: Monday, November 08, 2004 11:45 AM

Hi all,
I have a problem with my TEM. It has a trackball system but the system
is not tracking. I think the sensors are not working.
Here's a description of the system - it resides in a little black box
and is connected to the electronics via a cord that snaps into the box
very much like a telephone cord snaps into a phone:
The X and Y coordinates consist of two separate bars.
The trackball sits between the bars .
On each bar is a wheel that has small holes in it.
As the ball is turned it turns the bars that turn the wheels.
A sensor sits in front of each wheel and coordinates the movement of
the sample. The bars turn, the wheels turn, but there is no specimen
movement.

I want to understand how it works to better understand why it failed
and mainly how it might be fixed.

thanks in advance for any help.
best,
Beth

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 08:55:12 2004

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Xlyene-based mounting media often cause wrinkles in 'thick' sections.
Lots of labs just use a drop of the same embedding meduim (with
accelerator) the section is in, epon, araldite or Spurr.

Geoff

Kart Padari wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
--
**********************************************
Geoff McAuliffe, Ph.D.
Neuroscience and Cell Biology
Robert Wood Johnson Medical School
675 Hoes Lane, Piscataway, NJ 08854
voice: (732)-235-4583; fax: -4029
mcauliff-at-umdnj.edu
**********************************************

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 09:56:34 2004

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I simply use Permount.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Kart Padari [mailto:kartp-at-ut.ee]
Sent: Monday, November 08, 2004 6:45 AM
To: Microscopy-at-MSA.Microscopy.Com

Dear All,

I would like to know what mounting medium is used for araldite or epon
semithick sections (2-5 micrometer).
We have used canadian balsam so far but this causes wrinkles of sections
under the cover glasses.
So, my question is:
Is there known anything else beside canadian balsam for mounting semithick
epon/araldite sections to study with LM?

Kärt Padari
kartp-at-ut.ee
University of Tartu
Estonia

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 10:05:42 2004

Contents Retrieved from Microscopy Listserver Archives
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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Kärt Padari wrote:
============================================================
I would like to know what mounting medium is used for araldite or epon
semithick sections (2-5 micrometer).
We have used canadian balsam so far but this causes wrinkles of sections
under the cover glasses.
So, my question is:
Is there known anything else beside canadian balsam for mounting semithick
epon/araldite sections to study with LM?
============================================================
I would call your attention to the products called "Meltmount™ Thermoplastic
Liquid
Mounting Media" as described on URL
http://www.2spi.com/catalog/ltmic/melt-therm.shtml
and in particular, product Meltmount 1.539 Code 53 which is a direct
replacement for Canada Balsam. I have not heard of any of our customers
experiencing such problems with the Meltmount product.

The product is also available in a second form, Quick-Stick™ Thermoplastic
Liquid
Mounting Media, see URL
http://www.2spi.com/catalog/ltmic/quickstick.shtml

Disclaimer: SPI Supplies offers these two products as plug in replacements
for Canada Balsam and therefore has a vested interest in seeing more people
using them.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 12:36:18 2004

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Hi,
We have used immersion oil sealed with nail polish and it has worked very nice.

Robert Underwood
U of Washington

On Mon, 8 Nov 2004, Kart Padari wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
}
} Dear All,
}
} I would like to know what mounting medium is used for araldite or epon
} semithick sections (2-5 micrometer).
} We have used canadian balsam so far but this causes wrinkles of sections
} under the cover glasses.
} So, my question is:
} Is there known anything else beside canadian balsam for mounting semithick
} epon/araldite sections to study with LM?
}
}
} KĂŻÂżÂ˝rt Padari
} kartp-at-ut.ee
} University of Tartu
} Estonia
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 15:22:00 2004

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Hey folks we need to have a sample analyzed. This is a ceramic chip
capacitor with some foreign material on the top surface (metallic). Can any
one recommend a local service for just basic EDS analysis. Thank you

Robert Fowler
Quality Assurance Failure Analysis Technician
TDK Components USA, Inc.
Multilayer Ceramic Capacitor Division
1 TDK Boulevard
Peachtree City GA 30269-2051
Telephone: (770) 631-0410 Ext.249
Fax: (770) 487-1460
email: robert.fowler-at-tdktca.com
www.component.tdk.com

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 17:42:00 2004

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Hi,

I am trying to find info about possible upgrade of "Desktop Microscopist"
for the Mac OSX system. The web site of Virtual Labs/ Lacuna Labs which was
distributing the software seems to be hacked and I cannot get any contact
info.

Krassimir Bozhilov.

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 18:24:33 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (amarjit.s.brar-at-seagate.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, November 8, 2004 at 11:01:39
---------------------------------------------------------------------------

Email: amarjit.s.brar-at-seagate.com
Name: Amarjit S. Brar

Organization: ASM International

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Chemical etchant for Gold

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 8 21:00:08 2004

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Dear Amarjit:

I have shown below some chemical etch data for gold and gold alloys
extracted from a Metallographic Etch Database that we offer for sale.
You can get more details on it by typing in the search term "MED" on our
website at www.southbaytech.com. Alternatively, contact me off-line and
I can email the information to you.

DISCLAIMER: South Bay Technology produces equipment and supplies as
described above and, therefore, has a vested interest in promoting their
use.

Best regards-

David

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

Material: Gold-Silver-Platinum (Au-Ag-Pt)
Type: Microetchant
Method: Chemical etching
Etchant (Electrolyte): 20 ml KCN (10 %), 20 ml (NH4)2S2O8 (10 %).
Procedure: Use in a hood. Immerse at room temperature for 10-30 s.
Remarks: Electric contact material.
Reference: Metallography, Structures and Phase Diagrams, Metals
Handbook, 8th Edition, Vol. 8, ASM (American Society for Metals), Metals
Park, Ohio 44079, USA, 1973, p. 118.

Material: Gold alloys (Au), palladium alloys (Pd), silver alloys (Ag)
Type: Microetchant
Method: Chemical etching
Etchant (Electrolyte): 1 part 10 % aqueous solution of ammonium
persulphate, 1 part 10 % aqueous solution of potassium cyanide. With
extremely resistant alloys use 20 % solutions.
Procedure: The solution must be used within a few minutes after mixing.
It is very toxic and hence etching should be carried out under a fume
extraction hood.
Remarks: Extremely toxic.
Reference: H. Modin and S. Modin, Metallurgical Microscopy,
Butterworths, London, 1973., p. 392.

Material: Gold (Au), platinum (Pt), palladium (Pd)
Type: Macroetching
Method: Chemical etching
Etchant (electrolyte): 66 ml hydrochloric acid, 34 ml nitric acid.
Procedure: Few minutes. Use hot and fresh!.
Remarks: Au, Pt alloys and Pd alloys.
Reference: G. Petzow, Metallographic Etching, ASM (American Society for
Metals), 1978, p. 43.

Material: Gold (Au), palladium (Pd), platinum (Pt)
Type: Microetching
Method: Chemical etching
Etchant (electrolyte): 100 ml hydrochloric acid, 1-5 g chromium (VI) oxide.
Procedure: Seconds to minutes.
Remarks: Pure Au and Au-rich alloys. Pd and Pd alloys.
Reference: G. Petzow, Metallographic Etching, ASM (American Society for
Metals), 1978, p. 45.

Material: Gold (Au), palladium (Pd), platinum (Pt)
Type: Microetching
Method: Chemical etching
Etchant (electrolyte): 30 (50) ml distilled water, 25 (100) ml
hydrochloric acid, 5 (10) ml nitric acid.
Procedure: 1-5 min. Use hot.!. Remove precipitate of gold chloride with
ammonia water.
Remarks: Pure Pt and Pd. Au alloys. Proportions in parentheses
especially useful for Pt.
Reference: G. Petzow, Metallographic Etching, ASM (American Society for
Metals), 1978, p. 45.

Material: Gold (Au), Pt alloys (Pt), Pd alloys (Pt)
Type: Macroetchant
Method: Chemical etching
Etchant (Electrolyte): 66 ml HCl, 34 ml HNO3.
Procedure: Hot, few minutes.
Remarks: Grain contrast.
Reference: Practical Metallography, Vol. 7, No. 6, 1970, p. 314-324.

Material: Gold (Au) and precious metals.
Type: Microetchant
Method: Chemical etching
Etchant (Electrolyte): 1 part HNO3 (conc.), 10 parts HCl (conc.).
Procedure: Etching temperature 30-35 C (86-95 F). Use a fume cupboard.
Remarks: Gold and precious metals.
Reference: H. Modin and S. Modin, Metallurgical Microscopy,
Butterworths, London, 1973., p. 392.

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 05:14:16 2004

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hello,
Earlier I use to use the araldite kit and blocks were
} soft and good but now we have ordered the :
} "Durcupan water soluble kit" for embedding the
} tissue/culture whatever the mixture i try the
} resultant blocks are brittle and remain
unpolymerize.
} The standard procedure which came along with the kit
} is
} Durcupan A Resin - 27 g
} DDSA - 65 g
} DMP-30 - 6.6 g
} DPB - 2.2 g
}
} Since with this mixture even over a week of
} polymerization at 60 deg blocks are not completly
} polymerize therefore,
}
} I increase the concentration of DDSA, DMP-30 and DBP
} propertionately and tried three different
combinations
} but still i find the incomplete polymerization.
}
} I didnt understad why blocks are not plymerizing
} completly.
} May I have your suggestions comment please.
}
} I thank you in advance

Regards
Arti Harle
Scientist

__________________________________
Do you Yahoo!?
Check out the new Yahoo! Front Page.
www.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 07:16:39 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mingram-at-rohmhaas.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, November 9, 2004 at 07:07:37
---------------------------------------------------------------------------

Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Title-Subject: [Microscopy] [Filtered] SEM and X-rays

Question: All,

Has anyone who has been monitoring their SEM for X-ray leakage found any problems?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 07:36:21 2004

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The following tutorials from the MSA meeting in Savannah are now available
on DVD. See the video catalog at this url for details

http://www.biotech.ufl.edu/sems/newtape00.htm

# 266 - Techniques for Electron Tomography. by M. Marko $15.00
#267 - Energy Dispersive X-ray spectrometry in SEM. By Dale Newbury $15.00
# 268 - Introduction to Electron Holography - by Molly McCartney - $15.00
# 269 - Introduction to Fluorescence and Image Correlation Spectroscopy -
by P. Wiseman $15.00

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 08:10:55 2004

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Hi Sven,

Matrox does not support TWAIN. You can buy a twain driver; the demo version is
free: http://www.ebbosoft.com/Products/Demoversion/demoversion.html

There are some drivers for Linux: http://www.emlix.com/index.php?id=163

For Windows, Matrox frame grabbers need the drivers of the Matrox Imaging Library
(MIL), which comes in different versions. MIL is a programming environment. If you
are a good C++ programmer, this is the right thing for you. If not - you are screwed.
Well, these frame grabbers are for machine vision, anyway.

Other imaging packages depend on the MIL redistribution, which has to be installed
before installing the other software. Mathworks Matlab Image acquisition toolbox
does support your frame grabber. There are even drivers for National Instruments
IMAQ for the Matrox Meteor II.

More or less no programming is needed for other packages, like Mediacybernetics
Image Pro Plus, Optimas, AnalySIS, Matrox Inspector, Rauscher GrabIT, Streampix,
Fabrimex QuickView Software QView-C/M, and others:
http://www.matrox.com/imaging/third/3rdparty.cfm

The problem is: all these solutions are quite expensive (except Linux), or the software
does not more than any video freeware.

:-) Torsten

P.S. If somebody has drivers for Active Silicon Snapper-Dig16, please send me an
email. The company is not responding to emails (www.activesilicon.co.uk).

}
} Hi all,
}
} I have here a Sony CCD-camera which is connected to a Matrox Meteor II
} framegrabber card. Both in good conditions, no doubt, but is there
} some software I can use for live imaging and acquisition? Analysis is
} a nice extra, but is not necessary!
}
} I tried to connect to ImageJ, but this did not work out. I need to
} make it TWAIN. How does this works/is this possible?
}
} Thanks in advance,
}
} Sven Terclavers
}
}

Dipl. Biol. Torsten Fregin

Universität Hamburg - Biozentrum Grindel (ZIM)
Abt. Neurophysiologie
Martin-Luther-King-Platz 3
20146 Hamburg, Germany
Telefon *49-(0)40-42838-3931
Fax *49-(0)40-42838-3937
eMail Torsten.Fregin-at-zoologie.uni-hamburg.de

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 08:26:53 2004

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We used to monitor 2 SEMs and 2 TEMs and never found any leakage so we
stopped several years ago.

Joe Neilly, Research Investigator
Abbott Laboratories
R4R9, AP31
200 Abbott Park Rd.
Abbott Park, IL 60064-6202

Voice: 847-938-5024
Fax: 847-938-5027
E-mail: joe.neilly-at-abbott.com

mingram-at-rohmhaas.com (by way of MicroscopyListserver)
11/09/2004 07:32 AM

To: microscopy-at-microscopy.com
cc:
Subject: [Microscopy] viaWWW: SEM and X-rays

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mingram-at-rohmhaas.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, November 9, 2004 at 07:07:37
---------------------------------------------------------------------------

Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Title-Subject: [Microscopy] [Filtered] SEM and X-rays

Question: All,

Has anyone who has been monitoring their SEM for X-ray leakage found any
problems?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 09:26:15 2004

Contents Retrieved from Microscopy Listserver Archives
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Mike,

The state of Illinois used to require radiation surveys, but they deemed
that SEMs pose no risk for leakage. Vacuum requirements to turn on the beam
ensure that you don't have a major mechanical breach.

Alan Stone
ASTON

At 07:32 AM 11/9/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 11:23:06 2004

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On Nov 8, 2004, at 3:57 PM, K.N. Bozhilov wrote:

} I am trying to find info about possible upgrade of "Desktop
} Microscopist"
} for the Mac OSX system. The web site of Virtual Labs/ Lacuna Labs
} which was
} distributing the software seems to be hacked and I cannot get any
} contact
} info.
}
Dear Krassimir,
You might ask Scott Davilla of 4Pi Systems.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 12:25:43 2004

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Greetings,
This question concerns the way cameras digitize gray levels.
I have two cameras in my lab, one is an analog CCD camera (meaning it
puts out an NSTC composite video signal), about a dozen years old,
and connected to a frame grabber card in a computer; the other is a
new digital ccd camera (meaning built in "frame grabber") with
acquisition software on the computer. When I look at the image
histograms of the same object taken with the two cameras, the
histograms are different. In particular, while the older camera
generates a more or less smooth curve, the newer one generates a
really noisy curve with the number of pixels at adjacent gray levels
differing substantially. To put this intuatively, the new camera
seems to be noisy in gray-level space. Does anyone know why the two
set ups should digitize so differently?

Now (just to confuse matters) it is true that the new camera
captures 12-bit images and the old one just 8-bit, but I don't see
why having more gray levels should substantially increase the
digitization noise. (the increase is not small, it really obvious).

Thanks for any insight into this.

Tobias
--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 13:01:32 2004

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} Hello Listers:
}
} Does anyone out there know where I could get a part for a LKB NOVA
} ultramicrotome? The part needed is 90-00-0047 which is the band attached
} to the specimen arm of the microtome. I used to be able to get parts from
} Norman J. Woodside but can't find him anymore. He lived in Catonsville,
} MD. Anyone out there able to help?
}
} Thanks!
}
} Karen L. Bentley, M.S.(previously Jensen)
} Associate Scientist & Project Manager
} Electron Microscope Research Core
} University of Rochester Medical Center
} Rochester, NY 14642
} 585-275-1954
}

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 13:12:54 2004

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I used to use Durcupan water-miscible resin, or Aquembed which is the same
thing, all the time. I found the best way to use it is as a dehydrating
agent only (just the Durcupan A component), and then put the tissue through
graded mixtures of Durcupan A with Epon mix - Epon substitute plus DDSA and
NMA. After at least two changes of 100% Epon mix, infiltrate with the Epon
mix plus DMP30 before embedding and polymerising.

Lesley Weston.

on 09/11/2004 3:30 AM, Aarti Harle at aarti_harle-at-yahoo.co.in wrote:

}
}
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}
} hello,
} Earlier I use to use the araldite kit and blocks were
} } soft and good but now we have ordered the :
} } "Durcupan water soluble kit" for embedding the
} } tissue/culture whatever the mixture i try the
} } resultant blocks are brittle and remain
} unpolymerize.
} } The standard procedure which came along with the kit
} } is
} } Durcupan A Resin - 27 g
} } DDSA - 65 g
} } DMP-30 - 6.6 g
} } DPB - 2.2 g
} }
} } Since with this mixture even over a week of
} } polymerization at 60 deg blocks are not completly
} } polymerize therefore,
} }
} } I increase the concentration of DDSA, DMP-30 and DBP
} } propertionately and tried three different
} combinations
} } but still i find the incomplete polymerization.
} }
} } I didnt understad why blocks are not plymerizing
} } completly.
} } May I have your suggestions comment please.
} }
} } I thank you in advance
}
} Regards
} Arti Harle
} Scientist
}
}
}
}
} __________________________________
} Do you Yahoo!?
} Check out the new Yahoo! Front Page.
} www.yahoo.com
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 13:55:54 2004

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I've had our ESEM checked every year by the "radiation inspectors", as per
Canadian government requirements, but they never find any leaks.

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Alan Stone [mailto:as-at-astonmet.com]
Sent: Tuesday, November 09, 2004 11:41 AM
To: mingram-at-rohmhaas.com
Cc: microscopy-at-microscopy.com

Mike,

The state of Illinois used to require radiation surveys, but they deemed
that SEMs pose no risk for leakage. Vacuum requirements to turn on the beam
ensure that you don't have a major mechanical breach.

Alan Stone
ASTON

At 07:32 AM 11/9/2004, you wrote:

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Alan Stone
ASTON Metallurgical Services Co., Inc.
200 Larkin Drive Ste A
Wheeling, IL 60090
847/353-8100
www.astonmet.com

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 9 19:44:32 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mikeraj-at-streamyx.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, November 9, 2004 at 09:53:42
---------------------------------------------------------------------------

Email: mikeraj-at-streamyx.com
Name: Mike Marks

Organization: Seagate

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I would like to understand the difference between quantitative and semi-quantitative EDS analysis ? What are the differences between them ? Thanks !

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 02:14:58 2004

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Hi,

My personal experience is mostly with analog cameras, so my answer is
may be not complete.

In a CCD camera which provides an analog videosignal (NTSC or PAL) the
pixel-grid of the camera is resampled into a video signal, where NTSC is
525/60 Lines/Field and PAL is 625/50 Lines/Field.

So even if one line of the CCD-grid has more than 525 individual
elements, this will be resampled to 525 lines in a NTSC video signal.
The discrete pixelation of the image is smoothed into an analog
representation.

The framegrabber resamples this analog signal back into an digital image
with 525 lines (NTSC). An 8-bit framegrabber will resample the voltage
range of the videosignal into values ranging from 0 to 255. This
approach was done to make digital CCD cameras compatible with old analog
video systems.

This is one component which contributes to what you may see in an image
from your analog camera.

In the digital camera this back an forth conversion from digital to
analog and back to digital does not happen and what you get is the "raw"
pixelation at the CCD-grid.

If you sample the CCD-pixels at 8- or 12-bit, you express the dynamic
range of the CCD into a different subsampling. If you sample a CCD with
the same physical characteristics at 12-bit (4096 levels) or 8-bit (256
levels) you will have a finer or coarser redout for the same dynamic
range. The 8-bit readout will average adjacent grey levels into 1/128
size steps of the 12-bit system.

From what I understand the digital 12-bit image may look "uglier", but
better represents what a CCD-grid "sees".

Regards,

Peter

===================================================================================
Tobias Baskin wrote:
}
}
} ------------------------------------------------------------------------------
}
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} -------------------------------------------------------------------------------
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}
} Greetings,
} This question concerns the way cameras digitize gray levels. I have
} two cameras in my lab, one is an analog CCD camera (meaning it puts out
} an NSTC composite video signal), about a dozen years old, and connected
} to a frame grabber card in a computer; the other is a new digital ccd
} camera (meaning built in "frame grabber") with acquisition software on
} the computer. When I look at the image histograms of the same object
} taken with the two cameras, the histograms are different. In particular,
} while the older camera generates a more or less smooth curve, the newer
} one generates a really noisy curve with the number of pixels at adjacent
} gray levels differing substantially. To put this intuatively, the new
} camera seems to be noisy in gray-level space. Does anyone know why the
} two set ups should digitize so differently?
}
} Now (just to confuse matters) it is true that the new camera
} captures 12-bit images and the old one just 8-bit, but I don't see why
} having more gray levels should substantially increase the digitization
} noise. (the increase is not small, it really obvious).
}
} Thanks for any insight into this.
}
} Tobias

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 04:08:58 2004

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Please continue with radiation checks on electron microscopes. Our SEM
started leaking (30KV only) after 22 years. We are now constructing a
lead bucket (inverted!) to contain the leak.

Dave

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:mingram-at-rohmhaas.com]
Sent: 09 November 2004 13:33
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (mingram-at-rohmhaas.com) from
http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
November 9, 2004 at 07:07:37
------------------------------------------------------------------------
---

Email: mingram-at-rohmhaas.com
Name: Mike Ingram

Title-Subject: [Microscopy] [Filtered] SEM and X-rays

Question: All,

Has anyone who has been monitoring their SEM for X-ray leakage found any
problems?

------------------------------------------------------------------------
---

This incoming email to UWE has been independently scanned for viruses
and any virus detected has been removed using McAfee anti-virus software

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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 04:35:46 2004

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Mike Marks writes ...

} Question: I would like to understand the difference between
} quantitative and semi-quantitative EDS analysis ? What are the
} differences between them ? Thanks !

My 1st response is that "quantitative" numbers come with an error analysis
.. but hardly any EDS analysis does. In the context of EDS, qunatitative
would imply "each element measured against its reference standard" ... and
"semi-quantitative" would only imply an attempt to convert x-ray counts to
weight percent ... either by some standardless method, or by at least
scaling the spectrum with a minimum of standards (usually one).

hth & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 05:57:50 2004

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Hi,

There might be a very simple explanation for what you see.

First: Is the histogram really noisy or is it spiky?

I'm assuming that neighboring values in the histogram are very different but
in a systematic way.

In that case it could simply mean that you've digitized the image twice by
the time it reaches the computer, once to 12 bits in the camera and then to
8 bits to import it into the software you use for calculating the histogram.

What you see could be an effect of this two-step rounding procedure, which
can make every second 8-bit value more frequent than the neighboring one, if
the quantization levels don't happen to be exactly matched.

For (the extremest) example let's say you have output values 0, 1, 2, 3, 4
etc. from the first digitization and you requantize these at the levels 0,
1.5, 3, 4.5 etc. to produce new output values 0, 1, 2, 3 etc.
The inputs 0 and 1 will both be output as 0,
The input 2 will be output as 1,
The inputs 3 and 4 will both be output as 2,
and so on.

You see that even outputs will be twice as frequent as odd ones.

Maybe it's that.

Philip

-----Original Message-----
} From: Tobias Baskin [mailto:baskin-at-bio.umass.edu]
Sent: 09 November 2004 19:41
To: microscopy-at-msa.microscopy.com

Greetings,
This question concerns the way cameras digitize gray levels.
I have two cameras in my lab, one is an analog CCD camera (meaning it
puts out an NSTC composite video signal), about a dozen years old,
and connected to a frame grabber card in a computer; the other is a
new digital ccd camera (meaning built in "frame grabber") with
acquisition software on the computer. When I look at the image
histograms of the same object taken with the two cameras, the
histograms are different. In particular, while the older camera
generates a more or less smooth curve, the newer one generates a
really noisy curve with the number of pixels at adjacent gray levels
differing substantially. To put this intuatively, the new camera
seems to be noisy in gray-level space. Does anyone know why the two
set ups should digitize so differently?

Now (just to confuse matters) it is true that the new camera
captures 12-bit images and the old one just 8-bit, but I don't see
why having more gray levels should substantially increase the
digitization noise. (the increase is not small, it really obvious).

Thanks for any insight into this.

Tobias
--
_ ____ __ ____
/ \ / / \ / \ \ Tobias I. Baskin
/ / / / \ \ \ Biology Department
/_ / __ /__ \ \ \__ 611 N. Pleasant St.
/ / / \ \ \ University of
Massachusetts
/ / / \ \ \ Amherst, MA, 01003
/ / ___ / \ \__/ \ ____
http://www.bio.umass.edu/biology/baskin/
Voice: 413 - 545 - 1533 Fax: 413 - 545 - 3243

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 06:22:28 2004

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Dave
These things do not just happen spontaneously.
Presumably some change in the shielding has occurred since
manufacture. Can this be put down
to wear and tear, or has some critical item of the original shielding
been damaged or removed?
Chris

Dr. Chris Jeffree
University of Edinburgh

----- Original Message -----
} From: "David Patton" {David.Patton-at-uwe.ac.uk}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, November 10, 2004 10:24 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (leem-at-unorth.ac.za) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, November 10, 2004 at 06:15:43
---------------------------------------------------------------------------

Email: leem-at-unorth.ac.za
Name: Mike

Organization: University of the North

Title-Subject: [Microscopy] [Filtered] Quantitative versus semi-quantitative

Question: As I understand this issue, "Either a method is quantitative or it is qualitative". Two methods could be quantitative with a differing degree of uncertainty. Therefore semi-quantitaive does not exist.
Regards
Mike Lee

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 08:14:28 2004

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Where does it leak ? I suppose it is diffusion, but with the beam current
used in a SEM (a few pA up to a few 100 nA), I don't imagine what
measuable leaks you may have. Doing the X-ray generators control in our
lab, I'm quite familiar with these questions. But on a SEM, I don't see
what is possible. What kind of counter do you use to check the leakage ?

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

On Wed, 10 Nov 2004, David Patton wrote:

}
}
} ------------------------------------------------------------------------------
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} -------------------------------------------------------------------------------
}
} Please continue with radiation checks on electron microscopes. Our SEM
} started leaking (30KV only) after 22 years. We are now constructing a
} lead bucket (inverted!) to contain the leak.
}
} Dave
}
} -----Original Message-----
} } From: by way of MicroscopyListserver [mailto:mingram-at-rohmhaas.com]
} Sent: 09 November 2004 13:33
} To: microscopy-at-microscopy.com
} Subject: [Microscopy] viaWWW: SEM and X-rays
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} ------------------------------------------------------------------------
} -------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (mingram-at-rohmhaas.com) from
} http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
} November 9, 2004 at 07:07:37
} ------------------------------------------------------------------------
} ---
}
} Email: mingram-at-rohmhaas.com
} Name: Mike Ingram
}
} Title-Subject: [Microscopy] [Filtered] SEM and X-rays
}
} Question: All,
}
} Has anyone who has been monitoring their SEM for X-ray leakage found any
} problems?
}
} ------------------------------------------------------------------------
} ---
}
}
}
} This incoming email to UWE has been independently scanned for viruses
} and any virus detected has been removed using McAfee anti-virus software
}
}
}
} This email has been independently scanned for viruses and any virus detected has been removed using McAfee anti-virus software
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}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 08:19:12 2004

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Meeting Announcement

SEM WORKSHOP
November 19th 2004
Presented by:
Midwest Microscopy and Microanalysis Society
Affiliate of the Microscopy Society of America and the Microbeam Analysis
Society of America

RSVP to:

Mr. Arvid Casler
Federal Mogul Sealing Systems
7450 N. McCormick Blvd.
Skokie, IL 60076-8103
Tel: 847-568-2016
Fax: 847-568-1925
Email: arvid_casler-at-fmo.com

Note: Respondents will be responsible for registration fees

8:00AM 5:00PM

Baxter Corporate Headquarters
Deerfield, IL
(Directions below)

Registration Fees

MMMS members: before Nov. 12th - $ 25.00 after Nov. 12th - $ 35.00
Non-members: before Nov. 12th - $35.00, after Nov 12th -$ 45.00
(MMMS membership included in fee)
Students: before Nov. 12th - $15.00, after Nov 12th - $ 25.00 (MMMS
Student membership $5)

8:00AM 8:45AM Setup and registration

8:45 10:15AM James Pawley, University of Wisconsin,
What FE does for SEM?

Abstract Nowadays operation of the SEM at 1.5 kV or even 500v for high
resolution topographic imaging has become so commonplace that it is easy to
forget that it was not always thus. High resolution SEM at low beam voltage
is poses a number of important technological challenges.

This talk we will review the rationale for making the effort to overcome
these obstacles: Why is it worth it? It will also outline the technological
developments that were needed to make it a reality.

10:15 10:45AM Break

10:45AM 12:15PM John Mackenzie, North Carolina State University,
From Grains to Pixels: Digital Imaging Today

Abstract Digital imaging continues to encroach on the tasks formally
performed using wet silver halide photography. The improvements in inkjet
technology continue to advance with no sign yet of a ceiling. Although
still a fair way from matching photographic resolution at the grain level,
the inkjet resolution has matched the photographic resolution at the visual
level. Although cameras are available for the TEM are available, they are
extremely costly and inferior to film. Flatbed scanners do offer a
strikingly inexpensive alternative. The performance of these is currently
remarkable and they also show little sign of reaching a ceiling. Finally,
the core software for digital imaging is Adobe Photoshop. Photoshop
continues to in ways that may improve it's utility to scientists in the future.

12:15PM 1:15PM LUNCH Included

1:15PM 2:45PM Alwyn Eades, Lehigh University, Bethlehem, Pennsylvania
EBSD: An established technique and some new results.

Abstract Scanning electron microscopy (SEM) has, historically, had two
great strengths in the characterization of materials. The power of the
instrument to form images of the sample, up to very high resolution, has
provided excellent information on the morphology of samples. The addition
of energy dispersive x-ray spectroscopy (EDS) has made local chemical
analysis of samples possible and, indeed, routine. This information on the
shape and composition of samples has only more recently become complemented
by crystallographic information on the samples through electron
backscattering diffraction (EBSD).

The importance of this third facet of the characterization of materials is
so great that EBSD has become a standard technique in a very few
years. For scanning electron microscopes that are to be used for the study
of materials, it will very soon be (if it is not already) standard to order
an SEM with EBSD just as it is standard to order it with EDS.

The applications of Electron Backscattering Diffraction may currently be
separated into two groups. On the one hand, EBSD may be used to identify
an unknown phase within the sample. On the other hand, when the sample
consists of a known phase or phases, EBSD can be used to make orientation
maps, which, in turn, can be used to determine: texture, grain size,
strain, crystal quality, the character of grain boundaries, and other more
complex aspects of the microstructure.

As a new field, EBSD is still rapidly expanding in the tasks that can be
performed. It is also the case that aspects of the technique have not been
fully explored. Work at Lehigh has been extending the ability of EBSD to
determine local strain in samples and eliminating artifacts from the
standard analysis methods. Recent work has shown that there is potential
benefit in EBSD work from using an energy filter so that the patterns are
formed using only those electrons that have energies close to the energy of
the incident beam.

2:45 3:15PM Break

3:15 4:45PM Dennis Ward, Federal Bureau of Investigation,
Microanalysis A New Tool in Combating Terrorism

Abstract All of the intelligence agencies in the US have been tasked with
the unprecedented challenge of shifting their focus from traditional
criminalistics to investigating threats of terrorism. Some have been
reorganized under the umbrella of the Department of Homeland Security and
others, such as the FBI, continue to provide investigative services
independently. To succeed in the effort, we have had to identify and
implement enhancements that would benefit our investigative capabilities.
Locally, these include construction of an archival utility for
microanalysis, a rapid response initiative for elemental analysis, and
establishment of a mechanism for technical communications.

As our need to provide characterization of potential weapons of mass
destruction (WMD) has increased, we have realized the potential of
"signature analysis" direct spectral comparisons for providing
presumptive identification of questioned materials. Today's advances in
computer technology have permitted construction of a relational database of
reference materials. The core data of each record is the x-ray spectrum,
but also includes pertinent manufacturer data, laboratory and instrumental
data, reference material data, and other information. A "stand-alone"
utility (Spectral Library Identification and Classification
Explorer SLICE) has been completed, and we currently are considering a
networking utility to permit data sharing between all forensic
laboratories. We have successfully used this resource for presumptive
identification of materials purported to be WMD, and in these cases have
provided significant investigative direction.

The FBI laboratory is required to provide immediate, remote assessment of
materials of forensic significance at crime scenes and disaster sites.
Elemental analysis is not presently available in a mission-oriented,
portable configuration. We have an initiative established to interface
SLICE to recently developed mini XRF in order to provide presumptive
identification of a variety of materials in the field. It is anticipated
that this configuration will offer an important resource to evidence
recovery operations.

In order to provide a platform for rapid, technical communications between
investigators using these related technologies, a secure listserve was
established. It provides a link between every forensic laboratory in the
Western world.

We anticipate that these initiatives may also be useful in the non-forensic
arena, and therefore look forward to establishing mutually productive
collaboration with other federal and private agencies.

Directions to Baxter Corporate Headquarters: 1 Baxter Parkway, Deerfield
Illinois, 60015.

From South (O'Hare Airport): I-294 (Tri State Tollway) north to the merge
with I-94 (west) towards Milwaukee. North on I-94 to Lake Cook Road exit
(50 cents exact change toll). Turn left (west) to first light, Saunders
Road. Turn right on Saunders to Baxter Parkway. Turn right on Baxter
Parkway . Turn right. Follow sings to Visitor parking in garage. See
Deerfield Campus Map and proceed to "Cafeteria, Auditorium, Reception"
building on ground level.

From South (Edens): North to the merge with I-94 (west) towards Milwaukee
on Edens Spur. Exit on Deerfield Road. Turn left (west), then take left on
Saunders Road. Turn left on Baxter parkway. Turn right. Follow sings to
Visitor parking. See Deerfield Campus Map and proceed to "Cafeteria,
Auditorium, Reception" building on ground level.

From North (Milwaukee): From I-94 east, going south towards Chicago exit
at Lake Cook Road exit (50 cents exact change toll). Turn right (west) to
first light, Saunders Road. Turn right on Saunders to Baxter Parkway. Turn
right on Baxter Parkway. Turn right. Follow sings to Visitor parking. See
Deerfield Campus Map and proceed to "Cafeteria, Auditorium, Reception"
building on ground level.

There is a special rate at the Holiday Inn and Suites available for this
meeting, the rate is $ 79.99(ask for the Baxter rate)

Holiday Inn Express Hotel & Suites
CHICAGO-DEERFIELD/LINCOLNSHIRE
2600 LAKE COOK ROAD
RIVERWOODS, IL 60015
UNITED STATES
Tel: 1-847-3740260
Fax: 1-847-3740535

Alan W Nicholls, PhD
Director of Research Service Facility (Electron Microscopy)
Research Resources Center - East (M/C 337)
Room 100 Science and Engineering South Building
The University of Illinois at Chicago
845 West Taylor St
Chicago, IL 60607-7058

Tel: 312 996 1227
Fax: 312 996 8091
Office: Room 110

Web site www.rrc.uic.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 08:23:06 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

David Patton wrote:
====================================================
Please continue with radiation checks on electron microscopes. Our SEM
started leaking (30KV only) after 22 years. We are now constructing a lead
bucket (inverted!) to contain the leak.
=====================================================
Could you tell us more about this leak, which microscope and model you have,
where the leak is occurring, and help others assess whether that kind of
problem could be occurring on their instruments as well.

Conventional wisdom (I think) has suggested that this is something that
would not be happening. The hypothesis I have always been told is that for
an SEM to leak radiation, it would have to be so misaligned that you would
have a vacuum leak and therefore no beam in the first place....and you are
suggesting this is misguided thinking. The exception to this was the case
where there were radiation leaks at the column adjustment knobs and the
exposure would be confined to one's fingers.

Chuck

PS: Please remember that we are nearly 100% paperless and we would ask
that any reply to this message be by way of the "reply" feature on your
software, so that the entire string of correspondence can come back to us
and all be in one place.

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
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Look for us!
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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 09:06:59 2004

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I agree. It's either quantitative or it isn't. Degree of uncertainty
in quantification is a function of many things. There may be some
confusion with "semi-quantitative" and "standardless" quantification.
Again, there is no semi-quantitative analysis.

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:leem-at-unorth.ac.za]
Sent: Wednesday, November 10, 2004 8:29 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (leem-at-unorth.ac.za) from
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Wednesday, November 10, 2004 at 06:15:43
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Email: leem-at-unorth.ac.za
Name: Mike

Organization: University of the North

Title-Subject: [Microscopy] [Filtered] Quantitative versus
semi-quantitative

Question: As I understand this issue, "Either a method is quantitative
or it is qualitative". Two methods could be quantitative with a
differing degree of uncertainty. Therefore semi-quantitaive does not
exist. Regards Mike Lee

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 09:29:46 2004

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Some explanation, with the hands :

Castaing basis for microanalysis tells us that the ratio between

(UnknownConcentration / StandardConcentration) = Something *
(UnknownIntensit / StandardIntensity)

U% UI
- = STh -
S% SI

for each element.

Standards are samples from a known concentration acquired with the same
beam conditions (Primary energie, beam current, counting time, beam
geometrie) than the unknown sample.

"Something" is the matric correction, ZAF or phirhozed, etc. It describe
what hapends in the sample between electrons and atomes, giving photons,
and the relation between what has been measured and what has been emited
in the sample under these conditions. There is a directe proportionality
between the number of atoms from one element and the number of photons
emited, but the emited photons are not the detected ones.

Quantitative will perform the former completely. You need the standards,
for each element and much time to do the measurments, and much care and
much more....

In a Semi-quantitaive analysis, the standard will be replaced by a false
standard, a computation which takes in account all parameters/performences
of the theorie and hardware, to give the "best" result possible. That
result will always give a total concentration of 100%, even if you have
forgotten one element in the quantification list ! If you forget the Mo in
a 316l-stainless steel, the total will be 100%, without the 3% Mo. If you
have forgotten the iron... No comments

In quantitative analysis, the total will be... the reality of what you
have detected, declared, convolutated with the care in the measurements
and the accuracy on the standards. If you forget the Mo in that
316l-stainless steel again, you'll have a total of 95-99% and not 98-102%.

Something more : in quantitative analysis, the standards are measured with
the same hardware than the unknown. So a part of the hardware parameters
(and defects, such as tailing or non linearity of the detector) are the
same for both and don't play much in the computation. That will give
better accuracy in the result, and is not the case in semi-quantitaive.

Hope it helps

Lister, correct me if some is wrong or unclear !

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

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}
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} ---------------------------------------------------------------------------
}
} Email: leem-at-unorth.ac.za
} Name: Mike
}
} Organization: University of the North
}
} Title-Subject: [Microscopy] [Filtered] Quantitative versus semi-quantitative
}
} Question: As I understand this issue, "Either a method is quantitative or it is qualitative". Two methods could be quantitative with a differing degree of uncertainty. Therefore semi-quantitaive does not exist.
} Regards
} Mike Lee
}
} ---------------------------------------------------------------------------
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 10:47:22 2004

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We paid a yearly radiation fee to New Jersey ($106/SEM). The Radiation
Physicist who did our original radiation survey told me that he has
never found a leaky SEM. Apparently some R&D people at Bell Labs used
their SEM to study electron beam lithography and this triggered all
this fuss. I have been informed after our last inspection that our lab
will not have any further NJDEP inspections unless we purchase another
SEM.

FYI: NJDEP regulations exclude TV. TV often will run at 3,000,000
times the current of a tungsten filament SEM and at 25-30 kV.

Dr. J. Roy Nelson
Material Testing Lab
Pennington, NJ 08534

On Nov 9, 2004, at 8:32 AM, by way of MicroscopyListserver wrote:

}
}
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} America
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} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (mingram-at-rohmhaas.com) from
} http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
} November 9, 2004 at 07:07:37
} -----------------------------------------------------------------------
} ----
}
} Email: mingram-at-rohmhaas.com
} Name: Mike Ingram
}
} Title-Subject: [Microscopy] [Filtered] SEM and X-rays
}
} Question: All,
}
} Has anyone who has been monitoring their SEM for X-ray leakage found
} any problems?
}
} -----------------------------------------------------------------------
} ----
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 11:28:08 2004

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Greg;
What happened to the DVD of David Muller's superb tutorial on
STEM presented in Savannah?

John Mardinly
Intel

-----Original Message-----
} From: Greg Erdos [mailto:gwe-at-biotech.ufl.edu]
Sent: Tuesday, November 09, 2004 5:52 AM
To: Microscopy-at-sparc5.microscopy.com

The following tutorials from the MSA meeting in Savannah are now
available
on DVD. See the video catalog at this url for details

http://www.biotech.ufl.edu/sems/newtape00.htm

# 266 - Techniques for Electron Tomography. by M. Marko $15.00
#267 - Energy Dispersive X-ray spectrometry in SEM. By Dale Newbury
$15.00
# 268 - Introduction to Electron Holography - by Molly McCartney -
$15.00
# 269 - Introduction to Fluorescence and Image Correlation Spectroscopy
-
by P. Wiseman $15.00

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 11:56:37 2004

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I was in the front row. There was one person who was livid, almost out
of control. I did not sense any disturbing comments by David Muller, but
if there were, they were not bad enough to warrant the reaction, and he
was just as critical of his own past misunderstandings as he was of
anyone else's. Besides, he was commenting on science, not running for
office. To withhold this DVD would be a travesty. Should one person's
overreaction warrant this action? I think not.

John Mardinly
Intel

-----Original Message-----
} From: Greg Erdos [mailto:gwe-at-biotech.ufl.edu]
Sent: Wednesday, November 10, 2004 9:53 AM
To: Mardinly, John

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 12:02:41 2004

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Peter writes ...

} I agree. It's either quantitative or it isn't. Degree of uncertainty
} in quantification is a function of many things. There may be some
} confusion with "semi-quantitative" and "standardless" quantification.
} Again, there is no semi-quantitative analysis.

I'd agree as well ... but there does need be a term for any
attempt to quantify, but does not provide confidence versus error
analysis. You cannot call it "quantitative", nor can you call
it "qualitative". "Semi-quantitative" does seem to fit(?)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

} ------------------------------------------------------------------------
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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
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} ------------------------------------------------------------------------
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}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (leem-at-unorth.ac.za) from
} http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Wednesday, November 10, 2004 at 06:15:43
} ------------------------------------------------------------------------
} ---
}
} Email: leem-at-unorth.ac.za
} Name: Mike
}
} Organization: University of the North
}
} Title-Subject: [Microscopy] [Filtered] Quantitative versus
} semi-quantitative
}
} Question: As I understand this issue, "Either a method is quantitative
} or it is qualitative". Two methods could be quantitative with a
} differing degree of uncertainty. Therefore semi-quantitaive does not
} exist. Regards Mike Lee
}
} ------------------------------------------------------------------------
} ---
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 13:18:01 2004

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I seem to be getting emails that I assume are supposed to go to the
listserver directly from this gentleman. Perhaps someone could help him post
correctly?

I get this message every time and included is some sort of text attachment.

"This message uses a character set that is not supported by the Internet
Service. To view the original message content, open the attached message.
If the text doesn't display correctly, save the attachment to disk, and then
open it using a viewer that can display the original character set."

William Giles
Senior Electron Microscopist
Metallography Lab Coordinator
P.O. Box 2128
Henderson, Nevada 89009
(702) 566-4436
(702) 564-9038 (Fax)
William.Giles-at-timet.com

*

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 13:31:34 2004

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Of course there is the school of thought that holds that, as all elements are present in
all samples, it's only a question of whether the level of any particular element is above
or below the detection limit of whatever technique you happen to be using at the time.

So that kinda rules out 'qualitative' as a term or concept..................

cheers

rtch

} From: "michael shaffer" {michael-at-shaffer.net}
To: "Tomic, Peter (Peter)" {ptomic-at-agere.com} ,
{microscopy-at-microscopy.com}

Greetings,

We are looking to replace our very old Denton Vacuum Evaporator with a new
system. Our main use will be for SEM prep (carbon and Au/Pd), but we also
want explore thicker organic and metal deposits for R&D studies. I would
like to hear from folks that have recent systems. Do you like them? What
would you recommend? What don't you like. Thanks much in advance.

Joseph M. Oparowski
Center for Materials Science - Consulting and Failure Analysis
Bose Corporation Joseph_Oparowski-at-bose.com
The Mountain, M/S 415 Phone: (508) 766-1371
Framingham, MA 01701-9168 Fax: (508) 766-1313

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 15:05:38 2004

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Bill

I received his posting just fine and there was no attachment.
My guess is that your Email service is creating the attachment
to report the error.

Just a reminder to all subscribers:

You will never get an attachment of any kind from the Microscopy Listserver
all such items are filtered out. If you do receive an Email with an
attachment that "says" it is from the Microscopy Listserver it is
likely that this is a forged email and probably contains a virus or is spam.

I recommend you immediately delete any Email that says it is from
the Listserver
that has any attachment, regardless of the apparent sender (even if it appears
to be me!).

Nestor
Your Friendly Neighborhood SysOp

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} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
===========================================
Dr. Nestor J. Zaluzec
Argonne National Lab
Materials Science Division/Bldg 212
9700 S. Cass Ave
Argonne, Illinois 60439 USA
Tel: 630-252-7901, Fax: 630-252-4798
Email: Zaluzec-at-aaem.amc.anl.gov
===========================================
TPMLab: http://tpm.amc.anl.gov
NEESLab: http://neestpm.mcs.anl.gov
MMSite: http://www.amc.anl.gov
===========================================

The box said ...
"This program requires Win 95/98/NT or better..."
So I bought a G3 Mac !

===========================================

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 15:13:26 2004

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I suspect radiation leaks are rare on SEM's. However, I do remember a
leak on an SEM which had been modified by the manufacturer to do beam
blanking. The glass liner tube installed with the beam blanker had a
line of sight through one of the wire feedthroughs on the column. As I
recall this was discovered during a state radiation inspection.

Bill

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We paid a yearly radiation fee to New Jersey ($106/SEM). The Radiation
Physicist who did our original radiation survey told me that he has
never found a leaky SEM. Apparently some R&D people at Bell Labs used
their SEM to study electron beam lithography and this triggered all
this fuss. I have been informed after our last inspection that our lab
will not have any further NJDEP inspections unless we purchase another
SEM.

FYI: NJDEP regulations exclude TV. TV often will run at 3,000,000
times the current of a tungsten filament SEM and at 25-30 kV.

Dr. J. Roy Nelson
Material Testing Lab
Pennington, NJ 08534

On Nov 9, 2004, at 8:32 AM, by way of MicroscopyListserver wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (mingram-at-rohmhaas.com) from
} http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday,
} November 9, 2004 at 07:07:37
} -----------------------------------------------------------------------
} ----
}
} Email: mingram-at-rohmhaas.com
} Name: Mike Ingram
}
} Title-Subject: [Microscopy] [Filtered] SEM and X-rays
}
} Question: All,
}
} Has anyone who has been monitoring their SEM for X-ray leakage found
} any problems?
}
} -----------------------------------------------------------------------
} ----
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 15:16:00 2004

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As a minion in a strictly life science EM facility, I probably ought not to
express an opinion on EDS analysis - on the other hand, we have been doing
it on "life science" specimens in one way or another since 1979, so I CAN
speak to what we used to (pre flood) call "Semi Quantitative EDS". There
are times when you don't need or simply can't figure out how to get
accurate gram atom amount quantitation in specimens (ie - virtually any LS
sample) BUT you need to know the relative amount of some element or another
and need to have a portable or comparable number to assess a range of
specimens.

To make a longish story short, we have taken as an internal "standard" an
element whose peak area above background remains steady when analysed under
as nearly identical instrument and speciman prep conditions as possible -
say, the calcium level of the thylakoid region of the algal component of a
lichen. Knowing that the potassium levels of the same region of the cells
is extremely variable when the lichen is exposed to any detectable amount
of sulfur derivative stack gasses (or volcano emissions), one can then set
up a ratio of the background subtracted potassium peak to the background
subtracted calcium peak and then compare the RATIOS across specimens
collected from various areas as normalized spectra - say, known distances
from a sulfur-containing gas source. You can then build curves that are
sort of like dose-response curves and have a baseline to use when assessing
the amount of sulfur containing gas that may be/have been present in an
area where these lichens grow. Lots of variables, hard to control,
certainly NOT quantitative, but more useful that just looking at randomly
collected spectra and guessing - hence, the epithet Semi - Quantitative EDS.

Author's note - we haven't done this in anger since the first (in our life
times) Mt. St. Helen's eruption - around 20 plus years ago -

Bill Sharp

William P. Sharp
Arizona State University
School of Life Sciences, box 4501
Tempe, AZ 85287-4501
Phone - (480)-965-3210
Fax - (480)-965-6899

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 16:34:39 2004

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On Nov 10, 2004, at 1:12 PM, Oparowski, Joseph wrote:

} We are looking to replace our very old Denton Vacuum Evaporator with a
} new
} system. Our main use will be for SEM prep (carbon and Au/Pd), but we
} also
} want explore thicker organic and metal deposits for R&D studies. I
} would
} like to hear from folks that have recent systems. Do you like them?
} What
} would you recommend? What don't you like. Thanks much in advance.
}
Dear Joseph,
We bought the Cressington 208 about a year and a half ago for
evaporation of carbon and metals, so we needed two power supplies--one
for each substance. I like the turbopump feature and the fact that it
is a desktop unit, and we have had good performance with it. It takes
the unit about half an hour to reach the low 10^-5 range, which can be
problematic if you need to evaporate onto many specimens and cannot do
them all at once. I cannot say much about long-term reliability, since
the unit is still pretty new, but there have been no problems so far.
I have no affiliation with either the manufacturer or distributer (Ted
Pella) of this equipment except as a satisfied customer.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 17:09:29 2004

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We do quantitative x-ray analysis of frozen plant tissues, by using
standards which are frozen droplets of known element (ion) concentrations,
and analysing them in exactly the same way as we analyse the vacuole or
cytoplasm of the plant cells. Both plant tissues and droplets are planed
flat in a cryomicrotome, they are given the same etching to remove frost,
then coated with Al. Each sample/cell is counted for the same (live-)time,
and we check that all SEM parameters are the same each time and as steady as
possible. The SEM (JEOL 6400) is usually pretty stable after the first
hour. We can go down to about 20 mM for most biologically relevant
elements, which is less sensitive than we'd like, but still very useful.
The main limitation is the time required to do this....

This method was developed by a colleague, Cheng Huang, who, fortunately for
us, works just nearby.

cheers,
Rosemary Whtie

Dr. Rosemary White rosemary.white-at-csiro.au
Microscopy Centre ph. 61-2-6246 5475
CSIRO Plant Industry mob. 61-0402 835 973
GPO Box 1600 fax. 61-2-6246 5000
Canberra, ACT 2601
Australia

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 19:23:59 2004

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I survived Radiation Safety people attack, because it's considered now that
my "poor" JEM1200-EX TEM is "X-ray machine"... So, they applied all
requirements for radiation safety work on it... This is a bad news, the
good news - they excluded SEMs from that black list recently...

X-rays should be detected by special counter, Geiger counter does not react
on X-rays.
Sergey

At 06:38 AM 11/10/2004, you wrote:

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_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 19:31:17 2004

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Hi all;

The New York Times had an article this morning about the preservation of electronic data. Since this has been discussed here I thought some of you might be interested in the story. The link is http://www.nytimes.com/2004/11/10/technology/10archive.html?hp&ex=1100149200&en=0b6f57f06554be78&ei=5094&partner=homepage

Unfortunately a registration is required (no money, just info). I could have cut and pasted the article but that would likely violate a copyright. It is not a technical article but lists some resources.

cheers, John

********
John S. Vetrano
Sr. Research Scientist
Materials Structure and Performance Group
Pacific Northwest National Laboratory
MSIN P8-16
P.O. Box 999
Richland, WA 99352
Phone: (509)372-0724 Fax: (509)376-6308
Email: mailto:john.vetrano-at-pnl.gov

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 21:20:51 2004

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Paul & Co.;

I believe the EDX hardware vendors do use the words "standardless
quantification." Whether someone understands where the errors may come
from in standardless analyses is the real issue, in my opinion.

Peter Tomic
Agere Systems

-----Original Message-----
} From: Gerroir, Paul [mailto:paul.gerroir-at-xrcc.xeroxlabs.com]
Sent: Wednesday, November 10, 2004 2:47 PM
To: michael shaffer; Tomic, Peter (Peter); microscopy-at-microscopy.com

Peter writes ...

} I agree. It's either quantitative or it isn't. Degree of uncertainty

} in quantification is a function of many things. There may be some
} confusion with "semi-quantitative" and "standardless" quantification.
} Again, there is no semi-quantitative analysis.

I'd agree as well ... but there does need be a term for any attempt to
quantify, but does not provide confidence versus error analysis. You
cannot call it "quantitative", nor can you call it "qualitative".
"Semi-quantitative" does seem to fit(?)

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

} ----------------------------------------------------------------------
} --
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America To Subscribe/Unsubscribe --
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} ----------------------------------------------------------------------
} --
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}
} Below is the result of your feedback form (NJZFM-ultra-55). It was
} submitted by (leem-at-unorth.ac.za) from
} http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on
} Wednesday, November 10, 2004 at 06:15:43
} ----------------------------------------------------------------------
} --
} ---
}
} Email: leem-at-unorth.ac.za
} Name: Mike
}
} Organization: University of the North
}
} Title-Subject: [Microscopy] [Filtered] Quantitative versus
} semi-quantitative
}
} Question: As I understand this issue, "Either a method is quantitative

} or it is qualitative". Two methods could be quantitative with a
} differing degree of uncertainty. Therefore semi-quantitaive does not
} exist. Regards Mike Lee
}
} ----------------------------------------------------------------------
} --
} ---
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 10 21:45:37 2004

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Bill;

Perhaps we're taking the semantics too far but I might distill this down
by saying that if I were in a court of law testifying as an expert
witness I would state that the "quantitative analysis" has caveats
similar to what you stated below for LS samples. If one can compare two
results under identical analytical conditions one derives a quantity.
That, in my opinion, is different than saying an element is there or is
not there.

It was just said that a school of thought is that every sample contains
an atom of everything [entire periodic table], to paraphrase the
statement. That, of course, is a matter of detection limits or
sensitivity. I think Deepak Choprah said we all have an atom of Gandhi
in our bodies simply due to recycling. If so, I'm not sure the one I
have has imparted much wisdom to me in particular. Other atoms from
Gandhi may behave differently.

Cheers,

Peter Tomic
Agere Systems

-----Original Message-----
} From: William P. Sharp [mailto:wsharp-at-asu.edu]
Sent: Wednesday, November 10, 2004 4:31 PM
To: microscopy-at-microscopy.com

As a minion in a strictly life science EM facility, I probably ought not
to
express an opinion on EDS analysis - on the other hand, we have been
doing
it on "life science" specimens in one way or another since 1979, so I
CAN
speak to what we used to (pre flood) call "Semi Quantitative EDS". There

are times when you don't need or simply can't figure out how to get
accurate gram atom amount quantitation in specimens (ie - virtually any
LS
sample) BUT you need to know the relative amount of some element or
another
and need to have a portable or comparable number to assess a range of
specimens.

To make a longish story short, we have taken as an internal "standard"
an
element whose peak area above background remains steady when analysed
under
as nearly identical instrument and speciman prep conditions as possible
-
say, the calcium level of the thylakoid region of the algal component of
a
lichen. Knowing that the potassium levels of the same region of the
cells
is extremely variable when the lichen is exposed to any detectable
amount
of sulfur derivative stack gasses (or volcano emissions), one can then
set
up a ratio of the background subtracted potassium peak to the background

subtracted calcium peak and then compare the RATIOS across specimens
collected from various areas as normalized spectra - say, known
distances
from a sulfur-containing gas source. You can then build curves that are
sort of like dose-response curves and have a baseline to use when
assessing
the amount of sulfur containing gas that may be/have been present in an
area where these lichens grow. Lots of variables, hard to control,
certainly NOT quantitative, but more useful that just looking at
randomly
collected spectra and guessing - hence, the epithet Semi - Quantitative
EDS.

Author's note - we haven't done this in anger since the first (in our
life
times) Mt. St. Helen's eruption - around 20 plus years ago -

Bill Sharp

William P. Sharp
Arizona State University
School of Life Sciences, box 4501
Tempe, AZ 85287-4501
Phone - (480)-965-3210
Fax - (480)-965-6899

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 01:29:31 2004

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Dear All,
We would like to purchase one low-temperature stage (LN2 cooled) for our
JEOL 2010 UHR (with URP 22 pole piece). I am aware of GATAN make and have
contacts from them. I am wondering whether are there any other
manufacturer who can supply low-temperature stage for our machine?
Information may be given off-line also.
Best regards
Satyam
--
Dr. P. V. Satyam
TEM Laboratory
Institute of Physics
Sachivalaya marg
Bhubaneswar - 751005
India
Fax:+91-674-230 0142
Tel:+91-674-230 1058 extn 229
email:tem_iopb-at-iopb.res.in

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 02:36:27 2004

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Hi,

'Semi-quantitative analysis' is an expression we have been
using for several years to ensure that our students
appreciate the limitations of standardless analyses. It is
a very useful shorthand expression to distinguish between a
full quantitative analysis and a less rigorous standardless
analysis.

This does not affect the argument that an analysis is
either qualitative or quantitative with different degrees
of accuracy (or uncertainty) associated with the
quantitative analyses.

Most of our users accept the limitations of using a
semi-quantitative analysis technique instead of making up
reference standards but at least they should understand the
limitations and they can take steps to improve their
results. It is too easy for an unaware user to accept the
computer's 'quantiative' analysis to several decimal places
without questioning it.

Regards,
Ron

On Wed, 10 Nov 2004 07:29:02 -0600 by way of
MicroscopyListserver {leem-at-unorth.ac.za} wrote:

}
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}
} Email: leem-at-unorth.ac.za } Name: Mike } } Organization:
University of the North } } Title-Subject: [Microscopy]
[Filtered] Quantitative versus semi-quantitative } }
Question: As I understand this issue, "Either a method is
quantitative or it is qualitative". Two methods could be
quantitative with a differing degree of uncertainty.
Therefore semi-quantitaive does not exist. } Regards } Mike
Lee } }
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}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 02:37:13 2004

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32nd Scottish Microscopy Group Symposium

Wednesday 17thNovember 2004, Pentlands Science Park, Bush Loan, Penicuik,
nr Edinburgh

Late registration for this meeting via

http://www.abdn.ac.uk/emunit/smg2004.htm

also a programme is available at

http://www.gla.ac.uk/ibls/II/SMGSymp2004.pdf

and the directions for getting there by road are at

http://www.gla.ac.uk/ibls/II/map.pdf

There are over 20 companies represented in the Trade Exhibition
accompanying this meeting.

All welcome but registration forms should be FAXed to Stephan Helfer at
0131 248 2901 to assess numbers for catering.
This can be followed by payment made on arrival.

Dr Laurence Tetley
Division of Infection & Immunity, IBLS,
Integrated Microscopy Facility
Joseph Black Building
University of Glasgow
Glasgow G12 8QQ

l.tetley-at-bio.gla.ac.uk
tel 0141 330 4431
FAX 0141 330 3516

Integrated Microscopy
Facility: http://www.gla.ac.uk/Acad/IBLS/II/em/mcb-em.htm
Cryo Microscopy Group: http://www.cryomicroscopygroup.org.uk
Royal Microscopical Society: http://www.rms.org.uk

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 07:05:16 2004

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Bill,
We have the 208 and our pump time is much shorter than 30 min. In fact
it can be as short as 5-10 min if we do not have the bell jar open for an
extended period of time. Are you fighting high humidity in your lab that
could account for the long pump-down time?

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 11/10/04 6:00 PM, "Bill Tivol" {tivol-at-caltech.edu} wrote:

}
}
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-
}
}
} On Nov 10, 2004, at 1:12 PM, Oparowski, Joseph wrote:
}
} } We are looking to replace our very old Denton Vacuum Evaporator with a
} } new
} } system. Our main use will be for SEM prep (carbon and Au/Pd), but we
} } also
} } want explore thicker organic and metal deposits for R&D studies. I
} } would
} } like to hear from folks that have recent systems. Do you like them?
} } What
} } would you recommend? What don't you like. Thanks much in advance.
} }
} Dear Joseph,
} We bought the Cressington 208 about a year and a half ago for
} evaporation of carbon and metals, so we needed two power supplies--one
} for each substance. I like the turbopump feature and the fact that it
} is a desktop unit, and we have had good performance with it. It takes
} the unit about half an hour to reach the low 10^-5 range, which can be
} problematic if you need to evaporate onto many specimens and cannot do
} them all at once. I cannot say much about long-term reliability, since
} the unit is still pretty new, but there have been no problems so far.
} I have no affiliation with either the manufacturer or distributer (Ted
} Pella) of this equipment except as a satisfied customer.
} Yours,
} Bill Tivol, PhD
} EM Scientist and Manager
} Cryo-Electron Microscopy Facility
} Broad Center, Mail Code 114-96
} California Institute of Technology
} Pasadena CA 91125
} (626) 395-8833
} tivol-at-caltech.edu
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 17:49:35 2004

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I have a Leitz Ergolux with a broken focus mechanism and needs repairs.
Given the 20 year age of this model, Leica USA says it must go to Leica
Germany for repairs. Does anyone on the list have any qualified US
third-party repair sources?

I'm expecting a repair manual for the Ergolux any day so I should be able to
identify the parts for the repair. The replacement parts are still available
from Leica Germany.

Thanks for your help.

Doug Baldwin

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 20:05:53 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (somayyeh_kheiri-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, November 11, 2004 at 12:39:42
---------------------------------------------------------------------------

Email: somayyeh_kheiri-at-yahoo.com
Name: somayyeh

Title-Subject: [Microscopy] [Filtered] thank you for replying me for breaking seed dormancy

Question:

hello all
I would like to thank all the people who answered me
And gave me the solution for breaking seed dormancy of verbascum.

Dr cal lemke, Dr Brbara lotocka, Dr Robert Mcdonald,
Dr Fabian Tricarico and Dr valerie lycnch and Dr Lara sciaraffa and others.
Sincerely
Somayyeh

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From MicroscopyL-request-at-ns.microscopy.com Thu Nov 11 20:06:40 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rmwang-at-berkeley.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, November 11, 2004 at 19:00:20
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Email: rmwang-at-berkeley.edu
Name: Rongming Wang

Organization: National Center for Electron Microscopy, Lawrence Berkeley National Laboratory

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for some person who know how to use the software ěamiraî. I want to do tomography of some nanoparticles. I have used the TOM software and got files with .em and .vol extension and want to use amira for visualization. Or if the amira software can deal with all these from the series images taken from TEM?

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From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 05:05:47 2004

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Dear All,

I have problem as following:- I need to know the relationship between
spatial frequency, noise and SEM magnification. I am not sure the following
is true, please kindly correct me. Thanks

When typical specimen elements of an image occupy several image pixels, the
image itself will have suitable spatial components, i.e. rich information in
low spatial frequency element. Usually digital filtering imaging system
itself is in fact a low pass filter process, and high frequency component
will be treated as noise. Therefore in an image with high magnification, the
signal's spatial elements located at low frequency, it is then easier to
filter out high frequency element - noise. In another trend for an image
with low magnification while the signals will distribute at the high
frequency side. That is to say, some signals of useful information will be
considered as noise, in particular in actual high SNR case.

Pleaes kindly comment with many thanks
Ks.

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 05:29:19 2004

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Royal Microscopical Society

Institute of Physics

Materials Research Society

14th International Conference on

MICROSCOPY OF SEMICONDUCTING MATERIALS

11 - 14 April 2005, University of Oxford, UK

************************************************

Final Call for Papers

************************************************

This international conference will focus on the state-of-the-art in the

study of the structural and electrical properties of semiconductors

by the application of transmission and scanning electron

microscopy, scanning probe microscopy, X-ray techniques and all

related assessment methods.

Special conference sessions will concentrate on recent

developments in high-resolution imaging and analytical (S)TEM,

advances in SPM and SEM applications, the important

characteristics of epitaxial layers (including III-nitrides), quantum

nanostructures (dots, wires and wells), the effects of advanced

device processing treatments (especially for silicon technology),

metal-semiconductor contacts and silicides, together with critical

device properties, FIB applications and failure analysis. Prominent

invited speakers will introduce each topic area: full details are given

at the conference web site:

{underline} {color} {param} 0000,8000,0000 {/param} http://www.rms.org.uk/MSMXIV {/underline} {/color}

The Proceedings of the conference will be published and the final

call for papers has now been issued. Abstracts (deadline 3

DECEMBER 2004) should be submitted by E-mail to
{underline} {color} {param} 0000,7F00,0000 {/param} lucy-at-rms.org.uk {/underline} {/color} .

Additional general conference information can be obtained from the

Secretariat at the RMS ( {underline} {color} {param} 0000,7F00,0000 {/param} lucy-at-rms.org.uk {/underline} {/color} ). The conference

Chairmen are Prof Tony Cullis ( {underline} {color} {param} 0000,8000,0000 {/param} a.g.cullis-at-sheffield.ac.uk {/underline} {/color} ) and Dr

John Hutchison ( {underline} {color} {param} 0000,8000,0000 {/param} john.hutchison-at-materials.ox.ac.uk {/underline} {/color} ), who may be
contacted with any scientific programme enquiries.

************************************************

{nofill}
Professor Tony Cullis FRS
Dept of Electronic and Electrical Eng
University of Sheffield
Mappin Street
Sheffield
S1 3JD, UK

Tel: +44-114-222-5407
Fax: +44-114-272-6391
E-mail: a.g.cullis-at-sheffield.ac.uk

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 06:42:06 2004

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To Mike Marks and all, who have interest to this topic!

I agre with Mike Lee:
/As I understand this issue, "Either a method is quantitative or it
is
/qualitative". Two methods could be quantitative with a differing
/of uncertainty. Therefore semi-quantitaive does not exist.

My contribution:
There is no 'semiquantitative analysis'. The reasons are:

First:
Even, there does not exists really a pure qualitative analysis. In any
case 'qualitative' results should be reported only together with some
remarks for which elements are not detectable (e.g. Carbon if EDX with
Be-window is used) and that all other elements are below the detection
limit (e.g. between 0.1 to 0.3 % with EDX in EPMA / sometimes more /
depends from acquisition time, element overlaps, ...). If not, incorrect
decisions are risked, because the results-user may be is not informed,
that the detection limits are not in order of magnitude of ppm or ppb,
possible to analyze with other analytical techniques.

Second:
In the past, 'semiquantitativ anaysis' was used for 'stanardless
analysis'. But this is wrong because there is the indication, that
standardless is not really quantitative. But, both principle methods
(with or without standards) have errors sources. The advantages are with
standard comparison analysis in case of well defined specimens (flat,
polished) and a good known set of standards. Finally, if the standard is
with identical concentrations, the errors are reduced only to statistic
and systematic errors of data acquisition. But if the analyst has to
analyze rough surfaces, particles or other not well defined specimens
(in most cases given in SEM), the standardless method is the first
choice even from the point of view of errors. In such cases no standards
are really available. The errors of standardless analysis are possible
to get 3% and less (relatively, concentrations } 5% absolute), even in
case of irregular surfaces (P/B-method). And, using P/B methods, even an
absolut determination of element concentrations is given. No
normalization to 100% is necessary. The normalization to 100 per cent is
truly bad, like Jacques has indicated. But modern standardless analysis
has no longer an automatical normalization of results.

Third:
May be some analysts are using 'semiguantitative analysis' for EDX
systems, because the WDX has better detection limits and (sometimes not
ever) results with higher accuracy and precision. They claim, only WDX
analysis results are 'quantitative'. But the detection limits are only
better of factor ten. Then, all spectrometry methods in electron
microscopes are 'semi quantitative' from the point of view of other
analytical methods (XRF, HPLC, optical spectrometry, ...), because 0.01
per cent (or 100 ppm) are bad from their point of view.

Finally:
We should not longer use the term 'semi-quantitative'. It was used to
discredit EDX or standardless analysis, as well.
If an EPMA-result is reported, an error should be given for each
element concentration result (calculated errors with error propagation
with all statistical and systematical errors). The true errors of so
called 'only quantitative' method of standard comparison procedure can
be much higher than standardless. It depends e.g. from acquisition time
and other influences (see above). Unfortunately most commercial programs
does not have a proper error calculation (most cases only the statistic
error of net counts). That is why Ron wrote:
/It is too easy for an unaware user to accept the
/computer's 'quantiative' analysis to several decimal places
/without questioning it.
But whatever, standardless is quantitative. Errors are a little bit
higher in comparison to well defined standard-comparison, but not in any
cases! If there is a not well defined specimen, the analyst can rely on
standardless methods much more (without 100 per cent normalization!).
The normalization e.g. of net counts to 100 per cent and reporting
of these results... is simple wrong. The non-linear excitation and
absorption interactions in specimen are the reasons, that simple
normalization does not match. These kind of results are never
quantitative, from all point of view. Better is, to have no analysis
results or only qualitative list of elements (but take into mind:
chapter 'First').

Best regards

Frank Eggert

-------------------------------------------------
http://www.microanalyst.net
-------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 07:44:20 2004

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You are correct. It is inappropriate to use the same filter for the two
different images. A filter should be tuned to the frequency content of the
information contained in the image. If the image components and noise are of
similar spatial frequencies then at least some noise will necessarily be
passed along with the image components. Otherwise, your other choice is to
attenuate the noise to a greater degree at the expense of the high frequency
components of the image.

Simple low pass filtering is not the only option, though. Pattern noise,
such as diagonal bands, can be effectively removed in the frequency domain
without destroying the high frequency content of the entire image, for
example. Also, for spike noise, median filters can be very effective at
maintaining high frequency image information (edges) while dramatically
reducing the noise.

Bruce Girrell

} Usually digital filtering imaging system
} itself is in fact a low pass filter process, and high frequency component
} will be treated as noise. Therefore in an image with high
} magnification, the
} signal's spatial elements located at low frequency, it is then easier to
} filter out high frequency element - noise.

} In another trend for an image
} with low magnification while the signals will distribute at the high
} frequency side. That is to say, some signals of useful information will be
} considered as noise, in particular in actual high SNR case.

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 11:46:00 2004

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We also purchased a 208, at least 2 yrs ago now in my previous
position. Our pump down time was quite short compared to 30 min.
indicated by Bill Tivol in his note. The unit was easy to use i.e. user
friendly, and required only minimum maintenance. We had one carbon, and
two metal evaporation sources for high and low angle. We ordered a
rotary accessory however never received that. This was important to us
for SEM biological samples or any samples with very rough topography.
We had many users, and still had no problems. This was in general one
of the best evaporators I've purchased over the many years of my
microscopy career. I have no affiliation with the manufacturer of this
equipment except as a satisfied customer.

Cheers,
Judy Murphy
Stockton, CA

Oparowski, Joseph wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 12:31:16 2004

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Doug;
I know of two:
Optotek
Box 2140
Los Gatos, CA 95031-2140
Contact Klaus Ryser, (800) 924-6023

SERCO Technical Services, Inc.
12520 Morgan Territory Road
Livermore, CA 94551
Contact Emile Meylan, 800 (483) 0508

John Mardinly
Intel

-----Original Message-----
} From: Doug Baldwin [mailto:dougbaldwin-at-mindspring.com]
Sent: Thursday, November 11, 2004 4:05 PM
To: microscopy-at-msa.microscopy.com

I have a Leitz Ergolux with a broken focus mechanism and needs repairs.
Given the 20 year age of this model, Leica USA says it must go to Leica
Germany for repairs. Does anyone on the list have any qualified US
third-party repair sources?

I'm expecting a repair manual for the Ergolux any day so I should be
able to
identify the parts for the repair. The replacement parts are still
available
from Leica Germany.

Thanks for your help.

Doug Baldwin

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 13:50:48 2004

Contents Retrieved from Microscopy Listserver Archives
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We are interesting in buying a LVEM 5 microscopy. I really appreciate
anyinformation or any advice about it
I am sending you the web page of it:
http://www.lv-em.com/
Thank you in advance

Dr. Carina Ferrari

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 12 17:51:58 2004

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The following is forwarded from San Joaquin Delta College in Stockton, CA.
Sorry for the short notice, I just received it myself. Briefly, this is a
technical position at a community college. Lots of interaction with
students. Twelve months a year, they list salary at $ 3034 - 3687/mo.
Follow the link below for the details.

}
} Hi folks,
}
} I believe that the best way to advertise for our open EM Technician
} Position is through the EM community itself. So I'm asking you to
} forward this email to anyone who might be interested in applying for the
} position.
}
} Links to the job description and application forms can be found at:
}
} http://www.deltacollege.edu/dept/hr/classified.html
}
} The application deadline is December 3, so there isn't much time.
}
} Thanks for your help!
}

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Nov 13 08:57:09 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (cherry.greiner-at-tufts.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, November 12, 2004 at 16:04:32
---------------------------------------------------------------------------

Email: cherry.greiner-at-tufts.edu
Name: Cherry Greiner

Organization: Tufts University

Title-Subject: [Microscopy] [Filtered] MListserver:Non infinity corrected microscope

Question: I have a used Leica Orthoplan UV microscope, a non-infity corrected microscope that I am aligning. I'd like to understand what the optics are doing for reflected illumination. The instruction manual only describes transmission illumination.

I am coupling a collimated beam from a lamp (+condenser). First element my input beam encouters in the microscope is a lens with a focal length of } 100 mm, 2nd element is a smaller lens and an aperture diaphragm followed by a field diagphragm, splitter then objective. The 2nd smaller lens is only 90 mm from the first lens. Not sure why this is located { focal lenght of first lens. I am assuming that because they have 2 lenses, I'm suppose to have a collimated beam after my 2nd lens which is not true in this case. Can anyone give me any idea what the purpose of each lens and if these lenses are at the correct location? Anyone familiar with this microscope?

Thanks
Cherry Greiner

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From MicroscopyL-request-at-ns.microscopy.com Sat Nov 13 08:58:07 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (pollingmel-at-aol.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, November 13, 2004 at 08:33:46
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Email: pollingmel-at-aol.com
Name: Mel Pollinger

Organization: New York Microscopical Society

Title-Subject: [Microscopy] [Filtered] MListserver: Optical Microscopy - Olympus

Question:
I am looking for an Olympus MTV-S video adapter with lens. I also would like to find an NFK 6.7x LD. for the Olympus trinocular head for the BHT system. Does anyone have either or both of these items for sale or swap?

Mel Pollinger
H: 201-791-9826

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From MicroscopyL-request-at-ns.microscopy.com Sat Nov 13 08:57:42 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Bstud-at-yandex.ru) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, November 13, 2004 at 05:32:28
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Email: Bstud-at-yandex.ru
Name: Andrey

Title-Subject: [Microscopy] [Filtered] monte CArlo SImulation of electroN trajectory in sOlids

Question: Please, help me to use this program. It has a strange option "Surface radius of BE". Answer, if you know, what it means.

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From MicroscopyL-request-at-ns.microscopy.com Sat Nov 13 08:56:48 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, November 12, 2004 at 05:06:22
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Email: kssim-at-mmu.edu.my
Name: kssim

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear All,

I have problem as following:- I need to know the relationship between spatial frequency, noise and SEM magnification. I am not sure the following is true, please kindly correct me. Thanks

When typical specimen elements of an image occupy several image pixels, the image itself will have suitable spatial components, i.e. rich information in low spatial frequency element. Usually digital filtering imaging system itself is in fact a low pass filter process, and high frequency component will be treated as noise. Therefore in an image with high magnification,the signal's spatial elements located at low frequency, it is then easier to filter out high frequency element - noise. In another trend for an image with low magnification while the signals will distribute at the high frequency side. That is to say, some signals of useful information will be considered as noise, in particular in actual high SNR case.

Pleaes kindly comment with many thanks
Ks.

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 08:58:32 2004

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Greetings,

I'm looking for advice from anyone with experience in the preparation of
Xenopus eyes for TEM. Specifically interested in your favorite protocol for
basic anatomy.

Thanks, Robert
--
Robert Fitton
Teaching Associate/Director of Laboratories
Luther College
Department of Biology
700 College Drive
Decorah, IA 52101

Voice 563-387-1559
FAX 563-387-1080

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 11:35:34 2004

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Hi Robert,
Back some 25 yrs ago, we worked on TEM for Xenopus for 3 yrs or so. For
the eye, we used either Epon 812 (could substitute Embed 812 or any
successful Epon substitute) or LR White. The important part however was
the vacuum infiltration which we used at every step. Most of the
protocol was standard except we extended the times.

3% Glut or 3%Glut2.5%Paraformaldehyde - 3 hrs
Wash
2% OsO4 - 1.5 hrs
Wash
Dehydration in 25,50,75,95,100 EtOH
For Epon
PropOxide 2X
PO:Epon (2:1,1:1,1:2) 12 hrs each
Pure Epon 2 changes
Let sit in capsules 12 hr before polymerization in oven

LRWhite: same up to PropOxide
No PO
No ratio infiltration
Pure LRWhite - 5 changes
Polymerize

We also often did an en bloc uranyl acetate stain after the OsO4.

If I did it today, would use microwave protocols with cold stage and
vacuum unit in microwave.

Cheers,
Judy Murphy
Stockton, CA

Robert Fitton wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 12:43:12 2004

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Greetings,

I am currently working on a Hitachi S4800 FESEM with a snorkel-type
objective lens. I noticed that other than the beam crossover used for
imaging (which corresponds to the displayed working distance), there is a
second crossover that produces a half-decent image (probably larger spot).

I haven't looked into the electron optics (this should read: I was too
lazy), but I believe this has something to do with either the magnetic field
in the final lens or the field of the lower SE detector.

Can anyone explain this phenomenon?

Thanks,
Daniel Salamon
Technical Officer, Electron Microscopy

National Institute for Nanotechnology, NRC
W6-081 ECERF Bldg
9107-116 Street
Edmonton, AB. T6G 2V4

Phone: Office (780) 492 8878
Lab (780) 492 8872
DocuFax: (780) 492 8632

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 13:02:26 2004

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I really want to thank everyone, including all the sales reps, who have
answered my request for information on EDS systems.

I was out of town for a week and I was not able to access my E-mail or
office phone, for this I apologize. The information and literature has
been very helpful!

Thanks again to everyone who chipped in and contributed!!

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 13:25:09 2004

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Hello,

Do CE courses exist for microscopists?

If yes, could someone pls direct me to a site that has some.

Thank you,

Robert Harries

Robert E. Harries, PEng. MBA
General Manager
data Vinci, Inc
6362 First Line Road
Kars Ontario K0A2E0 Canada

Phone 613-489-2581
Fax 613-489-0739
Email reh-at-dataVinci.ca

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 15:53:23 2004

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Dear listers,

I am searching for manuals and electronic drawings for
ZEISS DSM 960 SEM that I am trying to revive. Any
information pointing to the possible source of such
documentation will be greatly appreciated.

Please respond directly, unless you think that this is
something what may be of general interest.

Thank you very much beforehand,
Valery Ray

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 16:06:39 2004

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Hi, Robert

There are several sources of courses, and most of them offer some sort of
CE credit:
Check out the LeHigh program (Charlie Lynch and team) and the program at
North Carolina State U (John Russ, et. al)
The Royal Microscopical Society in the UK has an on-going educational
program and also offers two levels of certifications.
McCrone Institute in Chicago also has a wide range of courses. I don't
know what their certification standard is but a good case could be made for
"CE" equivalencies.

Then, of course, if you are interested in more customized programs, MME
offers on-site courses. We follow the IACET guidelines for Continuing Ed
credits. If you are interested in this direction, please contact me off-line.

Thanks and good hunting!
Barbara Foster
Microscopy/Microscopy Education

We've moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
W: www.MicroscopyEducation.com

P. S.
Need a good general reference or light microscopy text? Visit our website
to learn more about "Optimizing LIght Microscopy". Copies still available
through MME... even for class-room lots ... and we give quantity discounts.

Caveat: MME has a commercial interest in providing customized, on-site
short courses

At 01:43 PM 11/15/2004, Robert Harries wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 17:14:44 2004

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Barbara Foster wrote:

} McCrone Institute in Chicago also has a wide range of courses. I don't
} know what their certification standard is but a good case could be made
} for "CE" equivalencies.

I have taken three McCrone courses and they granted CEUs. I highly
recommend MCRI. Expensive, but well worth it; very hands-on, Chicago is
a fun town, the instructors are great, and the whole experience is very
motivating.

Don J. Halterman, Jr.

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 17:57:24 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (ptibbits-at-emerson-ept.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, November 15, 2004 at 07:43:29
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Email: ptibbits-at-emerson-ept.com
Name: Patrick Tibbits

Organization: Emerson Power Transmission

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear Microscopists,

I'm seeing that blue-green powder again on the bottom of my Haskris chiller tank. Previous discussions on this list identified it as a corrosion product from the Copper coolant lines.

Can anyone suggest a corrosion inhibitor?

I run 10% ethylene glycol in distilled water. The closed-loop Haskris chiller maintains about 68 degrees F, 14 psi.

Patrick

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 15 21:27:19 2004

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Hi,

A colleague wants to make some Pt mirrors and has asked me to produce
them. I am having a great deal of difficulty evaporating the Pt though.
I have tried tungsten baskets, wires and boats, but when the Pt melts,
before it begins to evaporate the wire or boat breaks.

I have tried heating it up slowly and also quickly but with no luck!
Can anyone give me any clues as to how I might get the Pt films done?
Unfortunately evaporation is the only method I can use.

Thank you very much

Colin Veitch

Electron Microscopist

CSIRO Textile and Fibre Technology

PO Box 21, BELMONT, Vic. 3216. Australia.

E-mail: colin.veitch-at-csiro.au

Web: http://www.tft.csiro.au

Tel: +61 (0) 3 5246 4000
Mob: 0438 538 475
Fax: +61 (0) 3 5246 4811

The information contained in this e-mail message may be privileged or
confidential information. If you are not an intended recipient, you may
not copy, distribute or take any action in reliance on it. If you have
received this message in error, please telephone CSIRO Textile and Fibre
Technology on +61 3 5246 4000.

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 16 03:57:06 2004

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Dear Colin,

Have you tried evaporating the Pt alone, i.e. without involving
tungsten?
Perhaps one or several lengths of 1mm diameter Platinum wire spanning
the two boat electrodes might still give off enough metal to make the
mirror before melting through.
Alternatively, you could remain with tungsten because of its high
melting point. The fragility of tungsten may be due to some amalgamation
with the Pt, which will also perhaps add to your problem by depositing W
also on the mirror. To avoid this, could you perhaps try placing some
inert material between the boat and the Pt? I have never tried this, but
you might try using a thin bed of sand (or pure silica or even a small
piece of coverslip) beneath the Pt. An indirectly heated tiny porcelain
crucible with the Pt inside might also work within a tungsten basket.
The last and possibly most effective way might be to go to electron beam
evaporation (with the gun pointing upwards) because here the substrate
and evaporant do not have to bear any mechanical stresses. If you have
access to suitable EB electrodes and the associated controller
electronics this would be a logical choice
Good luck,

Jim Chalcroft

-----Original Message-----
} From: Colin.Veitch-at-csiro.au [mailto:Colin.Veitch-at-csiro.au]
Sent: Tuesday, November 16, 2004 4:46 AM
To: microscopy-at-msa.microscopy.com

Hi,

A colleague wants to make some Pt mirrors and has asked me to produce
them. I am having a great deal of difficulty evaporating the Pt though.
I have tried tungsten baskets, wires and boats, but when the Pt melts,
before it begins to evaporate the wire or boat breaks.

I have tried heating it up slowly and also quickly but with no luck!
Can anyone give me any clues as to how I might get the Pt films done?
Unfortunately evaporation is the only method I can use.

Thank you very much

Colin Veitch

Electron Microscopist

CSIRO Textile and Fibre Technology

PO Box 21, BELMONT, Vic. 3216. Australia.

E-mail: colin.veitch-at-csiro.au

Web: http://www.tft.csiro.au

Tel: +61 (0) 3 5246 4000
Mob: 0438 538 475
Fax: +61 (0) 3 5246 4811

The information contained in this e-mail message may be privileged or
confidential information. If you are not an intended recipient, you may
not copy, distribute or take any action in reliance on it. If you have
received this message in error, please telephone CSIRO Textile and Fibre
Technology on +61 3 5246 4000.

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 16 05:14:34 2004

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Colin

I normally only use platinum for simple shadowing so the quantities may be a bit less than you need for mirrors, but it should work if you're using a reasonably thick tungsten wire filament (0.5 to 1mm diam) and reasonably thin platinum wire (0.1 to 0.2mm diam) for evaporation. I make the filament by slowly bending a V-shape by hand (not too sharp a V perhaps more like a U) then making two more bends to give me the filament shape ( ___/\___ ). If you bend the tungsten too sharply it tends to greatly weaken it.

The other thing to be careful about is that the tungsten wire is not under any tension when it's held in the electrode connectors of the evaporator. If you can't adjust the filament holder then re-bend the wire until it fits. I would then carefully wrap a length of platinum around the pointed tip as tightly as possible. When heating up the filament keep an eye on it through smoked/dark glass and you should be able to see that the platinum is dark as the tungsten glows yellow/white then it will glow and form a droplet at the tip of the tungsten and with very little extra heat it should disappear over a few seconds. If you rush this final stage the platinum can heat unevenly and may even drop/ping off.

Even if you're careful you may only get 1 or 2 goes out of a tungsten filament especially if you move or adjust it.

Good luck

Malcolm

Malcolm Haswell
e.m. unit
School of Health, Natural and Social Sciences
Fleming Building
University of Sunderland
Tyne & Wear
SR1 3SD
UK

e-mail: malcolm.haswell-at-sunderland.ac.uk

----- Original Message -----
} From: Colin.Veitch-at-csiro.au

Hi Colin:

The melting point of Pt is well below that of W; 1174 vs. 3410 degrees C and
is recommended for evaporation of Pt. The difference in melting points would
preclude any W contamination of your mirror. I would use a Tungsten boat
rather than a basket because of its robust nature. Maybe the baskets you
are using are getting stressed when they are being fixed into the evaporator
causing breakage when heated. A Carbon crucible is really required for Pt
evaporation by the indirect heating method rather than a ceramic vessel
mentioned. James is correct that EB evaporation would give you the best
results, not only the quality of the thin film but better control of the
final thickness too. However, they are very expensive and you may not have
access to them at present.

Best,

Al Coritz
Electron Microscopy Sciences
----- Original Message -----
} From: "James Chalcroft" {jchalcro-at-neuro.mpg.de}
To: {Colin.Veitch-at-csiro.au}
Cc: {microscopy-at-msa.microscopy.com}
Sent: Tuesday, November 16, 2004 5:15 AM

michael shaffer wrote:

} Frank Eggert writes ...
}
}
}
} } To Mike Marks and all, who have interest to this topic!
} }
} } I agre with Mike Lee:
} } /As I understand this issue, "Either a method is quantitative or it
} } is
} } /qualitative". Two methods could be quantitative with a differing
} } /of uncertainty. Therefore semi-quantitaive does not exist.
} }
} }
}
} I agree that all methods which produce absolute values along with
} uncertainty, any uncertainty, should be considered a "quantitative" method.
}
Every quantitative method is charged with uncertainties. Yes, sometimes
these uncertainties are not known or possibly more than 100 per cent.
That is, if one has measured 5% of an element, the element concentration
is between 0..10% (an enormously intervall for confidence), but not
50%... That is quantitative, too. There are analytical methods which
have never better results.
The uncertainties should be distinguish between 'precision' and
'accuracy'. Sometimes it is very easy to measure very precise an
element-concentration (low deviation of different measure results) but
the mean value of all measurements is far away from the truth. You can
determinate an element concentration very precisely, but the result is
wrong. Simply, use a wrong standard or a standard with a false known
element content and that would be happen. Or a quantification of a rough
specimen surface with flat polished standards is the same. At other
hand, the precision can be bad (e.g. using P/B-methods, because of the
low count rate of the Bremsstrahlung background, always directly used).
The results are with higher fluctuations, but the mean value is near to
the truth. You have a statistical uncertainties, but you can rely in the
mean result.

} However, what would you call a method which made no attempt at including
} uncertainty at all?
}
Standardless and standard comparison analysis methods in EPMA as well
have uncertainties (errors always exist). It is not always common
decided, which of both methods have lower uncertainties. That depends
from different influences. The problem of normalization to 100 per cent
with common-used elderly standardless analysis is a source of wrong
results, that is true. Such a method made no attempt at including
uncertainity. It is possible, e.g. if there is a not detectable element
in specimen (or a wrong element identification), all element
concentration results are going to become wrong per definition. I would
call such methods as 'not quantitative' or the results are given with
'draft estimations'.

} There will always be those of us who believe a
} quantitative value includes an error analysis. That is, to be
} "quantitative" is to be "confident". Anything else is "something less than
} quantitative", and we don't care what it is called.
}
} my C&0.02 & cheerios ... shAf :o)
} Avalon Peninsula, Newfoundland
} www.micro-investigations.com (in progress)
}
}
It doesn't matter, I can be confident with an quantitative result and an
qualitative result, as well. The entire uncertainties should be known
(rough common estimations or direct output of the computer program - but
not only statistical error of net counts!) and added to the quantitative
results (to have a confidence intervall). If not, only qualitative
results should be given together with the detection limits for all
elements and the elements, which are not possible to detect.

Finally there are only quantitative results (with different
uncertainties depend from data acquisition time, the selected evaluation
method, the kind and behavior of specimen...) and qualitative analysis
(all 'detected' elements). Semi-quantitative is somewhat between
quantitative results and reporting the detected elements only, I'm not
able to imagine what it is?

Best regards

Frank Eggert
-------------------------------------------------
http://www.microanalyst.net
-------------------------------------------------

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Dear fellow Microscopists,

I have been asked to assemble a comparison list of usage rates for SEM,
EM, TEM, XRD, XRF, ICP-OES, ICP-MS, and for Stable Isotope MS. This
is a huge task and I am appealing to members of the forum for any related
information you can provide.

I am interested in College/University recharge rates as well as private
service
organization charges.

Your help would be most appreciated - Thank you,
Evelyn

Evelyn York

Analytical Facility
Scripps Institution of Oceanography
University of California, San Diego
9500 Gilman Drive
La Jolla, CA 92093-0208

(858) 534-2438

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 16 15:24:40 2004

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Colin
Last time I did Pt shadowing was many years ago. So, I don't remember all
details. What I remember is that I was able to evaporate Pt from the
basket or V-shaped filament. You need to use at least 0.5 mm W wire and
less than 0.1 mm Pt (2-3 cm long). You need to heat up filament very slow
until you melt Pt. At this point you'll see that Pt disappeared... it's
because surface tension - Pt spread on W surface. Than you need slightly
increase current, so Pt will start evaporate. It's just slightly above the
melting point. If you increase current too much or too "sharp" Pt will
splash. For some reason filament may be damaged at this point as well. I
think, with excessive heat, Pt just dissolved filament, it increases
current and finally blow filament out... This is a good news.

The bad news is that as far as I do remember, using "filament" technique,
you could not evaporate much Pt (most Pt will stick to the filament and
will not evaporate). Overloading with Pt will destroy filament (as it
happens in your case). So, you could not produce mirror from one
evaporation (I was trying, it does not work). You need to do multiple
evaporation using fresh pre-heated filament every time. Even than, mirror
would not be perfect: Pt tends to condense on the surface in huge
aggregates, which made surface very rough. The best I had was something
looks like polished graphite surface: silvering black. You better may try
Al or Cr. Good luck, Sergey

P.S. Another trick: you need to use pre-heated filament.
At 02:45 PM 11/16/2004 +1100, you wrote:

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From MicroscopyL-request-at-ns.microscopy.com Tue Nov 16 16:28:42 2004

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Al,
The difference in melting temperatures doesn't necessarily mean you won't
get any W contamination, after all W-Al dendrites is a resolution sample for
SEM. Metals do, very literally, dissolve in one another below their melting
points.

Ken Converse

owner
QUALITY IMAGES
Servicing Scanning Electron Microscopes
Since 1981
16 Creek Rd.
Delta, PA 17314
717-456-5491
Fax 717-456-7996
kenconverse-at-qualityimages.biz
qualityimages.biz

-----Original Message-----
} From: Sample Prep [mailto:sampleprep-at-earthlink.net]
Sent: Tuesday, November 16, 2004 7:51 AM
To: James Chalcroft; Colin.Veitch-at-csiro.au
Cc: microscopy-at-msa.microscopy.com

Hi Colin:

The melting point of Pt is well below that of W; 1174 vs. 3410 degrees C and
is recommended for evaporation of Pt. The difference in melting points would
preclude any W contamination of your mirror. I would use a Tungsten boat
rather than a basket because of its robust nature. Maybe the baskets you
are using are getting stressed when they are being fixed into the evaporator
causing breakage when heated. A Carbon crucible is really required for Pt
evaporation by the indirect heating method rather than a ceramic vessel
mentioned. James is correct that EB evaporation would give you the best
results, not only the quality of the thin film but better control of the
final thickness too. However, they are very expensive and you may not have
access to them at present.

Best,

Al Coritz
Electron Microscopy Sciences
----- Original Message -----
} From: "James Chalcroft" {jchalcro-at-neuro.mpg.de}
To: {Colin.Veitch-at-csiro.au}
Cc: {microscopy-at-msa.microscopy.com}
Sent: Tuesday, November 16, 2004 5:15 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (patricia.miller-at-loctite.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, November 16, 2004 at 13:03:28
---------------------------------------------------------------------------

Email: patricia.miller-at-loctite.com
Name: Patricia Miller

Organization: Henkel Corp.

Title-Subject: [Microscopy] [Filtered] SEM carbon adhesive tabs

Question: I have a scanning electron microscope and use carbon adhesive tabs for mounting specimens. I image a lot of particulates so the background of the mounting tab is visible in the images. I have tried several different suppliers and have not been able to find tabs with the mirror smooth surface I desire. The company I formerly purchased them from is no longer able to supply them. Has anyone recently purchased such tabs, and if not, are there any suggestions what to do about the pitted background my current tabs show?

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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 01:03:33 2004

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I have been very happy with my dealings with Terry Anderson at.
Advanced Instrument Mfg. LLC
15650 Vineyard Blvd.
Unit B
Morgan Hill, CA 95037
phone (408) 779-4240
Fax (408) 779-8492
{}

} From: "Mardinly, John" {john.mardinly-at-intel.com}

} Doug;
} I know of two:
} Optotek
} Box 2140
} Los Gatos, CA 95031-2140
} Contact Klaus Ryser, (800) 924-6023
}
} SERCO Technical Services, Inc.
} 12520 Morgan Territory Road
} Livermore, CA 94551
} Contact Emile Meylan, 800 (483) 0508
}
} John Mardinly
} Intel
}
} -----Original Message-----
} } From: Doug Baldwin [mailto:dougbaldwin-at-mindspring.com]
} Sent: Thursday, November 11, 2004 4:05 PM
} To: microscopy-at-msa.microscopy.com
} Subject: [Microscopy] Leitz Ergolux Repair Sources Needed
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ------------------------------------------------------------------------
} -------
}
} I have a Leitz Ergolux with a broken focus mechanism and needs repairs.
} Given the 20 year age of this model, Leica USA says it must go to Leica
} Germany for repairs. Does anyone on the list have any qualified US
} third-party repair sources?
}
} I'm expecting a repair manual for the Ergolux any day so I should be
} able to
} identify the parts for the repair. The replacement parts are still
} available
} from Leica Germany.
}
} Thanks for your help.
}
} Doug Baldwin
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 01:57:45 2004

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At which magnification, you see the pittings on adhesive? I use
adhesives from SPI and I have no problems about background? Can you send
me a photo of pitting occured at the background? I want to compare it
with background of my images...

Thanks...

Orkun ERSOY

Hacettepe University

Department of Geological Engineering

Beytepe-Ankara / TURKEY

06532

Ph: +90 312 2977700 / 126

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 06:40:24 2004

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Hi all,

We have a 5 year old Leica KMR2 knifemaker that is in need of service.
The scoring wheel has been changed, but it appears that the clamp arm
and pressure swing arm are loose and thus insufficient clamping is
available to create a break. Apparently LEICA doesn't do field service
on knifemakers in our area and requires return to their shop for repair
as many of their techs have limited experience on this instrument. Is
there anyone else in the Maryland area who services these onsite and has
access to LEICA parts?

If anyone knows Pat Capagrossi, our former LKB, then LEICA service
engineer, tell her we miss her and her expertise!

Thanks,
Mary Ellen Pease

Mary Ellen Pease, M.S.
Laboratory Manager
Glaucoma Research Lab & Microscopy and Imaging Core Facility
Wilmer Eye Institute, Johns Hopkins Hospital
175 Woods Research
600 N. Wolfe Street
Baltimore, MD 21287
410-955-3337 (phone/voicemail)
443-287-2711 (fax)
mpease-at-jhmi.edu

WARNING: Email sent over the Internet is not secure. Information sent
by email may not remain confidential.
DISCLAIMER: This email is intended only for the individual to whom it
is addressed. It may be used only in accordance with applicable laws.
If you receive this email by mistake, notify the sender and destroy the
email.

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 07:02:49 2004

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Patricia,
This matter was discussed some time ago so may be archived. I too have
observed "cracking" or "wrinkling" of the double-sided carbon adhesive
which makes for a very distracting background. I remember many
microscopists previously commented on this topic, however, I can't
recall whether a reliable solution to the problem was ever put forward.

Paul

Paul J. Gerroir
Microscopy
Materials Characterization
Xerox Research Centre of Canada
2660 Speakman Drive
Mississauga, Ontario L5K 2L1

Phone: 905-823-7091, ext.216
FAX: 905-822-7022
e-mail: paul.gerroir-at-xrcc.xeroxlabs.com

-----Original Message-----
} From: by way of MicroscopyListserver
[mailto:patricia.miller-at-loctite.com]
Sent: Tuesday, November 16, 2004 8:35 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (patricia.miller-at-loctite.com) from
http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on
Tuesday, November 16, 2004 at 13:03:28
------------------------------------------------------------------------
---

Email: patricia.miller-at-loctite.com
Name: Patricia Miller

Organization: Henkel Corp.

Title-Subject: [Microscopy] [Filtered] SEM carbon adhesive tabs

Question: I have a scanning electron microscope and use carbon adhesive
tabs for mounting specimens. I image a lot of particulates so the
background of the mounting tab is visible in the images. I have tried
several different suppliers and have not been able to find tabs with the
mirror smooth surface I desire. The company I formerly purchased them
from is no longer able to supply them. Has anyone recently purchased
such tabs, and if not, are there any suggestions what to do about the
pitted background my current tabs show?

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 07:56:34 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (vincent.otieno-alego-at-afp.gov.au) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, November 17, 2004 at 00:03:41
---------------------------------------------------------------------------

Email: vincent.otieno-alego-at-afp.gov.au
Name: Vincent

Title-Subject: [Microscopy] [Filtered] SEM Interfaced with a Raman

Question: We are considering the posibility of interfacing a Raman spectrometer with an SEM. I know Renishaw has a commercial unit (SCA) that can be used to achieve this interface.

Does anyone know if there are any alternative suppliers of such an interface?

Are there any 'home-made' types that are in use?

Thanks.

Vincent

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 08:10:26 2004

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Just a suggestion, but Ag tape works very nicely. It has higher electrical conductivity and hence less specimen charging. It also has the advantage of being less "sticky" which facilitates removing the specimen from the tape/stub if that is required. The only caveat is that it is much more expensive. However, if used sparingly, it seems to pay for itself in time. I ruined many fragile samples trying to pry them loose from carbon tape and even the carbon "dots."

I won't endorse any specific vendor since I'm sure everyone can find silver tape vis-ŕ-vis the web.

Regards to everyone,

Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Gerroir, Paul [mailto:paul.gerroir-at-xrcc.xeroxlabs.com]
Sent: Wednesday, November 17, 2004 8:20 AM
To: by way of MicroscopyListserver; microscopy-at-microscopy.com

I have had a problem with these as well and have returned to double sticky
scotch tape, which can be sputter coated. If I wanted a really smooth
background I use glass cover slips. There are round ones that fit a
Cambridge type stub. If stuff doesn't stick I will charge the glass with
poly-lysine or coat it with "grid glue". Grid glue is made by taking one
inch of scoth tape and dissolving off the sticky in 5 mls of
chloroform. (Some one will correct me if my recipe is wrong) dip the
coverslip in it and let it dry.

Greg

} -----Original Message-----
} } From: by way of MicroscopyListserver
} [mailto:patricia.miller-at-loctite.com]
} Sent: Tuesday, November 16, 2004 8:35 PM
} To: microscopy-at-microscopy.com
} Subject: [Microscopy] viaWWW: SEM carbon adhesive tabs
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Gregory W. Erdos Ph.D.
Assistant Director, Biotechnology Program
Scientific Director, Electron Microscopy
P.O. Box 118525
217 Carr Hall
University of Florida
Gainesville, FL 32611
gwe-at-ufl.edu
352-392-1295
fax- 352-846-0251

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 10:33:31 2004

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I have a question about the focus precision at different wavelengths using
an Olympus 60X N.A. 1.4 Phase 3 objective.

Has anybody noticed a difference in focal plane between images collected at
465 to 490 nm and images collected at 530 to 560 nm?

We thought we might be having a registration problem in our images of CFP &
YFP expressing cells. To confirm this, we looked at 0.1 um Tetraspeck
beads and 2.5 um beads with a broad 488 absorbing dye. (BTW, the
cells/beads are in 2X PBS, viewed through a 1.5 coverslip and using Cargill
Labs type DF oil.) In all the cases, the focal shift appears to be between
0.3 and 0.5 um in Z.

Just wondering if anybody else has seen this with the same type of objective?

Thanks.
____________________________________________________________________________
Michael Cammer Analytical Imaging Facility Albert Einstein Coll. of Med.
Jack & Pearl Resnick Campus 1300 Morris Park Ave. Bronx, NY 10461
(718) 430-2890 Fax: 430-8996 URL: http://www.aecom.yu.edu/aif/
**This electronic transmission contains information that is privileged.**

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 11:33:41 2004

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Workshop Announcement
University of California at Santa Barbara

The Department of Molecular, Cellular, and Developmental Biology and the
Neuroscience Research Institute are sponsoring an advance course on light
microscopy. This 5-day workshop will be offered from March 20 through March
25, 2005 and will consist of lectures and laboratory exercises that will run
from 9 am to approximately 5 pm each day. The seminar/workshop will be
intensive enabling participants to develop theoretical and hands-on
expertise with light microscopes. Attendees will interact closely with the
instructors while using modern research grade microscopes, cameras, and
computers. The seminars and laboratories will cover basic optical theory and
how it pertains to increasing contrast (signal to noise ratio) in biological
samples. Fundamental techniques such as fluorescence, phase contrast,
Nomarski differential interference contrast, and darkfield imaging will be
taught and attendees will use microscopes equipped with these optical
enhancement accessories. In addition, the theory and practice of electronic
image acquisition (analog and digital) will be presented and attendees will
work with low-light cameras, digital image processing computers, and
morphometric programs. There are five research grade microscopes, five
electronic imaging cameras, two computer workstations, and one confocal
microscope. With a maximum enrollment of 10 students, there will be ample
opportunity to work with all of the microscopes and cameras. For those so
interested, intensive hands-on instruction and guidance on the confocal
microscope will be provided.

For a fuller description of the workshop please check the web address below.
Enrollment forms can be completed online and this workshop provides an
opportunity to have a working-vacation in Santa Barbara, California.

http://www.lifesci.ucsb.edu/mcdb/events/imaging_workshop/index.html

Brian Matsumoto
Adjunct Associate Professor
Dept. MCDB, Neuroscience Research Institute
UCSB
Santa Barbara, CA 93106

voice mail 805-893-8702
FAX 805-893-2005

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 12:41:26 2004

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The 38th Annual Fall Symposium of the New England Society for Microscopy (NESM)
will again be held on the campus of Gordon College in Wenham, MA. The Symposium
runs from 12Noon - 8pm on Thursday, December 2nd. There will be 2 scientific
sessions with 5 invited speakers, as an after-dinner speaker. Details can be
found on NESM's website (http://prism.mit.edu:8083) under "current newsletter".

Advance registration for this meeting is REQUIRED. The registration form is
included in the newsletter and the registration fee (as well as dinner choice &
registration form) should be sent to: Paul Bain, NESM Treasurer, HMS-Countway
212, 10 Shattuck Street, Boston, MA 02115. If you have any questions, please
contact Paul at 617-432-3236 or via email: paul_bain-at-hms.harvard.edu. The
deadline for registration is Monday, November 29th.

There has been one change to the program listed: the after-dinner speaker will
now be Dan Gibson of Worcester Polytechnic Institute who will speak on
"Horseshoe Crabs-Lessons from a Living Legend). Dan is currently a Biological
Director of NESM's Board and is running for President-Elect for 2005.

Please mark your calendars and plan to attend this most interesting meeting.

Peggy Sherwood
Corresponding Secretary & Newsletter Editor, NESM

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 13:39:40 2004

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I have wondered about this too, with other lenses. Do you think
that there might be some wavelength dispersion in the specimen
optical system (that is the sample, its mounting medium, the glass
cover slip, and the oil)?

}
}
} ----------------------------------------------------------------------
} -------- The Microscopy ListServer -- Sponsor: The Microscopy Society
} of America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ----------------------------------------------------------------------
} ---------
}
} I have a question about the focus precision at different wavelengths
} using an Olympus 60X N.A. 1.4 Phase 3 objective.
}
} Has anybody noticed a difference in focal plane between images
} collected at 465 to 490 nm and images collected at 530 to 560 nm?
}
} We thought we might be having a registration problem in our images of
} CFP & YFP expressing cells. To confirm this, we looked at 0.1 um
} Tetraspeck beads and 2.5 um beads with a broad 488 absorbing dye.
} (BTW, the cells/beads are in 2X PBS, viewed through a 1.5 coverslip
} and using Cargill Labs type DF oil.) In all the cases, the focal
} shift appears to be between 0.3 and 0.5 um in Z.
}
} Just wondering if anybody else has seen this with the same type of
} objective?
}
} Thanks.
} ______________________________________________________________________
} ______ Michael Cammer Analytical Imaging Facility Albert Einstein
} Coll. of Med. Jack & Pearl Resnick Campus 1300 Morris Park Ave.
} Bronx, NY 10461 (718) 430-2890 Fax: 430-8996 URL:
} http://www.aecom.yu.edu/aif/
} **This electronic transmission contains information that is
} privileged.**
}
}

Joel B. Sheffield, Ph.D.
Biology Department, Temple University
1900 North 12th Street
Philadelphia, PA 19122
jbs-at-temple.edu
(215) 204 8839, fax (215) 204 0486
http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 15:00:32 2004

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Colin,

We agree with Sergey on his assessment concerning the difficulties of
coating with platinum.

We coat substrates with PT/IR wire and have a little better success. You
might also consider a tungsten/alumina crucible, perhaps a medium size.

John Arnott

Disclaimer: Ladd Research sells microscopy supplies and accessories,
including tungsten/alumina crucibles

Ladd Research
83 Holly Court
Williston, VT 05495

On-line Catalog: http://www.laddresearch.com

tel: 1-802-658-4961(anywhere) or 1-800-451-3406(US)
fax: 1-802-660-8859
e-mail: ladres-at-att.net

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 16:15:02 2004

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I often have a problem with ultrathin sections of non decalcified bone.
Regions of mineralized tissue have a lot of wrinkles and folds so that
the whole grids could be not usable. Regions of soft tissue on the same
sections are flat. What is the possible cause and how to avoid it?
Thank you,

Vladimir

Vladimir M. Dusevich, Ph.D.
Electron Microscope Lab Manager
3127 School of Dentistry
650 E. 25th Street
Kansas City, MO 64108-2784

Phone: (816) 235-2072
Fax: (816) 235-5524
Web: http://www.umkc.edu/dentistry/microscopy

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 18:34:10 2004

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Thank you very much to all of those who replied to my question on Pt
evaporation. It looks like we'll go down the path of sputtering, with
the help of a colleague nearby.

Cheers

Colin Veitch

Electron Microscopist

CSIRO Textile and Fibre Technology

PO Box 21, BELMONT, Vic. 3216. Australia.

E-mail: colin.veitch-at-csiro.au

Web: http://www.tft.csiro.au

Tel: +61 (0) 3 5246 4000
Mob: 0438 538 475
Fax: +61 (0) 3 5246 4811

The information contained in this e-mail message may be privileged or
confidential information. If you are not an intended recipient, you may
not copy, distribute or take any action in reliance on it. If you have
received this message in error, please telephone CSIRO Textile and Fibre
Technology on +61 3 5246 4000.

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 17 23:30:21 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Paul Gerroir wrote:
==========================================================
This matter was discussed some time ago so may be archived. I too have
observed "cracking" or "wrinkling" of the double-sided carbon adhesive which
makes for a very distracting background. I remember many microscopists
previously commented on this topic, however, I can't recall whether a
reliable solution to the problem was ever put forward.
==========================================================
The adhesive used for carbon tape and the die cut discs "ages" like any
pressure sensitive acrylic-based adhesive. As time goes on, two things seem
to be happening:

1. The bond between the adhesive and release paper seems to increase so
that when separated, the surface comes out somewhat mottled in appearance
and

2. The adhesive seems to lose some of its "tac" and when this happens, the
surface seems to become more sensitive to the beam.

We advise our customers to not purchase more than a year's requirements for
the best results. And if someone does end up with a large amount, we
advise heatsealing the tape/discs into a plastic polybag followed by
refrigerated storage.

Fresh tape and die cut discs should have a reasonably smooth surface and
should be reasonably resistant to cracking in the beam but it still can be
made to crack, given a high enough beam intensity.

So one might ask: Would an SEM lab be using "old" adhesives? And I can
assure you that the answer is a resounding "yes". I have had the personal
experience of visiting laboratories where the tape they were trying to use
was more than ten years old and they wondered why they were having problems
! Also tape left on a window ledge ,sitting in bright sunlight, will age
in a few months what would otherwise take some number of years.

So the point is, when comparisons are made, keep this in mind so that you
are comparing apples with apples. Do the comparisons with fresh tapes or
discs.

Disclaimer: SPI Supplies is a major supplier of double sided conductive
adhesive tapes, discs, and sheets so we have a major interest understanding
how these materials age. See URL
http://www.2spi.com/catalog/spec_prep/cond_adhes.html

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 00:51:04 2004

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Hello,

what you see seems to be chromatic aberration. Here is
some explanation from the Nikon pages
http://www.microscopyu.com/tutorials/java/aberrations/chromatic/

The focal length f varies with the wavelength of light
as illustrated in the tutorial window and Figure 1(a),
which demonstrates the effects of chromatic aberration
on a beam of white light passing through a simple lens.
The component colors (wavelengths) are focused at varying
distances from the lens (Figure 2) to produce an image
having an arbitrary blur radius approximately 0.3 millimeters
in diameter.

Blue light is refracted to the greatest extent followed
by green and red light, a phenomenon commonly referred
to as dispersion. The inability of a lens to bring all
of the colors into a common focus results in a slightly
different image size and focal point for each predominant
wavelength group. This leads to colored fringes surrounding
the image. When the focus is set for the middle of the
wavelength band, the image has a green cast with a halo of
purple (composed of a mixture of red and blue)surrounding it.

When you go to the link mentioned above you will find more
information about "chromatic aberration" as well as
interesting images which explain the result without many words.

The better the objectives are corrected the better the
result of your images with less chromatic aberration.

mfg / regards

Anneliese Schmaus
Product Manager

klughammer gmbh
Strassbach 9
85229 Markt Indersdorf
Germany
Tel. +49 08136 6011
Fax +49 08136 7098
info-at-klughammer.de
www.klughammer.de

JS} ------------------------------------------------------------------------------
JS} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
JS} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
JS} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
JS} -------------------------------------------------------------------------------

JS} I have wondered about this too, with other lenses. Do you think
JS} that there might be some wavelength dispersion in the specimen
JS} optical system (that is the sample, its mounting medium, the glass
JS} cover slip, and the oil)?

} }
} }
} } ----------------------------------------------------------------------
} } -------- The Microscopy ListServer -- Sponsor: The Microscopy Society
} } of America To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ----------------------------------------------------------------------
} } ---------
} }
} } I have a question about the focus precision at different wavelengths
} } using an Olympus 60X N.A. 1.4 Phase 3 objective.
} }
} } Has anybody noticed a difference in focal plane between images
} } collected at 465 to 490 nm and images collected at 530 to 560 nm?
} }
} } We thought we might be having a registration problem in our images of
} } CFP & YFP expressing cells. To confirm this, we looked at 0.1 um
} } Tetraspeck beads and 2.5 um beads with a broad 488 absorbing dye.
} } (BTW, the cells/beads are in 2X PBS, viewed through a 1.5 coverslip
} } and using Cargill Labs type DF oil.) In all the cases, the focal
} } shift appears to be between 0.3 and 0.5 um in Z.
} }
} } Just wondering if anybody else has seen this with the same type of
} } objective?
} }
} } Thanks.
} } ______________________________________________________________________
} } ______ Michael Cammer Analytical Imaging Facility Albert Einstein
} } Coll. of Med. Jack & Pearl Resnick Campus 1300 Morris Park Ave.
} } Bronx, NY 10461 (718) 430-2890 Fax: 430-8996 URL:
} } http://www.aecom.yu.edu/aif/
} } **This electronic transmission contains information that is
} } privileged.**
} }
} }

JS} Joel B. Sheffield, Ph.D.
JS} Biology Department, Temple University
JS} 1900 North 12th Street
JS} Philadelphia, PA 19122
JS} jbs-at-temple.edu
JS} (215) 204 8839, fax (215) 204 0486
JS} http://astro.temple.edu/~jbs

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 06:31:47 2004

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It has been brought to my attention that I may have implied that LEICA
service was not helpful to me. Please let me correct that
mis-impression by clearly stating that I received great help from one of
the engineers via phone call later that day, thus eliminating the need
for either field service or returning the instrument for repair. I am a
big fan of Leica products and have been very happy with their
instruments over the past 20 years.

Mary Ellen

} } } Mary Ellen Pease 11/17/04 07:58AM } } }
Hi all,

We have a 5 year old Leica KMR2 knifemaker that is in need of service.
The scoring wheel has been changed, but it appears that the clamp arm
and pressure swing arm are loose and thus insufficient clamping is
available to create a break. Apparently LEICA doesn't do field service
on knifemakers in our area and requires return to their shop for repair
as many of their techs have limited experience on this instrument. Is
there anyone else in the Maryland area who services these onsite and has
access to LEICA parts?

If anyone knows Pat Capagrossi, our former LKB, then LEICA service
engineer, tell her we miss her and her expertise!

Thanks,
Mary Ellen Pease

Mary Ellen Pease, M.S.
Laboratory Manager
Glaucoma Research Lab & Microscopy and Imaging Core Facility
Wilmer Eye Institute, Johns Hopkins Hospital
175 Woods Research
600 N. Wolfe Street
Baltimore, MD 21287
410-955-3337 (phone/voicemail)
443-287-2711 (fax)
mpease-at-jhmi.edu

WARNING: Email sent over the Internet is not secure. Information sent
by email may not remain confidential.
DISCLAIMER: This email is intended only for the individual to whom it
is addressed. It may be used only in accordance with applicable laws.
If you receive this email by mistake, notify the sender and destroy the
email.

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 08:15:10 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (m.serracino-at-igag.cnr.it) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, November 18, 2004 at 08:04:33
---------------------------------------------------------------------------

Email: m.serracino-at-igag.cnr.it
Name: marcello serracino

Organization: Institute of Environmental Geology and Geoengineering

Title-Subject: [Microscopy] [Filtered] Link exl computer graphics board

Question: Nestor:
Thank you very much for having set up this Listserver,
without it i could not have resolved my Exl problem, and
many many special thanks to you for your courtesy and
patience in helping to replace the board.

I want to add that, besides my specific problem,I really enjoy the listserver for the many advices, hints and infos i always find on it.

Marcello Serracino
Istituto di Geologia Ambientale e Geoingegneria - CNR
c/o Dipartimento di Scienze della Terra
Universita' "La Sapienza"
p.le A. Moro 5
00185 Roma
Italy

tel. +39 06.4991.4793
fax +39 06.446.8632
e-mail: marcello.serracino-at-igag.cnr.it

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From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 08:21:47 2004

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Dear Listservers,

I am pleased to announce that a vacancy for an Electron Microscopist
has arisen here at Johnson Matthey (Sonning Common, near Reading, U.K.).
The successful candidate will work in an extremely well equipped
department.

Please apply directly to Georgie Floyd (see address below).

Thank you for your attention.

Dr Gregory Goodlet
Electron Optics
Johnson Matthey Technology Centre

VACANCY

TECHNOLOGY CENTRE - SONNING COMMON (U.K.)

Electron Microscopist

Johnson Matthey PLC is a world leader in advanced materials technology.
The Technology Centre, based at Sonning Common, undertakes research
work for the group

A vacancy has arisen at the Technology Centre for an Electron
Microscopist to join our team working with both Scanning and
Transmission microscopes. The precise duties will depend on the
experience of the successful candidate but will include sample
preparation, microscopy work, interpretation, reporting and
collaboration with other project scientists. Some technique development
work will also be involved

The successful candidate will be educated to minimum HNC/Degree level
and should possess a sound knowledge of electron microscopy in materials
characterisation.

Applications must be made in writing with full CV and current salary
details to:
Georgie Floyd, Personnel Officer, Johnson Matthey Technology Centre,
Blounts Court, Sonning Common, Reading, RG4 9NH or e-mail
hrjmtc-at-matthey.com

Closing date for applications: Tuesday 30th November 2004

**********************************************************************************************
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From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 08:26:18 2004

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Hello !
Does anybody know if Spurr embedded biological material can be sectioned
with a Ralph knife for light microscopy (1-2 µm thick)? (Technical
handbooks usually relate Raplh knives only with metacrilate sections).
Thanks

Raúl Pozner
Instituto de Botánica Darwinion
CC 22, B1642HYD San Isidro
Buenos Aires - ARGENTINA
rpozner-at-darwin.edu.ar

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 17:11:30 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (sargenkn-at-westminster.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Thursday, November 18, 2004 at 13:32:50
---------------------------------------------------------------------------

Email: sargenkn-at-westminster.edu
Name: Kristen Sargent

Organization: Westminster College

Education: Undergraduate College

Location: New Wilmington, Pa 16172

Question: I am taking an electron microscopy course where we are in charge of creating our own project. My pet interest are Venus Flytraps, so I chose to work with that. I'm looking at the trap leaves and the spines. My probelm is identifying what I'm seeing. Are there any hints you can give me, or can you point me to some good sources for this.

Thankyou
Kristen Sargent

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 18 23:40:05 2004

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You could cut Spurr resin with glass knife. I don't think, the geometry of
knife is much important here. Sergey

At 06:47 AM 11/18/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 19 04:48:14 2004

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Dear All,
I was not successful in my first attemt (message sent on nov 11) to get
a response from the list. Is the low-temperature stage (LN2 cooled) for
JEOL 2010 UHR (with URP22 pole piece) available from GATAN only? I.e., is
this a proprietary item of Gatan?

Best regards
Satyam

} Message sent to the list on November 11, 2004

} Dear All,
} We would like to purchase one low-temperature stage (LN2 cooled) for
} our JEOL 2010 UHR (with URP 22 pole piece). I am aware of GATAN make and
} have contacts from them. I am wondering whether are there any other
} manufacturer who can supply low-temperature stage for our machine?
} Information may be given off-line also.
} Best regards
} Satyam

--
TEM Laboratory
Institute of Physics
Sachivalaya marg
Bhubaneswar - 751005
India
Fax:+91-674-230 0142
Tel:+91-674-230 1058 extn 124

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 19 05:11:14 2004

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Dear Kristen,

You could perhaps look at the research work published by the Heidelberg
botanist, Eberhard Schnepf, who did a lot of pioneering TEM work on
plant secretory cells (including Nepenthes, Drosera etc.) years ago. He
may also have described structures in the Venus Fly-trap.
Best wishes,

Jim

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:sargenkn-at-westminster.edu]
Sent: Friday, November 19, 2004 12:30 AM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (sargenkn-at-westminster.edu) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Thursday, November 18, 2004 at 13:32:50
------------------------------------------------------------------------
---

Email: sargenkn-at-westminster.edu
Name: Kristen Sargent

Organization: Westminster College

Education: Undergraduate College

Location: New Wilmington, Pa 16172

Question: I am taking an electron microscopy course where we are in
charge of creating our own project. My pet interest are Venus Flytraps,
so I chose to work with that. I'm looking at the trap leaves and the
spines. My probelm is identifying what I'm seeing. Are there any hints
you can give me, or can you point me to some good sources for this.

Thankyou
Kristen Sargent

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 19 06:23:08 2004

Contents Retrieved from Microscopy Listserver Archives
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I normally use an old Edwards 306A Coating unit with carbon rods to produce
support films. But have read that carbon fibre will give a much thinner
coating when compared to carbon string or cord. Therefore is it possible to
use carbon fibre to produce carbon support films for TEM using a carbon
attachment with a sputter coater?

many thanks

Kevin

------------

Kevin Mackenzie
Histology and EM Core Facility
Institute of Medical Sciences
University of Aberdeen
Foresterhill

k.s.mackenzie-at-abdn.ac.uk

01224 555822

www.abdn.ac.uk/ims/h-em

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 19 11:28:08 2004

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We purchased one from Oxford Instruments. The design was much different
than Gatan's, and did not use the hex-ring. It also had a much better
drift performance, but then Gatan bought Oxford Instruments holder
division, so now it is a Gatan.

John Mardinly
Intel

-----Original Message-----
} From: Incharge - TEM Laboratory [mailto:tem_iopb-at-iopb.res.in]
Sent: Friday, November 19, 2004 2:00 AM
To: Microscopy-at-microscopy.com
Cc: tem_iopb-at-iopb.res.in

Dear All,
I was not successful in my first attemt (message sent on nov 11) to
get
a response from the list. Is the low-temperature stage (LN2 cooled) for
JEOL 2010 UHR (with URP22 pole piece) available from GATAN only? I.e.,
is
this a proprietary item of Gatan?

Best regards
Satyam

} Message sent to the list on November 11, 2004

} Dear All,
} We would like to purchase one low-temperature stage (LN2 cooled) for

} our JEOL 2010 UHR (with URP 22 pole piece). I am aware of GATAN make
and
} have contacts from them. I am wondering whether are there any other
} manufacturer who can supply low-temperature stage for our machine?
} Information may be given off-line also.
} Best regards
} Satyam

--
TEM Laboratory
Institute of Physics
Sachivalaya marg
Bhubaneswar - 751005
India
Fax:+91-674-230 0142
Tel:+91-674-230 1058 extn 124

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 19 12:24:28 2004

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Short answer is yes, it can be done. But...you will have to experiment with
the formula (as with any thermoset resin). The goal is to make the final
hardness flexible enough to cut large areas at 2-3 microns thickness. I used
to work at an Eye Institute at the Univ of SoCal and the ocular pathologist
was very interested in embedding hemispherical cut human autopsy eyes in a
suitable plastic for whole sections containing pupil/optic nerve, hence the
name PO sections. We were able to do this successfully by altering the
ingredients in the Spurr formula and sectioning the eye as a whole mount on
a ralph glass knife. We chose Spurr resin because of its toughness under the
electron beam and low viscosity for infiltration through the sclera wall.
The idea here was to use the embedded sample for light microscopy histology
with routine H&E stains (another revised protocol), immunohisto and if
desired, selected areas for further study by TEM. It took some
experimenting with but we were successful in coming up with a soft enough
formula to allow the whole sectioning for histo and still use the block for
TEM. The big tradeoff was thin sectioning for TEM. The formula tended to be
too soft for 80-90nm sections but was doable with patience and practice.
Sections from what I remember did have a some compression issues. I imagine
if you could cryo the sample at say -60C, you would be more successful with
regard to sectioning artifact.

Good luck

Fred Hayes
Ann Arbor MI
----- Original Message -----
} From: "Raúl Pozner" {rpozner-at-darwin.edu.ar}
To: {Microscopy-at-microscopy.com}
Sent: Thursday, November 18, 2004 9:47 AM

Hi All,
We have an old "Fume-Gard" portable hood in our lab that we use for
slide staining. Lerner Labs (the manufacturer) seems to be defunct.
We need to replace the vapor absorbent (activated carbon?) filter
pack for it. The old cat. # is 906. The filter pack measures 11.25
long x 5.75 high and 1 3/8 deep (all inches).
does anyone have an idea where an equivalent filter can be found?
Our Office of Environmental Safety is having puppies over how old
this filter is!
Thanks,
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 19 21:03:50 2004

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I'm an artist seeking to buy an ElectroImage/Tetracam TriPix RGB
microscope camera in any condition, as long as it's functioing properly.
Used would be ideal.
Camera is a small blue case with "TRIPIX" in white, lens mount is C
mount- may have a
lens on it but it's a microscope camera. There are three models- I only
seek the RGB model.
Any ideas, leads would be most appreciated.
Thanks all.

John Lovell
--
John Lovell
j_lloyd-at-letterboxes.org

From MicroscopyL-request-at-ns.microscopy.com Sat Nov 20 08:02:50 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (padmashree-at-excite.com) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Saturday, November 20, 2004 at 06:42:59
---------------------------------------------------------------------------

Email: padmashree-at-excite.com
Name: Rajesh

Organization: Shenoy

Education: Graduate College

Location: Bangalore, Karnataka, India

Question: Sir/madam,
we have a sony DSC 717 digital camera and we have also have a suitable adapter for it to be fixed to the microscope we are not able to get sharp images of the stained histology sections, kindly let me know as to what settings should be kept for such camera to take images from a binocular microscope.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Nov 20 14:09:05 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Kevin Mackenzie wrote:
==============================================================
I normally use an old Edwards 306A Coating unit with carbon rods to produce
support films. But have read that carbon fibre will give a much thinner
coating when compared to carbon string or cord. Therefore is it possible to
use carbon fibre to produce carbon support films for TEM using a carbon
attachment with a sputter coater?
==============================================================
Two things:

1. I have never heard of an instance where a "carbon attachment" to
anyone's sputter coater (with a rotary vane pump) could be used to make
carbon films of an acceptable quality such that they could be used as TEM
support films. Carbon films meeting the standard for TEM support films have
to be made in a diffusion pump or better pumped system, done in a vacuum
evaporator.

2. The terms, carbon "string", "cord", "thread" and "fiber" seem to have
developed their own meanings in different markets and sometimes the same
word means different things in different markets.

At one time there were two diameters, "thick" and "thin". The "thick"
material was called carbon "fiber" in North America and "braid" in most of
Europe. In some countries it was called "cord". This was typically
material that was about 2 mm diameter.

The "thin" material, which typically had a diameter closer to 1 mm, was
called "string" in North America and "thread" in Europe.

Many people now use these terms all interchangeably without regard to this
history of the terms. So when communicating it is always going to be better
to talk in terms of "carbon fiber diameter" and possibly also, the origin
(brand) of the carbon fiber being described. For further information see
URL
http://www.2spi.com/catalog/spec_prep/carbon-fiber.shtml

Carbon fiber does not all come from the same place.

Disclaimer: SPI Supplies is one of the main manufacturers of high purity
carbon fiber of all diameters so we have a vested interest in making sure
that product is described in an unambiguous way.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 09:43:21 2004

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Hi,

We have an operating Hitachi S520 SEM that is no longer
required and will be disposed of in the coming months. If
anyone has an interest in this machine please let me know.

Regards,
Ron
----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 13:27:43 2004

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On Nov 15, 2004, at 4:16 PM, by way of MicroscopyListserver wrote:

}
} Email: ptibbits-at-emerson-ept.com
} Name: Patrick Tibbits
}
} Organization: Emerson Power Transmission
}
} Title-Subject: [Microscopy] [Filtered] MListserver:
}
} Question: Dear Microscopists,
}
} I'm seeing that blue-green powder again on the bottom of my Haskris
} chiller tank. Previous discussions on this list identified it as a
} corrosion product from the Copper coolant lines.
}
} Can anyone suggest a corrosion inhibitor?
}
} I run 10% ethylene glycol in distilled water. The closed-loop Haskris
} chiller maintains about 68 degrees F, 14 psi.
}
} Patrick
}
Dear Patrick,
On the East Coast, we used AquaTreet 42 from Aqua Laboratories; on the
West Coast, we are using TST303 from Skasol, Inc. Both are
molybdenum-based and work very well. Call the appropriate company for
your location to get more info. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 13:40:57 2004

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Responses for: Low temp stage for JEOL 2010

Dear friends
This time, I have got good suggestions (many of them were written
privately). Thanks for your help.
Best regards
Satyam
} -------------------------------------------------------------------------
-----
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------
------
}
} Dear All,
} I was not successful in my first attemt (message sent on nov 11) to
} get
} a response from the list. Is the low-temperature stage (LN2 cooled) for
} JEOL 2010 UHR (with URP22 pole piece) available from GATAN only? I.e.,
} is this a proprietary item of Gatan?
}
} Best regards
} Satyam
}
}
} } Message sent to the list on November 11, 2004
}
} } Dear All,
} } We would like to purchase one low-temperature stage (LN2 cooled) for
} }
} } our JEOL 2010 UHR (with URP 22 pole piece). I am aware of GATAN make
} } and have contacts from them. I am wondering whether are there any
} } other manufacturer who can supply low-temperature stage for our
} } machine? Information may be given off-line also.
} } Best regards
} } Satyam
}
} --
} TEM Laboratory
} Institute of Physics
} Sachivalaya marg
} Bhubaneswar - 751005
} India
} Fax:+91-674-230 0142
} Tel:+91-674-230 1058 extn 124

--
TEM Laboratory
Institute of Physics
Sachivalaya marg
Bhubaneswar - 751005
India
Fax:+91-674-230 0142
Tel:+91-674-230 1058 extn 124

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 14:06:48 2004

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}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Gatan currently still make both the 'Oxford' CT3500 and 'Gatan' Model
626 Cryotransfer version.

I am not aware of any other supplier of TEM cold/cryotransfer holders
although it might be worth contacting Fischione.

--
Larry Stoter
JEOL (UK) Ltd
tel: +44-(0)1707-377117, fax: +44-(0)1707-373254, e-mail: larrys-at-jeoleuro.com

PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 15:34:26 2004

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Dear listers,

I have a question concerning etching metals in a failure analysis lab. We
have an oxford ICP etcher that we normally run fluorine based chemistries
in. We are considering the advantages of running chlorine gas as well. Will
running the two chemistries (at different times) be problematic as far as
change over? The etcher is not used for production or manufacturing, but
only for Failure analysis. What are the recommendations for trying to run a
system in this manner.
Thanks for your time
Nick

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 18:57:49 2004

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Nicol;

You may want to query the manufacturer of the system. Chlorine, as you
may know, is very corrosive. There may also be some guidance from
people that use gas assisted FIB's.

If I may ask, what metals are you trying to etch and is there a problem
with wet chemistry?

Regards,
Peter Tomic
Agere Systems
Allentown, PA

-----Original Message-----
} From: Nicol Aitken [mailto:nicol-at-semiconductor.com]
Sent: Monday, November 22, 2004 4:57 PM
To: microscopy-at-msa.microscopy.com

Dear listers,

I have a question concerning etching metals in a failure analysis lab.
We have an oxford ICP etcher that we normally run fluorine based
chemistries in. We are considering the advantages of running chlorine
gas as well. Will running the two chemistries (at different times) be
problematic as far as change over? The etcher is not used for production
or manufacturing, but only for Failure analysis. What are the
recommendations for trying to run a system in this manner. Thanks for
your time Nick

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 22 21:24:28 2004

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Charles, great response!
The only thing I want to add is that best way to produce the carbon film is
to do so in oil-free high vacuum (2*10-6 torr) with electron gun. Mica
should be highest quality as well (natural one without oil). Sergey

At 12:27 PM 11/20/2004, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

_____________________________________

Sergey Ryazantsev Ph. D.
Electron Microscopy
UCLA School of Medicine
Department of Biological Chemistry
10833 Le Conte Ave, Room 33-080
Los Angeles, CA 90095

Phone: (310) 825-1144 (office)
(310) 206-1029 (Lab)
FAX (departmental): (310) 206-5272
mailto:sryazant-at-ucla.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 06:40:44 2004

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I'm looking for additional information and experience from the microscopy
community. I am quickly moving towards installing a basic EDS detector on
my Phillips 400 TEM. I have no intention of installing the STEM or other
electron detectors for imaging. My limited understanding is I should be
able to collect element information about my sample. My grid holder has a
beryllium insert to hold the grid and I anticipate needing to use beryllium
grids or get use to copper peaks.

what am I missing?

Do Be grids require special disposal? I know the overall count rate will
be low, but are their problems or factors I should be aware of? I am
especially concern that the installation of the EDS probe will not
significantly degrade my image (I typically work under 100KX) .

Any thoughts and suggestions would be welcome!

Season greetings to all..............

Frank Karl
Degussa Corporation
Akron Technical Center
3500 Embassy Parkway
Suite 100
Akron, Ohio 44333

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 07:20:01 2004

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Tuesday 11 January 2005
University of Oxford, Department of Materials
A one-day meeting organised by the Royal Microscopical Society (RMS)
Organisers: Dr Angus Kirkland and Dr Crispin Hetherington

The arrival of aberration correctors for transmission electron microscopes and the recent developments in exit-wave restoration have highlighted the importance of quantitative imaging. However, the factors causing the mismatch between experimental and simulated images are still poorly understood. This conference will address experimental techniques and theories available for obtaining quantitative structural information from images, holograms and diffraction patterns.
The programme will include the following speakers:
Professor Henny Zandbergen, Delft University of Technology, The Netherlands
Professor Hannes Lichte, Dresden University, Germany
Professor Dirk Van Dyck, University of Antwerp, Belgium
Professor Laurence Marks, North Western University, Chicago

The organisers are also planning to hold an informal discussion workshop on the following day, Wednesday 12th January 2005, to which delegates are invited.

Registrants are invited to submit abstracts for consideration as oral presentations. A maximum of 300 words, to be emailed to Victoria at the RMS office. The abstract deadline is Friday 10th December 2004.

Further information can be obtained from:
Royal Microscopical Society, 37/38 St Clements, Oxford OX4 1AJ, UK
Tel: + 44 (0) 1865 248 768, Fax: + 44 (0) 1865 791237
victoria-at-rms.org.uk
You can also register online at www.rms.org.uk

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 08:49:58 2004

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EDS in the EM 400 without a STEM unit.

There should be no problem doing this but there are some points to look
out for. The EM 400 was built at a time when EDS was still quite new
and it is not as fully optimized for EDS as a newer microscope would be.
In particular the EDS spectrum is likely to have spurious peaks,
corresponding to electrons and x-rays generating a signal from areas far
from where you think the beam is hitting.

First you should check the apertures you have installed. Both the fixed
apertures as well as the alignable apertures. You should talk to a
Philips (FEI) service engineer and consider changing the fixed apertures
for a set designed to improve the EDS signal and you should start using
"top hat" apertures in the aperture holders.

Even if you do a good job of cleaning up the beam in this way, you will
find that you still have a rather high set of systems peaks, if you
operate the microscope in the normal way (which Philips call
microprobe). You will get better data if you go to the configuration
used for STEM (Philips call it nanoprobe), which you can do even if you
have no STEM unit. There is a little switch to the left of the column,
next to the "Intensity" knob.

The problem with this is that, when you go to nanoprobe, you have to
realign the microscope. With this system the advantage of having a STEM
unit (even if you have no STEM detectors and have no intention of ever
making a STEM image) is that you can leave the microprobe alignment on
the microscope and leave the nanoprobe alignment on the STEM unit, and
hence switch easily between them. It would be worth your while to try
to pick up a second hand STEM unit for this purpose. As STEM units they
were not very useful, so they should be cheap.

Frank.Karl-at-degussa.com wrote:

}
} ------------------------------------------------------------------------------
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}
}
}
}
} I'm looking for additional information and experience from the microscopy
} community. I am quickly moving towards installing a basic EDS detector on
} my Phillips 400 TEM. I have no intention of installing the STEM or other
} electron detectors for imaging. My limited understanding is I should be
} able to collect element information about my sample. My grid holder has a
} beryllium insert to hold the grid and I anticipate needing to use beryllium
} grids or get use to copper peaks.
}
} what am I missing?
}
} Do Be grids require special disposal? I know the overall count rate will
} be low, but are their problems or factors I should be aware of? I am
} especially concern that the installation of the EDS probe will not
} significantly degrade my image (I typically work under 100KX) .
}
} Any thoughts and suggestions would be welcome!
}
} Season greetings to all..............
}
} Frank Karl
} Degussa Corporation
} Akron Technical Center
} 3500 Embassy Parkway
} Suite 100
} Akron, Ohio 44333
}

--
..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 09:31:01 2004

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Dear Listers,

I'm checking with the collective microscopy mind for favorite techniques
of using LR White for embedding cell culture layers. What we want to do
is use the "pop-off" technique of snapping the cover slip off the end of
a resin block after immersion in liquid nitrogen. For regular
ultrastructure work this is by far the easiest and most relliable method
I've tried, but it's been a problem with immuno samples.

We are experimenting somewhat successfully with using flat molds with
circular cover slips on the top, covered in turn with large rectangular
coverslips to seal out the oxygen. Our next tests will be with
polymerization chambers filled with nitrogen, argon, or some gas other
than pesky oxygen.

If anyone has any pet techniques for this they might be willing to
share, I'd love to hear them. This has been a recurring problem for us
and we seem to be getting more cell cultures for immuno work all the
time. I'd be happy to share the results of our tests, as well.

Finally, on an entirely different note, we have an office pool going on
whether or not a set of car keys with a remote door/window/etc. opener
will function after having been flushed down a toilet, rescued, and
subjected to a bleach bath for 24 hours. I say no, and lab-mate Cheryl
says yes (after putting in a new battery). Before investing a whole
buck in this, I need opinions.

Happy Thanksgiving!

Randy

Randy Tindall
EM Specialist {/}
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu {http://www.emc.missouri.edu/}

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 10:06:22 2004

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Dear All,

I am trying to preparing TEM specimen from the micrometer Ta powders, here
is my procedure

"The powder was mixed with Gatan G1 epoxy resin in a Teflon cup and then
the mixture was transferred to a Cu tube with a diameter of 3 mm. After
curing at 373 K the tube was sliced into a series of 500 micrometer thick
discs using a low speed diamond saw, Finally, the discs were mechanically
ground to a thickness of 20 micrometer prior to ion thinning to electron
microscopy transparency in the PIPS. As I tried to polish it thinner, the
particles started to pull out.
"PIPS operating conditions were: acceleration voltage of the ion gun 3.4
keV, rotation frequency 3 rpm, and incidence angle of the two ion beams on
both sides of the sample 3-4 deg.

Due to the different milling rate between G1 epoxy and Ta particle, I got
very few particles electron transparent. my questions are

1. If anyone had experience on embedding particles on different matrixes
(such as Al, Ag), please give me some advices

2. Since I was using low angle and low voltage to mill the specimen, I got
redeposition from the Cu grid, how to avoid the redeposition at low angle
milling?

Any advice on the sample prep. of this material would be greatly appreciated.

Thanks a lot

Jinguo Wang

Jinguo Wang, Ph.D
The Pennsylvania State University
Materials Research Institute
194 Materials Research Institute Building
University Park, PA 16802
Tel: (814) 865-9285
Fax: (814) 863-8561, 814) 863-0637
Email: jqw11-at-psu.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 13:21:20 2004

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A lot of unspecified variables here, Randy. Seems to me you need more
practice getting
your experiments peer-reviewed. How many replicates? Has the toilet
been, like, used? And
what is the recovery mode? Fishing them out of the sewage treatment
plant could take a little time.
The concentration of the bleach? And what make is the car? I'm willing
to bet that a set from a
Mercedes S-class would survive that, no problem. Don't know about Ford
though.

Best wishes
Chris

Dr. Chris Jeffree

----- Original Message -----
} From: "Tindall, Randy D." {TindallR-at-missouri.edu}
To: {microscopy-at-msa.microscopy.com}
Sent: Tuesday, November 23, 2004 3:52 PM

hey randy, it's only a buck US. it's not like it's real money.

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Work Phone: 204-789-3313
Pager: 204-931-954
Home Phone: 204-489-6924
Cell: 204-781-1502
Fax: 204-789-3926/204-489-6924

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 18:23:37 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (bert.reuss-at-tufts.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, November 23, 2004 at 12:46:03
---------------------------------------------------------------------------

Email: bert.reuss-at-tufts.edu
Name: Bert Reuss

Organization: Tufts University Geology Department

Title-Subject: [Microscopy] [Filtered] MListserver:Cambridge 100S parts available

Question: We have a non-functional 1985 Cambridge 100S SEM that is
available for parts. We have no means of shipping this
unit so you should be willing to pick it up at our Medford, MA
campus. The SEM was operational until last April but was shut
down because of problems with the scans, stage, and roughing pump.

Please contact off-line:

Bert Reuss email bert.reuss-at-tufts.edu
Geology Department
Medford, MA 02155

617-627-3494

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From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 21:33:01 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (henry-at-cmsp.com) from http://microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, November 23, 2004 at 09:29:33
---------------------------------------------------------------------------

Email: henry-at-cmsp.com
Name: Henry Schleichkorn

Organization: Educational Pictures

Education: 6-8th Grade Middle School

Location: Chicago, Illinois USA

Question: Hello,
I am looking for old EM prints and negatives that EM Departments want to discard. I'll pay for shipping expenses. SEMs, EM, TEM, etc. I'll take boxes, binders, files, whatever. Thanks, Henry 773-267-3100
henry-at-cmsp.com

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 23 23:23:43 2004

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Randy,
Regarding the LR White question: I had great success with completely
filled flat bottom BEEM capsules and also with a small vacuum oven that
I flushed with nitrogen gas and pumped down 3 times then left pumped
down overnight at 60 degrees. I polymerized lots of material in open
dishes that way.

Regarding the remote opener: I successfully revived mine after doing a
wet exit from a kayak with my keys on my belt. It was fun watching the
car lock and unlock itself while the remote was drying out at the other
side of the house. I opened it and washed it with clean water then
allowed it to dry and all was well. I never dried bleaching it, though.
Good luck.

Kim
{} {} {} {} {} {} {} {} {} {}
Kim Rensing PhD
Research Associate
Wood Science, UBC
2424 Main Mall
Vancouver BC, Canada
V6T 1Z4
{} {} {} {} {} {} {} {} {} {}

On 23-Nov-04, at 7:52 AM, Tindall, Randy D. wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} Dear Listers,
}
} I'm checking with the collective microscopy mind for favorite
} techniques
} of using LR White for embedding cell culture layers. What we want to
} do
} is use the "pop-off" technique of snapping the cover slip off the end
} of
} a resin block after immersion in liquid nitrogen. For regular
} ultrastructure work this is by far the easiest and most relliable
} method
} I've tried, but it's been a problem with immuno samples.
}
} We are experimenting somewhat successfully with using flat molds with
} circular cover slips on the top, covered in turn with large rectangular
} coverslips to seal out the oxygen. Our next tests will be with
} polymerization chambers filled with nitrogen, argon, or some gas other
} than pesky oxygen.
}
} If anyone has any pet techniques for this they might be willing to
} share, I'd love to hear them. This has been a recurring problem for us
} and we seem to be getting more cell cultures for immuno work all the
} time. I'd be happy to share the results of our tests, as well.
}
} Finally, on an entirely different note, we have an office pool going on
} whether or not a set of car keys with a remote door/window/etc. opener
} will function after having been flushed down a toilet, rescued, and
} subjected to a bleach bath for 24 hours. I say no, and lab-mate Cheryl
} says yes (after putting in a new battery). Before investing a whole
} buck in this, I need opinions.
}
} Happy Thanksgiving!
}
} Randy

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 24 04:58:01 2004

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About the car key problem - my own experience is that if you go
swimming in salt water with the keys to your new Saab in your bathing suit
pocket, you won't be able to disable the alarm later and your car won't
start, no matter what you do. Boy, did I find that out the hard way....

Frank

F.C. Thomas
FThomas-at-NRCan.gc.ca, 902-426-4635, facsimile 902-426-6152
GSC Atlantic
Natural Resources Canada, Bedford Institute of Oceanography,
P.O. Box 1006, Dartmouth, Nova Scotia B2Y 4A2
Ressources naturelles Canada, l'Institut Oceanographique du Bedford, B.P.
1006, Dartmouth, (Nouvelle-Ecosse)
B2Y 4A2
Government of Canada/Gouvernement du Canada

-----Original Message-----
} From: Chris Jeffree [mailto:c.jeffree-at-ed.ac.uk]
Sent: Tuesday, November 23, 2004 3:42 PM
To: Tindall, Randy D.
Cc: microscopy-at-msa.microscopy.com

Could anyone please tell me a ** simple ** way to estimate the thickness of
sputtered gold, for example by light or IR absorbance of a film on glass?
All my searches so far have turned up apparatus like the Hummer thickness
monitor.

-----------------------------------
Robert H. Olley
Reply to: R.H.Olley-at-reading.ac.uk
URL: http://www.rdg.ac.uk/~spsolley
-----------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 24 12:43:23 2004

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A simple method is to use a color spectrophotometer in a transmission or reflectance mode and use thin film modeling techniques. See any book on spectrophotometry of thin films or ellipsometry. There are commercial thin film programs available. Two that I am familiar with are TFCalc and FilmStar. You can also write your own. The principles are straightforward and you can implement them even in Excel. The optical properties of gold, n and k, as a function of wavelength are well known and can easily be found.

You might want to try to get your hands on some back issues of Vacuum Technology and Coatings. Peter Martin from Pacific Northwest National Laboratories has a regular series in it and he had one on optical coatings and how they are characterized. The basics were covered in his articles. Sorry, I do not hve the issue numbers, but you might want to either contact the editor or Peter directly.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Robert H. Olley [mailto:hinmeigeng-at-hotmail.com]
Sent: Wednesday, November 24, 2004 8:59 AM
To: microscopy-at-microscopy.com

Could anyone please tell me a ** simple ** way to estimate the thickness of
sputtered gold, for example by light or IR absorbance of a film on glass?
All my searches so far have turned up apparatus like the Hummer thickness
monitor.

-----------------------------------
Robert H. Olley
Reply to: R.H.Olley-at-reading.ac.uk
URL: http://www.rdg.ac.uk/~spsolley
-----------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 24 12:56:55 2004

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We used AFM to measure the thickness of sputtered coatings.

========================
Evgenia Pekarskaya
Keck Electron Microscopy Laboratory
University of Massachusetts, Amherst
Tel. 413 545 2261
E-fax 325 202 7338
http://www.umassmicroscopy.com/
========================

-----Original Message-----
} From: Robert H. Olley (by way of MicroscopyListserver)
[mailto:hinmeigeng-at-hotmail.com]
Sent: Wednesday, November 24, 2004 8:59 AM
To: microscopy-at-microscopy.com

Could anyone please tell me a ** simple ** way to estimate the thickness
of
sputtered gold, for example by light or IR absorbance of a film on glass?
All my searches so far have turned up apparatus like the Hummer thickness
monitor.

-----------------------------------
Robert H. Olley
Reply to: R.H.Olley-at-reading.ac.uk
URL: http://www.rdg.ac.uk/~spsolley
-----------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 24 14:22:25 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Although now working for JEOL, I used to work for Philips and know
the EM400 series fairly well ...

You don't say if this is a new or used EDS detector but absolutely
critical to successful operation of the EDS is the right collimator.
This must have been designed to work with your specific model of 400
and EDS detector. Otherwise, any data will probably be useless.

The collimator should also have some sort of electron trap or shield.
In the main mag ranges, the field of the objective lens completely
contains the electrons coming down the column. When you go into the
low mag range, the objective lens goes to a very low current. You can
then get significant scattering of primary electrons into the ED
detector - this will, in the short term swamp the detector which will
then take some time to recover. Longer exposure or repeated
short-term exposure will trash the Si(Li) crystal. Some collimators
have a mechanical shutter which uses the objective field to open and
close it. Permanent magnet systems have also been used. Of course,
you can physically retract the detector if you are going to go into
low mag mode but that is a bit of a pain.

You can do a lot of useful EDS with Cu or Al grids but don't forget
Cu has low-energy L lines. I never used Be grids - principally
because of cost, which also meant that throwing them away wasn't an
issue since they had to be recycled! I'm sure there are now health
and safety regulations but I doubt that disposing of such small
amount of metalic Be is a real problem.

Check your condenser apertures - although a matter for debate, I
always used 'top-hat' apertures. These have a thick section around
the hole and reduce X-rays coming down the column which may result in
misleading spectra or spurious peaks.

Don't forget - you can only do decent ED analysis with the object
aperture 'out' otherwise BS electrons from the objective aperture
also hit the sample and completely mess up the spectra.

There should be an adjustable 'bar' which goes under the ED dewar and
braces it against the main frame of the TEM. There is a threaded
collar to adjust which should be set fairly tight. Depending on the
age of your 400, there may or may not be a hole in the panelling,
just to the left of the column for the lower end of this bar to pass
through, to brace against the frame. If this bar is not used, you
'may' get vibration problems affecting the image at higher
magnification.

Also be aware that any build up of water ice in the dewar might also
cause sufficient noise to cause problems with both the ED spectra and
the TEM image.

Hope that is useful.
--
Larry Stoter
JEOL (UK) Ltd
tel: +44-(0)1707-377117, fax: +44-(0)1707-373254, e-mail: larrys-at-jeoleuro.com

PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Wed Nov 24 17:22:55 2004

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Dear Robert,
I always told my students who wanted to know the thickness of the sputtered
gold to weight the glass piece before and after deposition and work it out.
That usually convinced them that they didn't really need to know. Most times
I just tell them what I think it is, about ten nanometers; who's to say it
isn't right. I used to have a chart from Hummer with a curve showing the
thickness of deposition vs. time for a specified voltage and current.
Good luck,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Robert H. Olley (by way of MicroscopyListserver)"
{hinmeigeng-at-hotmail.com}
To: {microscopy-at-microscopy.com}
Sent: Wednesday, November 24, 2004 5:59 AM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (wqsm-at-hotmail.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, November 24, 2004 at 16:20:14
---------------------------------------------------------------------------

Email: wqsm-at-hotmail.com
Name: Ming

Organization: University of Alberta

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I wanna stain the ultrathin HDPE sample(after section) using RuO4 vapour. Could anyone give me some idear about the suitable stain time?
Thans!

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From MicroscopyL-request-at-ns.microscopy.com Wed Nov 24 21:13:05 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (wall1-at-llnl.gov) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, November 24, 2004 at 16:45:37
---------------------------------------------------------------------------

Email: wall1-at-llnl.gov
Name: Mark Wall

Organization: LLNL

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for software that will create a single in-focus image (tiff image files) from a series of images that are taken at different (known) focus settings/heights. The application is for imaging metallography samples that are not very flat or have considerable roughness to them.

An additional bonus for us is to be able to have a 3-D plot of the surface topography as well.

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From MicroscopyL-request-at-ns.microscopy.com Thu Nov 25 05:10:56 2004

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Dear listers,

I would like to know if somebody has experienced high
amplitude low frequency noise in tapping mode and
hence no images. Whereas in contact mode images are
okay if we lower the gains.
Shashi Singh
Hyderabad
India

__________________________________
Do you Yahoo!?
Meet the all-new My Yahoo! - Try it today!
http://my.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Thu Nov 25 12:28:02 2004

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Please check out our website
(http://www.soft-imaging.com/rd/english/416.htm) for our EFI (Extended Focal
Imaging). It does precisely what you are looking for. If you need further
information, please contact me by email or call me.

Thanks.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: wall1-at-llnl.gov [mailto:wall1-at-llnl.gov]
Sent: Wednesday, November 24, 2004 20:35
To: microscopy-at-microscopy.com

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Please check out our website
(http://www.soft-imaging.com/rd/english/416.htm) for our EFI (Extended Focal
Imaging). It does precisely what you are looking for. If you need further
information, please contact me by email or call me.

Thanks.

Mike

Michael Bode, Ph.D.
Soft Imaging System Corp.
12596 West Bayaud Avenue
Suite 300
Lakewood, CO 80228
===================================
phone: (888) FIND SIS
(303) 234-9270
fax: (303) 234-9271
email: mailto:info-at-soft-imaging.com
web: http://www.soft-imaging.com
===================================

-----Original Message-----
} From: wall1-at-llnl.gov [mailto:wall1-at-llnl.gov]
Sent: Wednesday, November 24, 2004 20:35
To: microscopy-at-microscopy.com

There have been a number of requests, including from Nestor but ...

{Rant mode on :-))

IF YOU ARE NOT COLLECTING YOUR E-MAIL, UNSUBSCRIBE FROM THE LIST.

DO NOT JUST SET UP AN 'OUT OF OFFICE' AUTO REPLY.

OTHERWISE ANYBODY POSTING TO THE LIST GETS DELUGED WITH 'OUT OF
OFFICE AUTO REPLIES'.

(because the default reply address for the list is the originator)

To such an extent, that I am tempted to not only not post to the list
anymore but permanently unsubscribe.

IF ANY SUBSCRIBERS CAN'T UNDERSTAND THIS, PLEASE CONTACT ME AND I
WILL TRY TO EXPLAIN EVEN MORE SIMPLY.

{Rant Mode Off :-))

Thank you,
--
Larry Stoter
PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 26 10:00:38 2004

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Hi-

This is my first post to the Microscopy list and it concerns an image
processing problem that I need help with. I am looking
at cell-size and morphology in an epithelial cell-structure. To help
illustrate my problem I have put some images on a webpage and I will
be referring to those images below:
{http://www.homepages.ucl.ac.uk/~smgxro1/page1.html}

The cell-structure is imaged with a fluorescent Microscope at 40x. To
determine the individual cell size I look at a region-of-interest
(ROI) in the Frequency domain where the peak spatial frequency can
easily be converted into the average cell-size (top-right corner of
image 4 and 5). The tissue sample is around 5 cm square and it is
quite a delicate process to prepare and flat-mount it (image 1). To
get the Fourier transform to register a distinct peak frequency I use
the
following pre-processing steps (results can be seen on the left of
image 4 and 5):
1) Blind deconvolution - to improve image resolution and compensate
for out-of-focus areas of the flat-mounted tissue.
2) Uniform local histogram equalisation (CLAHE) - to optimally enhance
image contrast.
3) Gaussian low-pass filtering - to eliminate low-frequency changes
(due to uneven illumination, tissue thickness etc.).

Once I have the peak frequency of a given ROI and I know the image
px/µm ratio I can derive the mean cell-size. Finally, I plot the mean
cell-size and the standard deviation against the distance from the
centre of the tissue (the cell-size increases with distance from
centre). In the centre of the tissue the cells are tightly packed in a
hexagonal lattice, which makes it ideal for an isotropic Fourier
analysis (image 2 and 4). However, towards the extreme periphery
several morphological changes take place: The cell shapes becomes
severely deformed, the cell contents change (and hence, the pixel
brightness, edge gradients etc.) and none-RPE cells are mixed into the
lattice. Image 3 illustrates but one of countless and random cell
configurations and as a consequence the frequency spectra becomes even
harder to evaluate (top-right of image 5).

These are my two questions:
1) How can I improve on the pre-processing of the microscopic images
to enhance the cell-walls, or edges and eliminate other non-continues
cell artefacts?
2) The mean cell size and it's standard deviation give a very accurate
measurement of the central and highly regular lattice, but when the
cell structure becomes more irregular, it is less meaningful. Are
there better spatial descriptors - and methods to measure them - for
the random cell shapes that I encounter at the periphery of the
tissue?

Thanks!

-Peter
--
Peter Lundh
E: peter.lundh-at-ucl.ac.uk
T: +44 (0) 207-608 4049
M: +44 (0) 788-195 2645
F: +44 (0) 207-608 6909

Visual Science Department
Institute of Ophthalmology
11 - 43 Bath Street
EC1V 9EL London

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 26 14:22:55 2004

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Good Afternoon,
I have samples that when viewed by reflected light have an undulating
surface with fine texture on both the high and low areas. I would like
to quantify areas of the sample according to texture. Any suggestions
how this might be done? Is there software available for such an
application?

Thanks,
Paul

Paul J. Gerroir
Microscopy
Materials Characterization
Xerox Research Centre of Canada
2660 Speakman Drive
Mississauga, Ontario L5K 2L1

Phone: 905-823-7091, ext.216
FAX: 905-822-7022
e-mail: paul.gerroir-at-xrcc.xeroxlabs.com

From MicroscopyL-request-at-ns.microscopy.com Fri Nov 26 15:27:36 2004

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In a message dated 11/26/04 4:38:38 PM, paul.gerroir-at-xrcc.xeroxlabs.com
writes:

} I have samples that when viewed by reflected light have an undulating
} surface with fine texture on both the high and low areas. I would like
} to quantify areas of the sample according to texture. Any suggestions
} how this might be done? Is there software available for such an
} application?

There are quite a few ways to convert textural differences to brightness
differences that can be used to threshold the image for measurement of areas. Most
image processing programs include at least things like the calculating the
variance of a neighborhood centered on each pixel, or the range between the
brightest and darkest pixel. Also useful is the local neighborhood entropy, the
loca fractal dimension, etc. If you can either mail me an example image or the
address of an ftp site to get it, I will see which of the routines in Fovea Pro
work best for your particular images.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Sat Nov 27 12:17:31 2004

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Our Extended Dept of Focus provides not only the in-focus image, but also
the anaglyph image, and the 3D surface plot. Please visit our web:

http://www.laboratory-imaging.com/index.php?lang=en&inc=3DFocus

If you would like to get more detailed information please contact me.

Regards,

Josef Mikes
Laboratory Imaging, s.r.o.
Prague, Czech Republic
Tel: +420 272 081 400
Fax: 420 271 732 657
E-mail: josef.mikes-at-lim.cz
Web: www.laboratory-imaging.com

Please check out our website
(http://www.soft-imaging.com/rd/english/416.htm) for our EFI (Extended Focal
Imaging). It does precisely what you are looking for. If you need further
information, please contact me by email or call me.

Thanks.

Mike

----- Original Message -----
} From: "by way of MicroscopyListserver" {wall1-at-llnl.gov}
To: {microscopy-at-microscopy.com}
Sent: Thursday, November 25, 2004 4:34 AM

Some time ago, wishing to break the instant film photography stranglehold
on microscopy, I purchased a Kodak MDS100 digital camera on eBay. The
camera has been working quite well, but I recently made a discovery (for
myself, at least) that a blue filter dramatically improved its image quality.
My original application, on an Olympus SZH stereomicroscope, does not
permit the practical recording of images with a blue filter because of the
dramatic reduction in transmitted light, but the Bausch & Lomb Research
(I) 'scope about which I recently gloated does. This metallograph uses a
patented system of vertical illumination that greatly increases the image
brightness, so enough light gets to the MDS100's CCD sensor to overcome
its low sensitivity to the shorter wavelengths of visible light. What a
difference the blue filter makes in comparison to the usual dichroic green
filter that one usually uses for greyscale imaging ! I puzzled over this at
first, but then I realized that the image color that the MDS100 sensed with
the green filter is still somewhat reddish, whereas the blue filter gives a
bright blue image. And the focal distance changes dramatically as well.
That gives away the secret of the blue filter - it blocks the longer
wavelengths. On the other hand, the bias in sensitivity of the CCD for long wavelengths is
able to overcome the lesser ability of the green filter to
block the red & IR light. On the Olympus stereomicroscope I use an IR
filter, and that works well enough if I adjust the colors after making the
images.

George Langford, Sc.D.
amenex-at-amenex.com
http://www.amenex.com/

From MicroscopyL-request-at-ns.microscopy.com Sun Nov 28 18:15:03 2004

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Larry et all,

Most end users have no control when out of office(OOF) replies are sent.
Microsoft mail servers(which are the biggest cause of this problem) default to
send OOF messages to the internet instead of only to "local" users.

Last time I posted, 99% of the OOF replies I received were from MS mail
servers. This stupid default option cannot usually be altered by the end user,
it can only be changed by the network/mail administrator.

Bob

On 26 Nov 2004, at 7:48, Larry Stoter wrote:

}
}
} There have been a number of requests, including from Nestor but ...
}
} {Rant mode on :-))
}
} IF YOU ARE NOT COLLECTING YOUR E-MAIL, UNSUBSCRIBE FROM THE LIST.
}
} DO NOT JUST SET UP AN 'OUT OF OFFICE' AUTO REPLY.
}
} OTHERWISE ANYBODY POSTING TO THE LIST GETS DELUGED WITH 'OUT OF
} OFFICE AUTO REPLIES'.
}
} (because the default reply address for the list is the originator)
}
} To such an extent, that I am tempted to not only not post to the list
} anymore but permanently unsubscribe.
}
} IF ANY SUBSCRIBERS CAN'T UNDERSTAND THIS, PLEASE CONTACT ME AND I
} WILL TRY TO EXPLAIN EVEN MORE SIMPLY.
}
} {Rant Mode Off :-))
}
} Thank you,
} --
} Larry Stoter
} PLEASE NOTE
} 1. Any mail other than plain text will be automatically deleted.
} 2. Any mail, legitimate or not, apparently or actually from hotmail,
} netscape, yahoo or excite will automatically be deleted.
} 3. Mail with no subject or without a clear subject will be ignored :-)
}

From MicroscopyL-request-at-ns.microscopy.com Sun Nov 28 19:31:30 2004

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Yes, but the suggestion I made a few months ago after receiving a flood of autoreplies
would work, ie subscribe to the list with a different email address, even a hotmail
account.

cheers

rtch

Date sent: Sun, 28 Nov 2004 18:39:24 -0600
} From: Bob Sunley {rosunley-at-shaw.ca}

I have had little success in ruthenium tetroxide staining thin sections of
polyethylene or any other polyolefin. Recommend that you check out the
following reference for staining of polyolefins for SEM or TEM:

G.M. Brown and J.H. Butler, Polymer, 38 (15), 3937, 1997.

Cheers,

"The statements and opinions expressed here by Gary M. Brown represent
neither those of ExxonMobil Corporation nor its affiliates."

Gary M. Brown
ExxonMobil Chemical Company
Baytown Technology & Engineering - West
5200 Bayway Drive
Baytown, Texas 77520-2101
phone: (281) 834-2387
fax: (281) 834-2395
e-mail: Gary.M.Brown-at-ExxonMobil.com

wqsm-at-hotmail.com (by
way of To: microscopy-at-microscopy.com
MicroscopyListserver) cc:
Subject: [Microscopy] viaWWW: stain the ultrathin HDPE sample

11/24/04 09:34 PM

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Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (wqsm-at-hotmail.com) from
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Wednesday, November 24, 2004 at 16:20:14
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Email: wqsm-at-hotmail.com
Name: Ming

Organization: University of Alberta

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I wanna stain the ultrathin HDPE sample(after section) using RuO4
vapour. Could anyone give me some idear about the suitable stain time?
Thans!

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 08:58:10 2004

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Hello, Everyone,

I am testing various soil samples for Phosphorus content. Any suggestions given the fact that P is very low in content and silicon is everywhere.

Your suggestions, please. I am not a soil scientist.

Thanks.
Winnie

Edwina W. Westbrook
Electron Microscopy Laboratories
Agricultural Research Station
M. T. Carter Building, room 129
P.O.Box 9061
Virginia State University
Petersburg, VA 23806
(804)-524-5659
fax (804)-524-5622
ewestbro-at-vsu.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 09:19:16 2004

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It has become essential that we retrofit a CM10 TEM with a digital
camera system. I am trying to get information together for a grant
application. The microscope currently has a 35mm camera system, with no
other imaging system installed other than the viewing screen, of
course. We have received a quote from FEI for a system which would
entail modifying the column. I am aware of one alternate supplier.
However, I believe there must be more out there. Could anyone advise as
to alternative suppliers? Both who they are and what experiences you
may have had with them? As someone who has been forced to become more
realistic in life, I realize some responses will come from suppliers of
equipment. If you are a supplier, could you please tell me what you
have that would entail column modifications, what you have that would
not, performance specifications, and provide a rough idea of the cost.
I am not be asking for a quote today, just general ranges of cost.

Obviously, since we do not want to get into advertising and
testimonials, perhaps off the list
server would be best.

Thanks

paul

Paul R. Hazelton, PhD
Electron Microscope Unit
University of Manitoba
Department of Medical Microbiology
531 Basic Medical Sciences Building
730 William Avenue
Winnipeg, Manitoba, Canada, R3E 0W3
e-mail: paul_hazelton-at-umanitoba.ca
Phone:204-789-3313
Pager:204-931-954
Cell:204-781-1502
Fax:204-789-3926

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 10:02:39 2004

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ok i never get many out od office replies, if i do I
know where the delete button is, rather than rasie an
issue that only contributes to the excess junk email.
i allso have a bulk mail folder where everything goes
that i don't care about.
john
--- Ritchie Sims {r.sims-at-auckland.ac.nz} wrote:

}
}
}
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http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
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}
}
} Yes, but the suggestion I made a few months ago
} after receiving a flood of autoreplies
} would work, ie subscribe to the list with a
} different email address, even a hotmail
} account.
}
} cheers
}
} rtch
}
} Date sent: Sun, 28 Nov 2004 18:39:24 -0600
} } From: Bob Sunley {rosunley-at-shaw.ca}
} Subject: [Microscopy] Re: Errgrh -
} Please READ!
} To: Microscopy-at-MSA.Microscopy.Com
} Send reply to: rosunley-at-shaw.ca
} Priority: normal
}
} }
} }
} }
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} }
}
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}
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} } ---------
} }
} } Larry et all,
} }
} } Most end users have no control when out of
} office(OOF) replies are
} } sent. Microsoft mail servers(which are the
} biggest cause of this
} } problem) default to send OOF messages to the
} internet instead of only
} } to "local" users.
} }
} } Last time I posted, 99% of the OOF replies I
} received were from MS
} } mail servers. This stupid default option cannot
} usually be altered by
} } the end user, it can only be changed by the
} network/mail
} } administrator.
} }
} } Bob
} }
} }
} } On 26 Nov 2004, at 7:48, Larry Stoter wrote:
} }
} } }
} } }
} } } There have been a number of requests, including
} from Nestor but ...
} } }
} } } {Rant mode on :-))
} } }
} } } IF YOU ARE NOT COLLECTING YOUR E-MAIL,
} UNSUBSCRIBE FROM THE LIST.
} } }
} } } DO NOT JUST SET UP AN 'OUT OF OFFICE' AUTO
} REPLY.
} } }
} } } OTHERWISE ANYBODY POSTING TO THE LIST GETS
} DELUGED WITH 'OUT OF
} } } OFFICE AUTO REPLIES'.
} } }
} } } (because the default reply address for the list
} is the originator)
} } }
} } } To such an extent, that I am tempted to not only
} not post to the
} } } list anymore but permanently unsubscribe.
} } }
} } } IF ANY SUBSCRIBERS CAN'T UNDERSTAND THIS, PLEASE
} CONTACT ME AND I
} } } WILL TRY TO EXPLAIN EVEN MORE SIMPLY.
} } }
} } } {Rant Mode Off :-))
} } }
} } } Thank you,
} } } --
} } } Larry Stoter
} } } PLEASE NOTE
} } } 1. Any mail other than plain text will be
} automatically deleted. 2.
} } } Any mail, legitimate or not, apparently or
} actually from hotmail,
} } } netscape, yahoo or excite will automatically be
} deleted. 3. Mail
} } } with no subject or without a clear subject will
} be ignored :-)
} } }
} }
} }
} }
}
} --
} Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
} Microanalyst Fax : 64 9
} 3737435
} Department of Geology email :
} r.sims-at-auckland.ac.nz
} The University of Auckland
} Private Bag 92019
} Auckland
} New Zealand
}
}
}

__________________________________
Do you Yahoo!?
The all-new My Yahoo! - Get yours free!
http://my.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 11:23:04 2004

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Winnie,

Soil is such a heterogeneous material, I wonder if x-ray microanalysis is
the right method to use when one ends up looking at such a small sample
size.

Damian Neuberger, Ph.D.
Tel: (847) 998-8574
email: neuberger1234-at-comcast.net {mailto:neuberger1234-at-comcast.net}

Hello, Everyone,

I am testing various soil samples for Phosphorus content. Any suggestions
given the fact that P is very low in content and silicon is everywhere.

Your suggestions, please. I am not a soil scientist.

Thanks.
Winnie

Edwina W. Westbrook
Electron Microscopy Laboratories
Agricultural Research Station
M. T. Carter Building, room 129
P.O.Box 9061
Virginia State University
Petersburg, VA 23806
(804)-524-5659
fax (804)-524-5622
ewestbro-at-vsu.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 11:36:29 2004

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I have recently been researching this same software. Also, check out
Auto-Montage from Syncroscopy.
www.auto-montage.com

Shannan Little
Electron Microscopy and Image Analysis Lab
Agriculture & Agri-Food Canada
Lethbridge AB Canada

-----Original Message-----
} From: by way of MicroscopyListserver [mailto:wall1-at-llnl.gov]
Sent: Wednesday, November 24, 2004 8:35 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (wall1-at-llnl.gov) from
http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on
Wednesday, November 24, 2004 at 16:45:37
------------------------------------------------------------------------
---

Email: wall1-at-llnl.gov
Name: Mark Wall

Organization: LLNL

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for software that will create a single in-focus
image (tiff image files) from a series of images that are taken at
different (known) focus settings/heights. The application is for imaging
metallography samples that are not very flat or have considerable
roughness to them.

An additional bonus for us is to be able to have a 3-D plot of the
surface topography as well.

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 11:54:05 2004

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Hi, all,

A colleague has prepared some plant samples using HMDS. For the final step, he removed the samples from the bath and let them air dry. But the HMDS in the last bath is left over.

Depending on his results, he may want to process the rest of his samples using HMDS, and would expect to use quite abit. He has asked me whether it is possible to reuse what is left at the last step. Is there any reason why he can't do this? Should it be filtered to get rid of any small pieces of sample which broke off during handling?

Please let me know, and I'll forward the replies to him.

Thanks in advance for your help.

Regards,

Paula.

Paula M. Allan-Wojtas
Research Scientist - Food Microstructure/chercheur scientique - microstructure des aliments
Food Safety and Quality team/ Salubrité et qualité des aliments
Agriculture and Agri-Food Canada/Agriculture et Agroalimentaire Canada
Telephone/Téléphone: 902-679-5566
Facsimile/Télécopieur: 902-679-2311
32 Main Street/ 32, rue Main
Kentville, Nova Scotia/ Kentville (Nouvelle-Écosse)
B4N 1J5

allanwojtasp-at-agr.gc.ca

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 12:04:55 2004

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Dear Paul,

Three approaches come to mind, depending on the size of the fine structure:
a. Simple interferometry - several of the manufacturers carry small
Michelson or Tolansky interferometers which typically fit 10x objectives
but, in some cases, go up to 50x objectives. Interferometry is one of
those forgotten techniques that is very useful in this sort of application.
b. More advanced interferometry - companies such as Zygo and the Wyko part
of Veeco make scanning white light interferometers which will automatically
calculate a number of parameters which can be used to characterize the
surface. Visit either www.zygo.com or www.veeco.com and look up their
interferometry tools.
c. Atomic force microscopy also provides a number of topography
measurements. We've been working a lot lately with NTMDT (distributed
through Nanotech-America... new website is due to go up shortly at
www.nt-america.com, but you can also visit www.ntmdt.com - caveat... we do
have a commercial interest in this product), but there are also a number of
other AFM/SPM companies in the field.

Hope this was helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education

We've moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
W: www.MicroscopyEducation.com

P. S.
Need a good general reference or light microscopy text? Visit our website
to learn more about "Optimizing LIght Microscopy". Copies still available
through MME... even for class-room lots ... and we give quantity discounts.

At 02:43 PM 11/26/2004, Gerroir, Paul wrote:

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 12:54:14 2004

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We have looked at soils from time to time. I don't think I would want to
try to analyze phosphorus by EDS. You could try doing a shotgun analysis,
but you will have some problems unless you have a thick, smooth layer of
soil. The phosphorus may not be uniformly distributed and even through you
analyze at low magnification, you run a risk of finding a few grains in any
given field that would skew the results.

The content is generally quite low and EDS is limited to a detection limit
of about 0.3%. Even then, you wouldn't have very good sensitivity for
comparing samples.

In short, I would probably look for an x-ray fluorescence unit or some
other means better suited to bulk analysis at low concentrations.

Warren

At 09:17 AM 11/29/04, you wrote:

} Hello, Everyone,
}
} I am testing various soil samples for Phosphorus content. Any suggestions
} given the fact that P is very low in content and silicon is everywhere.
}
} Your suggestions, please. I am not a soil scientist.
}
} Thanks.
} Winnie
}
} Edwina W. Westbrook
} Electron Microscopy Laboratories
} Agricultural Research Station
} M. T. Carter Building, room 129
} P.O.Box 9061
} Virginia State University
} Petersburg, VA 23806
} (804)-524-5659
} fax (804)-524-5622
} ewestbro-at-vsu.edu

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 13:06:08 2004

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FYI. If you are interested please visit the site or contact me directly
with your resume.

Thanks

The Johns Hopkins Medical Laboratories

Employment Opportunities

The Johns Hopkins Department of Pathology is searching for a several
outstanding individuals to fill the following positions:

Electron Microscopy Technician I/II (requisition 14523)
Bachelor's degree, or equivalent, in the sciences plus two years of
training as an Electron Microscopy technician required. Comparable
experience may be substituted for degree requirement.

Sr. Histology Technician II (requisition 17869)
Bachelor's degree, or equivalent, in the sciences plus two years of
histology experience required. Comparable experience may be substituted
for degree requirement. HT(ASCP) eligible with recommended registry
within one year of employment.

Sr. Histology Technician III (requisition 17868)
Bachelor's degree, or equivalent, in the sciences plus two years of
histology experience required. Comparable experience may be substituted
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Bachelor's degree, or equivalent, in the sciences plus five years of
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for degree requirement. HT(ASCP) certification preferred.

We have a comprehensive salary program and excellent benefits,
including tuition remission at the University, in a smoke/drug free
workplace located at the main hospital campus in Baltimore, MD. For
consideration, please apply on-line at http://jobs.jhu.edu
EOE/AA/D/V.; www.jhu.edu

Lois Anderson
Johns Hopkins University
Dept. of Pathology
Laboratory Manager
EM/IF/Reference Histology
600 N. Wolfe Street/Pathology 709 A
Baltimore, MD 21287
(410) 955-2861/fax (410) 614-7110
landers-at-jhmi.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 13:13:22 2004

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I should have been a bit more detailed. Remember, I am not the soil scientist, however, wet chemistry is the method of testing...spectroscopy (ICP) and chromatography. Those methods are performed in the soil lab. My task is simply to place a dbl sticky SEM stub into a soil sample, coat with carbon and view in the SEM (randomly selected areas), generate a spectra and maps. SEM/EDAX is in addition to the well documented soil analysis methods.

Wanted to get some feedback or direction from all of you who are far more knowledgeable and generate discussion that may benefit others as well.

Thank you.

Winnie

Edwina W. Westbrook
Electron Microscopy Laboratories
Agricultural Research Station
M. T. Carter Building, room 129
P.O.Box 9061
Virginia State University
Petersburg, VA 23806
(804)-524-5659
fax (804)-524-5622
ewestbro-at-vsu.edu

} } } "Edwina Westbrook" {ewestbro-at-vsu.edu} 11/29/04 10:17AM } } }

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Hello, Everyone,

I am testing various soil samples for Phosphorus content. Any suggestions given the fact that P is very low in content and silicon is everywhere.

Your suggestions, please. I am not a soil scientist.

Thanks.
Winnie

Edwina W. Westbrook
Electron Microscopy Laboratories
Agricultural Research Station
M. T. Carter Building, room 129
P.O.Box 9061
Virginia State University
Petersburg, VA 23806
(804)-524-5659
fax (804)-524-5622
ewestbro-at-vsu.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 13:29:29 2004

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Image-Pro from Media Cybernetics has all these features, among a great
many others.

http://www.mediacy.com/ipp/imageproplus.htm

Disclaimer - I write the software; naturally, I'm biased.

-- Kevin Ryan
kevin-at-mediacy.com

----------------------------------------

Email: wall1-at-llnl.gov
Name: Mark Wall

Organization: LLNL

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I am looking for software that will create a single in-focus
image (tiff image files) from a series of images that are taken at
different (known) focus settings/heights. The application is for imaging
metallography samples that are not very flat or have considerable
roughness to them.

An additional bonus for us is to be able to have a 3-D plot of the
surface topography as well.

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 14:40:37 2004

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Hello,

My Name is Tom Sadowski and I am currently a student at Southern Connecticut
State University. I am currently involved in a project that is using a
Digital Instruments AFM microscope. Unfortunately, all of the images are
stored in their own proprietary format. I wish to do a batch conversion of
these images to a more standard format, especially uncompressed TIFF. Does
anyone know of a method I can use to do this? Any help would be greatly
appreciated

Thank you once again
Thomas Sadowski
Southern Connecticut State University

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 14:44:38 2004

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Due to space constraints, our department must part with bound copies of
the following journals. If you can provide a good home for these journals
please contact me off-line by email or phone.

Scanning Electron Microscopy 1972-1986
Proceedings of the Electron Microscopy Scociety of America (a.k.a. MSA)
1967-1999, and 2002.

Regards,
Joe Neilly, Research Investigator
Abbott Laboratories
R4R9, AP31
200 Abbott Park Rd.
Abbott Park, IL 60064-6202

Voice: 847-938-5024
Fax: 847-938-5027
E-mail: joe.neilly-at-abbott.com

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 15:28:39 2004

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I understand your frustration. I have been the recipient of such messages
numerous times.

But there really is no need to unsubscribe. As you noted, the replies go
back to the poster rather than the list. (That would be really messy.)
Therefore, if you never post, you would never get an OUT OF OFFICE reply. {g}
However, I think most of us hope that you would stick around _and_ continue
posting.

Warren Straszheim
Iowa State University

P.S. So far I have only gotten one of these infernal replies to my recent
posting. I expect more will be on the way. Then there will also be the crop
that results from this posting.

At 01:48 AM 11/26/04, you wrote:

} There have been a number of requests, including from Nestor but ...
}
} {Rant mode on :-))
} IF YOU ARE NOT COLLECTING YOUR E-MAIL, UNSUBSCRIBE FROM THE LIST.
} DO NOT JUST SET UP AN 'OUT OF OFFICE' AUTO REPLY.
} OTHERWISE ANYBODY POSTING TO THE LIST GETS DELUGED WITH 'OUT OF OFFICE
} AUTO REPLIES'.
} (because the default reply address for the list is the originator)
} To such an extent, that I am tempted to not only not post to the list
} anymore but permanently unsubscribe.
} IF ANY SUBSCRIBERS CAN'T UNDERSTAND THIS, PLEASE CONTACT ME AND I WILL TRY
} TO EXPLAIN EVEN MORE SIMPLY.
} {Rant Mode Off :-))
}
} Thank you,
} --
} Larry Stoter

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 16:48:32 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jean-paul.bailon-at-polymtl.ca) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, November 29, 2004 at 12:18:24
---------------------------------------------------------------------------

Email: jean-paul.bailon-at-polymtl.ca
Name: Jean-Paul Bailon

Organization: Ecole Polytechnique Montreal (QC) canada

Title-Subject: [Microscopy] [Filtered] Re: monte CArlo SImulation of electroN trajectory in sOlids

Question: The "surface radius of BE" generated by CASINO is in fact a simple histogram : "Number of backscattered electrons - vs - Radius". Here, "Radius" is defined as the distance at which a given BE is exiting the specimen. The origin of this distance is taken at the entry point of the electron probe (primary electrons).
If you simulate the trajectories for a large number of primary electrons, this histogram gives you an good approximation of the size of the specimen surface emitting the BE. This information may be useful if you want to known, at least as a first approximation, the spatial limit of resolution of a BE image.

Jean-Paul BaÔlon
Ecole Polytechnique de Montreal (QC) Canada

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From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 17:05:13 2004

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______________________________________________________________________

(11/29/04 14:32) Edwina Westbrook {ewestbro-at-vsu.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

While I certainly understand that you've been asked to do a particular test, I think the point that Damian was making is that it seems to some of us to be the wrong test to do. As Warren pointed out, XRF would be the first choice for this kind of analysis, but you're telling us that your analytical chem folks are already doing bulk analysis.

Maybe a better question to ask would be why someone thinks that an EDX spectrum would be useful in this situation? Doing randomly selected areas at a low mag might give you a decent bulk value, but XRF will give you the same information with better sensitivity - on the order of parts per million. If they want close ups - i.e., high mag, then the question is how they plan to eliminate the sampling bias? You're not guaranteed to sample all the species in the sample.

Brent

--
Brent Neal, Ph.D.
Reindeer Graphics, Inc.
brent-at-reindeergraphics.com

From MicroscopyL-request-at-ns.microscopy.com Mon Nov 29 21:24:03 2004

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Dear Sadowski
You can save veeco images in their soft ware only.
After doing offline correction, the images can be
saved ib tiff, jpeg or any other format by going to
utilities.
Shashi singh
CCMB
Hyderabad
INdia

Hello,

My Name is Tom Sadowski and I am currently a student
at Southern
Connecticut
State University. I am currently involved in a project
that is using a
Digital Instruments AFM microscope. Unfortunately, all
of the images
are
stored in their own proprietary format. I wish to do a
batch conversion
of
these images to a more standard format, especially
uncompressed TIFF.
Does
anyone know of a method I can use to do this? Any help
would be greatly
appreciated

Thank you once again
Thomas Sadowski
Southern Connecticut State University

DeleteReplyForwardSpam Move...

__________________________________________________
Do You Yahoo!?
Tired of spam? Yahoo! Mail has the best spam protection around
http://mail.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 30 03:33:49 2004

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Hello,
Our problem is solved. It was caused by PS2 power supply. The PC part of DX4
was completely without any energy.
If you like to see PS2 power supply, the image is on following page:

http://www2.biomed.cas.cz/~benada/DX4_troubles.html

Oldrich

P.S. Many thanks again for all advices and suggestions.

On 2 Nov 2004 at 13:35, Jim Quinn wrote:

} Oldrich
}
} Please remember to post your final outcome.
} We can all learn from it.
}
} regards,
}
} Jim

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 30 07:04:35 2004

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I think that the recent post on this subject from Jean-Paul BaÔlon is
misleading - sorry Jean-Paul. I started to look into this but have not
had time to finish the investigation but...

The size of the region from which backscattered electrons come is much
bigger than the resolution in the image.

The resolution in a secondary electron image corresponds to a distance
much smaller than the size of the area from which the secondary
electrons are emitted. This is well known. See for example, page 197
of the latest edition of the Goldstein et al book.

Something similar happens with backscattered electrons, though this is
more controversial. The plot that Jean-Paul refers to is a plot of
number of backscattered electrons against distance. If instead the
graph is made to plot number of electrons against position (divide the
first plot by 2pi times the radius) then the situation looks quite
different.

The number of backscattered electrons per unit area from the surface is
sharply peaked at the center and details in the image can be seen at
lengths related to this sharpness rather than the size of the whole area
from which electrons come.

This is the explanation for the fact that backscattered images show
details much smaller than a simple Monte Carlo result would suggest.

Alwyn
--
..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 30 07:39:46 2004

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If I understand your problem, what you (or your colleagues) are tying to
determine is what mineral phase the P is present in. This would require
that you analyze individual particles, and enough particles enriched
with P to say something about the sample. If you are making maps of
your sample you must be interested in some spatial features of P
distribution in your sample. While X-ray mapping is a way to get at
this, you might want to try a different prep technique to improve the
mapping results. I recall reading an article on preparing polished
cross sections of soil samples in the July 2004 Microscopy and Analysis
that dealt with archaeological soil samples and might be of some use.

Hope this helps,

Bryan Bandli

Edwina Westbrook wrote:

} I should have been a bit more detailed. Remember, I am not the soil scientist, however, wet chemistry is the method of testing...spectroscopy (ICP) and chromatography. Those methods are performed in the soil lab. My task is simply to place a dbl sticky SEM stub into a soil sample, coat with carbon and view in the SEM (randomly selected areas), generate a spectra and maps. SEM/EDAX is in addition to the well documented soil analysis methods.
}
} Wanted to get some feedback or direction from all of you who are far more knowledgeable and generate discussion that may benefit others as well.
}
} Thank you.
}
} Winnie
}
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 30 07:48:38 2004

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Thomas,
My experience with proprietary software formats has been that the
vendor (in your case Digital Instruments) provides a means to
"export" your data from their format into others. I would be
surprised if they did not, since most of their end-users would want
to take data from the microscope work with it either with analysis
software or simply put it into Photoshop or PhotoImpact etc. which
handle TIF.
Check the manual and/or help menu for the AFM or call Digital
Imaging. If they don't supply a conversion method, they should.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Tue Nov 30 08:50:51 2004

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Tom,

you should find the TIF export function through the
menu of Utility in the Nanoscope offline data
processing program bundled with the realtime software.

Hope it helps,

Susheng Tan

--- Thomas Sadowski {tommy91779-at-hotmail.com} wrote:

}
}
}
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} The Microscopy ListServer -- Sponsor: The
} Microscopy Society of America
} To Subscribe/Unsubscribe --
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} On-Line Help
}
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}
-------------------------------------------------------------------------------
}
} Hello,
}
} My Name is Tom Sadowski and I am currently a student
} at Southern Connecticut
} State University. I am currently involved in a
} project that is using a
} Digital Instruments AFM microscope. Unfortunately,
} all of the images are
} stored in their own proprietary format. I wish to do
} a batch conversion of
} these images to a more standard format, especially
} uncompressed TIFF. Does
} anyone know of a method I can use to do this? Any
} help would be greatly
} appreciated
}
}
} Thank you once again
} Thomas Sadowski
} Southern Connecticut State University
}
}
}
}

=====
Susheng TAN, D.Sc.
Department of Chemistry, Oklahoma State University
107 Physical Science
Stillwater, Oklahoma 74078
Phone: (405)744-4835 Fax:(405)744-6007
eMail:tsushen-at-okstate.edu sstan33-at-yahoo.com

__________________________________
Do you Yahoo!?
Yahoo! Mail - Helps protect you from nasty viruses.
http://promotions.yahoo.com/new_mail

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 08:31:19 2004

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Thanks to all how offered to house the MSA and SEM journals. We have
found a good home for them so they are no longer available.

Regards,
Joe Neilly, Research Investigator
Abbott Laboratories
R4R9, AP31
200 Abbott Park Rd.
Abbott Park, IL 60064-6202

Voice: 847-938-5024
Fax: 847-938-5027
E-mail: joe.neilly-at-abbott.com

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 09:16:55 2004

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I would like to do some tomography of vesicles in cryo conditions, can anyone recommend what grid type I should use and what sort of support film would be best? Also for negative stain tomography which grids and support films should be best?

Many thanks,
Anna Young

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 09:35:06 2004

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Hi

Does anyone out there have good experience of zinc formaldehyde or
alternative 'metal-formaldehyde ' fixatives?

Thanks in advance

Nadolig Llawen a Blwddyn Newydd Dda / God Jul och Gott Nytt Ĺr / Merry
Christmas and a Happy New Year

Gareth

http://www.ki.se/biomedlab
e-mail Gareth.Morgan-at-labmed.ki.se

Tel +46 8 5858 1038
Fax +46 8 5858 7730

Gareth Morgan MPhil MSc FIBMS,
Department of Laboratory Medicine (Labmed),
Karolinska Institute,
Karolinska University Hospital at Huddinge, F46
SE 141 86 Stockholm
Sweden

OBS! Besöksadress: F-Huset, Forskningsgatan 2 F52, Rum 2.10. Laboratoriet
för klinisk patologi och cytologi.

NB! Visiting address: Building F, Research Corridor 2 F52, Room 2.10.
Clinical Histo- and Cytopathology Laboratory.

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 13:08:54 2004

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Thank you all for the great suggestions both on and off line. XRF, etc, however, are not available. The soil testing is being conducted with already well established protocols. The hope was/is to use the SEM/EDAX to look at P associations in the soil--perhaps associated with clay, Al, Fe, or Ca. Using mapping we have been able to locate some P-rich regions. We have tried RGB mixing to find regions where there are associations(P with other elements).

I hope this discussion has helped others as much as it has helped me. Hopefully, I can contact any of you offline when I get stuck with another 'where do I go from here question'.

Regards,
Winnie

Edwina W. Westbrook
Electron Microscopy Laboratories
Agricultural Research Station
M. T. Carter Building, room 129
P.O.Box 9061
Virginia State University
Petersburg, VA 23806
(804)-524-5659
fax (804)-524-5622
ewestbro-at-vsu.edu

} } } bbandli {bbandli-at-mvainc.com} 11/30/04 09:06AM } } }

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If I understand your problem, what you (or your colleagues) are tying to
determine is what mineral phase the P is present in. This would require
that you analyze individual particles, and enough particles enriched
with P to say something about the sample. If you are making maps of
your sample you must be interested in some spatial features of P
distribution in your sample. While X-ray mapping is a way to get at
this, you might want to try a different prep technique to improve the
mapping results. I recall reading an article on preparing polished
cross sections of soil samples in the July 2004 Microscopy and Analysis
that dealt with archaeological soil samples and might be of some use.

Hope this helps,

Bryan Bandli

Edwina Westbrook wrote:

} I should have been a bit more detailed. Remember, I am not the soil scientist, however, wet chemistry is the method of testing...spectroscopy (ICP) and chromatography. Those methods are performed in the soil lab. My task is simply to place a dbl sticky SEM stub into a soil sample, coat with carbon and view in the SEM (randomly selected areas), generate a spectra and maps. SEM/EDAX is in addition to the well documented soil analysis methods.
}
} Wanted to get some feedback or direction from all of you who are far more knowledgeable and generate discussion that may benefit others as well.
}
} Thank you.
}
} Winnie
}
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 15:59:02 2004

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On Dec 1, 2004, at 7:39 AM, Anna Young wrote:

} I would like to do some tomography of vesicles in cryo conditions, can
} anyone recommend what grid type I should use and what sort of support
} film would be best? Also for negative stain tomography which grids and
} support films should be best?
}
Dear Anna,
We use Quantifoils, and they work very well for cryotomography. Get
200-mesh grids, since smaller mesh sizes will occlude the specimen at
high tilt angles. I'd use carbon film for negative stain tomography.
Carbon-formvar will also work well with essentially no loss of
resolution, and the film is stronger under some circumstances than just
carbon, but, since the formvar is not conducting, sometimes a
carbon-formvar film will be less stable than just carbon. Again, use
200-mesh or larger grids. I am not affiliated with Quantifoil or other
grid suppliers (coated or not), except as a satisfied customer.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 16:02:57 2004

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Hi-

Want to determine the PSF of our Confocal Scanning Laser Ophthalmoscope
(used to image the retina in the eye, but very similar in design to the
Confocal Microscope). Unfortunately, I only had access to 10µm beads and
they have a 12px diameter when imaged at the highest magnification. Can I
still derive the PSF from these images, or do I have to buy smaller beads?
If yes, how should I go about it?

Grateful for advice.

Thanks!

-Peter
--
Peter Lundh
E: peter.lundh-at-ucl.ac.uk
T: +44 (0) 207-608 4049
M: +44 (0) 788-195 2645
F: +44 (0) 207-608 6909

Visual Science Department
Institute of Ophthalmology
11 - 43 Bath Street
EC1V 9EL London

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 16:25:16 2004

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Hello Xavier !

You wrote:

} Re: Using a Kodak MDS100 on a B&L Research I metallograph

Aha ! You went to the Amenex website ...

} We have an ETEC Autoscope SEM from 1969. We have problems with
} the image when we rotate from 180 to 90 degrees. The images seem
} like a compact shape (see the photos below). Does someone has
} information that help us to fix this?
} Not good image (seems like compact image)
Oh, oh. Aspect ratio isn't adjusted correctly
} This the correct form of the image
Looks OK.
} This is our ETEC Autoscope SEM:
Wow. Very clean & neat setup.

Ken Converse may chime in on this, but my first impression is that
your 'scope has an adjustment for specimen tilt that restores the
apparent shape of the specimen so that a square looks square
even when the specimen tilt would introduce foreshortening. You
had it adjusted OK at zero degrees, and now it's exactly wrong at
90 degrees. It's been four years since I last looked at our ETEC
Autoprobe (now hopefully ensconced at or near UC Berkeley) but
memory says that this adjustment is associated with the magnification
selector. There's a set of thumbwheels at the lower end, I think.

Be sure to watch those red rockets - the Tantalum electrolytics that
were _our_ Autoprobe's weak links. I'd look for the ones that had
turned black and replace 'em with foil electrolytics from our local
Radio Shack. Used the same or higher voltage and the same
microfarad rating. The cans were bigger but they worked fine.

I just finished a report in which I used the MDS100 with the Research
I metallograph to make quite a few photomicrographs, using a proper
green interference filter (Kodak standard issue) which allowed me
to see the images in the microscope eyepieces much more easily
than with the blue interference filter. This green filter blocks the
longer wavelengths far more effectively than the plain green filter
that I first tried. Now I get green images with the MDS100 ! And then
I convert them to greyscale, of course.

Best regards to all,
George Langford, Sc.D.
amenex-at-amenex.com
http://www.amenex.com/

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 1 23:53:12 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Anna Young wrote:
============================================================================
============
I would like to do some tomography of vesicles in cryo conditions, can
anyone recommend what grid type I should use and what sort of support film
would be best? Also for negative stain tomography which grids and support
films should be best?
============================================================================
============
The Quantifoil® grids were developed for just this application. See URL
http://www.2spi.com/catalog/grids/quantifoil-carbon-films.html

Another, but not as well proven possibility, for this application, would be
our perforated silicon nitride membrane window grids, see URL
http://www.2spi.com/catalog/instruments/perforated-membrane-window-grids.
shtml

Disclaimer: SPI Supplies offers both types of grids so we would have a
vested interest in seeing more of either of them being used.

Chuck

PS: Please remember that we are nearly 100% paperless and we would ask
that any reply to this message be by way of the "reply" feature on your
software, so that the entire string of correspondence can come back to us
and all be in one place.

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 07:20:22 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (lan.xu-at-fmi.ch) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, December 2, 2004 at 02:36:08
---------------------------------------------------------------------------

Email: lan.xu-at-fmi.ch
Name: Lan Xu

Organization: FMI

Title-Subject: [Microscopy] [Filtered] EM

Question: Dear sir or madam,
I would like to know a potocol for Formvar-coat single slot grides. I need to do a consecutive serial section for EM stduy in brain sections, but I don't know how to coat the single slot grides, (I have the normal potocol for coat Mesh square grides) If you could give me a potocol for Formvar-coat single slot grides, I would be very gladful.
Thank you in advence,
Lan Xu

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 13:45:26 2004

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Hi Listers,

The following question was forwarded to me, so I'm passing it on to the
collective for possible suggestions.

"Do you know of any ways of labeling/marking or otherwise making Cd in
brain tissue visisble, either by light or TEM?

We are doing blood and brain studies on cadmium exposure in rats.

I have been doing the Cd analysis in the tissues (blood and whole
brains), but we want to look at areas of the brain for Cd levels. That
puts the sample amount in the 15mg range and for me to analyze, that
gives me values in the ppt range, which is too low. So we'd have to pool
brain samples to get enough.

I wondered if there was some way to label the Cd in tissue prior or
after making slides with some countable/fluorescent or otherwise
quantifiable materials. So he could do brain sections and figure it
out."

This looks like way too little for EDS analysis and I know nothing about
labeling techniques for low concentrations of heavy metals. Any
thoughts?

Thanks!

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 14:39:32 2004

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Please note that the deadline for MSA Award nominations if fast
approaching (December 15, 2004). Information is available in the
current issue of Microscopy and Microanalysis (vol 10 (6): facing page
822).

Categories include 2 Distinguished Scientist Awards (Biological and
Physical Sciences), the Burton Medal (young investigator), 2 Outstanding
Technologist Awards, and the Morton D. Maser Distinguished Service
Award.

Please feel free to contact me for additional information if needed.

William T. Gunning, Ph.D.
Professor of Biochemistry and
Cancer Biology; Pathology
Medical College of Ohio
Departments of Biochemistry and
Cancer Biology; Pathology
Medical College of Ohio
BHSB 140
3035 Arlington Avenue
Toledo, Ohio 43614-5806
Phone: 419-383-4131 or 3752
Fax: 419-383-6228
email: wgunning-at-mco.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 15:56:14 2004

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Dear Randy,
I recall an aluminum x-ray map of an Alzheimer's patient's dried brain
tissue, showing Al in ppm levels. It was done in an automated EPMA (WDX) and
took about 16 hours to collect, with a long dwell time on each point. The
presenter said that the EPMA wasn't being used overnight, so why not. The
dried tissue will concentrate the metal somewhat. The other possibility is
to use the backscattered detector. This will only work if the Cd is
concentrated somewhat in some areas, but it should show up bright against
the organic background.
Your levels may be too low for either of these techniques. The only other
one I know that is more sensitive is an x-ray microscope.
Good luck.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "Tindall, Randy D." {TindallR-at-missouri.edu}
To: {microscopy-at-microscopy.com}
Sent: Thursday, December 02, 2004 12:09 PM

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (markjaco-at-hotmail.com) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Thursday, December 2, 2004 at 11:23:50
---------------------------------------------------------------------------

Email: markjaco-at-hotmail.com
Name: Mark Jacobs

Organization: Minneapolis, washburn high school

Education: 9-12th Grade High School

Location: Minneapolis, MN USA

Question: What education level do you need to work in microscopy? Where are the programs?

I love biology and working with microscopes.
thanks
Mark

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 19:12:45 2004

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Randy,

You probably already saw this but check out this website

www.scripps.edu/news/press/112304.html

wherein they announce a "ligand" that will detect heavy metals such
as Hg and Cd but is not reactive with Fe, etc.

The article, "A Precipitator for the Detection of Thiophilic Metals
in Aqua," is authored by Tobin J. Dickerson, Neal N. Reed, James J.
La Clair, and Kim D. Janda and will appear in an upcoming issue of
the Journal of the American Chemical Society.

It may be applicable in microscopy.

John
--
##############################################################
John J. Bozzola, Ph.D., Director
I.M.A.G.E. (Integrated Microscopy & Graphics Expertise)
750 Communications Drive - MC 4402
Southern Illinois University
Carbondale, IL 62901 U.S.A.
Phone: 618-453-3730
Email: bozzola-at-siu.edu
##############################################################

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 23:04:44 2004

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Dear Anna,

How small are the vesicles you are interested in imaging? Next week at Cell Bio, NT-MDT is going to announce a new integrated product which puts an AFM into a microtome. The AFM will image directly from the block face, eliminating typical errors from slippage, pull-out, tears, or wrinkles, then do a 3D reconstruction from the resulting image stack. I think it might be a faster, more effective solution to your application. Anton Efimov, the inventor of this technique, will also be available for discussion at the show. NT-MDT is being distributed here in the US through Nanotech America. They will be in booth 1129-1130, if you are interested.

Caveat: MME is providing support for this project.

I hope this is helpful,
Barbara Foster
Microscopy/Microscopy Education

We've moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
W: www.MicroscopyEducation.com

P. S.
Need a good general reference or light microscopy text? Visit our website to learn more about "Optimizing LIght Microscopy". Copies still available through MME... even for class-room lots ... and we give quantity discounts.

At 09:39 AM 12/1/2004, Anna Young wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 23:17:11 2004

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Dear Mark,

If you love biology, then I would recommend that you major in that field,
but find a subspecialty that takes you into microscopy and
imaging. Today there is a lot of work done in live cell imaging and in
fluorescence.

I am sure that your guidance counselor can help you to find a good bio
program. There are so many choices, from genetics to marine
biology,etc. Be prepared for the long haul, however, because you will most
likely need to get a PhD and then do post doctoral work.

There are also interesting jobs opening up in industry (biotechnology,
nanobiology, etc.).

Good hunting!

Best regards
Barbara Foster
Microscopy/Microscopy Education

We've moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
W: www.MicroscopyEducation.com

At 05:17 PM 12/2/2004, markjaco-at-hotmail.com wrote:

} ------------------------------------------------------------------------------
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From MicroscopyL-request-at-ns.microscopy.com Thu Dec 2 23:59:33 2004

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Hi Mark,
I'm happy to hear you're interested in Microscopy. I'm an instructor at
Madison Area Technical College in Madison, Wisconsin. We offer a two
year Associate in Applied Science Degree in Electron Microscopy. It
covers both biological and materials. There is also Delta College in
California that offers a two year EM Program. There are a lot of other 4
year colleges and graduate programs that offer many great opportunities
in this field. Check out some websites, and if you have any questions,
please feel free to contact me.
Bill

Bill Carmichael
wcarmichael-at-matcmadison.edu
http://matcmadison.edu/electronmicros

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:markjaco-at-hotmail.com]
Sent: Thursday, December 02, 2004 5:18 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (markjaco-at-hotmail.com) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html
on Thursday, December 2, 2004 at 11:23:50
------------------------------------------------------------------------
---

Email: markjaco-at-hotmail.com
Name: Mark Jacobs

Organization: Minneapolis, washburn high school

Education: 9-12th Grade High School

Location: Minneapolis, MN USA

Question: What education level do you need to work in microscopy? Where
are the programs?

I love biology and working with microscopes.
thanks
Mark

------------------------------------------------------------------------
---

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 00:34:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi listers,

For a long time, we have been trying to operate the integrated SX-50
unit (CAMECA). Although the system comprise of only one WDS, we believe
that is fine too. When we try to calibrate the spectro we could not be
able to catch any peaks in the "expected" region, for example:

Fe Ka peak in LIF crystal should be around 48084 (sine-theta) but when
we scan the pure iron standart we see the peak around 74064 (sine-theta)

Or;

Si Ka peak in PET crystal should be around 81444 (sine-theta) but when
we scan the pure Si standart we see the peak around 106497 (sine-theta).

There is an evident peak shift, nearly 25000 (sine-theta).

I have noticed that the spectrometer limits exceed the suggested values.
In the troubleshooting section of reference guide; it says that limits
of the spectrometer, namely; pmin should be { 22000 and pmax should be }
83000. Also the difference (pmax-pmin) should be greater than 61000. Our
pmin is 46616 and pmax is 108545. We have the mentioned difference
(108545-46616=61929) but the limits are shifted evidently. It should be
expected that if we lower these two values by 25000, these would be in
the suggested limits and there would be no peak shift!

I have done the following steps to lower pmin and pmax:

1) I have tried to initialize the WDS by "INIT WDS" or even by "INIT"
commands in the SU Local console.

2) I have tried to reset the WDS Motorola 68000 microprocessor by its
switches

3) I have even tried to look up the machine codes in the debugging mode

4) I used all variations (as far as I understand) of "FIX" commands

5) and lastly I decided to change the pmin and pmax variables by "DEFI"
command, but I could not, as they are "system protected variables"

I decided to choose another way for it; I calibrated Fe Ka line on pure
Fe sample with LIF crystal. But as expected, the "peaks" were nearly at
the same intensities with background noise as a result of peak shift.

I prepared a declaration file, defining a chemical shift of 25000. I
knew it was very unpractical and somehow random. Such a chemical shift
value causes the software crash a lot and keeps giving the error message
".... beyond spectrometer limits"

I am desperately seeking help, I assume it is not a great technical
problem but I must confess that I am stuck. Any reply would be highly
and sincerely appreciated.

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
Beytepe-Ankara / TURKEY
06532
Ph: +90 312 2977700 / 126

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 07:03:13 2004

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Hey Mark,

The education level you need to work in microscopy you already have. It is
the second word in your message. Formal schooling helps, of course, if you
want to get paid for it. But don't let the schooling get in the way of your
education. Even if you become a professional, always strive to be an
amateur (from 'amator', 'amare') that is, one who does something out of
love, rather than for financial gain.

Paul

-------------------------------------------

Work like you don't need the money;
Love like you've never been hurt;
Dance like nobody's watching.
- Satchel Paige

(The opinions expressed here do not necessarily represent those of my
employer or Purdue University)

-----Original Message-----
} From: by way of Ask-A-Microscopist [mailto:markjaco-at-hotmail.com]
Sent: Thursday, December 02, 2004 6:18 PM
To: microscopy-at-microscopy.com

Below is the result of your feedback form (NJZFM-ultra-55). It was
submitted by (markjaco-at-hotmail.com) from
http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on
Thursday, December 2, 2004 at 11:23:50
---------------------------------------------------------------------------

Email: markjaco-at-hotmail.com
Name: Mark Jacobs

Organization: Minneapolis, washburn high school

Education: 9-12th Grade High School

Location: Minneapolis, MN USA

Question: What education level do you need to work in microscopy? Where are
the programs?

I love biology and working with microscopes.
thanks
Mark

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 08:12:22 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Thank everyone who replies about our problem,

We could not find the offsett value established by the installation
engineer which Michael Shaffer told, but instead of 150 000 we wrote 100
000 and followed the procedure which Graham Hutchinson
told.

Now it works!

Everything seems fine now! Thanks all....

Best regards

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
Beytepe-Ankara / TURKEY
06532
Ph: +90 312 2977700 / 126

My problem was;

For a long time, we have been trying to operate the integrated SX-50
unit (CAMECA). Although the system comprise of only one WDS, we believe
that is fine too. When we try to calibrate the spectro we could not be
able to catch any peaks in the "expected" region, for example:

Fe Ka peak in LIF crystal should be around 48084 (sine-theta) but when
we scan the pure iron standart we see the peak around 74064 (sine-theta)

Or;

Si Ka peak in PET crystal should be around 81444 (sine-theta) but when
we scan the pure Si standart we see the peak around 106497 (sine-theta).

There is an evident peak shift, nearly 25000 (sine-theta).

I have noticed that the spectrometer limits exceed the suggested values.
In the troubleshooting section of reference guide; it says that limits
of the spectrometer, namely; pmin should be { 22000 and pmax should be }
83000. Also the difference (pmax-pmin) should be greater than 61000. Our
pmin is 46616 and pmax is 108545. We have the mentioned difference
(108545-46616=61929) but the limits are shifted evidently. It should be
expected that if we lower these two values by 25000, these would be in
the suggested limits and there would be no peak shift!

I have done the following steps to lower pmin and pmax:

1) I have tried to initialize the WDS by "INIT WDS" or even by "INIT"
commands in the SU Local console.

2) I have tried to reset the WDS Motorola 68000 microprocessor by its
switches

3) I have even tried to look up the machine codes in the debugging mode

4) I used all variations (as far as I understand) of "FIX" commands

5) and lastly I decided to change the pmin and pmax variables by "DEFI"
command, but I could not, as they are "system protected variables"

I decided to choose another way for it; I calibrated Fe Ka line on pure
Fe sample with LIF crystal. But as expected, the "peaks" were nearly at
the same intensities with background noise as a result of peak shift.

I prepared a declaration file, defining a chemical shift of 25000. I
knew it was very unpractical and somehow random. Such a chemical shift
value causes the software crash a lot and keeps giving the error message
".... beyond spectrometer limits"

I am desperately seeking help, I assume it is not a great technical
problem but I must confess that I am stuck. Any reply would be highly
and sincerely appreciated.

Orkun ERSOY
Hacettepe University
Department of Geological Engineering
Beytepe-Ankara / TURKEY
06532
Ph: +90 312 2977700 / 126

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 08:49:50 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

John,

Thanks for this suggested link. The article is available on-line now. If
your institution has a subscription to the Journal of the American Chemical
Society for on-line content, this link should work:

http://pubs.acs.org/cgi-bin/asap.cgi/jacsat/asap/pdf/ja045798r.pdf

Doug

At 06:36 PM 12/2/2004, you wrote:
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

....................................................................
Douglas W. Cromey, M.S. Dept. of Cell Biology & Anatomy
Research Specialist, Principal University of Arizona
(office: AHSC 4212A) P.O. Box 245044
(voice: 520-626-2824) Tucson, AZ 85724-5044 USA
(FAX: 520-626-2097) (email: Cromey-at-Arizona.edu)
....................................................................
http://swehsc.pharmacy.arizona.edu/exppath/
Home of: "Microscopy and Imaging Resources on the WWW"

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 11:15:44 2004

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Hi,

I need suggestions on how to do micro-structure analysis on automotive
emission catalytic converter (honeycomb). Can anyone tell me how to prepare
SEM and TEM samples from the honeycomb? Does the process follow the basic
procedure: cutting, grinding, polishing and ion-milling? Basically, I want
to get noble metal particles' (such as Pt) size and dispersion on the
supports, such as alumina.

Thanks in advance for your advice. Any suggestion would be highly
appreciated!

*******************************************
Juan Cai, Ph. D.
Scientist
Nanostellar
3603 Haven Avenue, Suite A
Menlo Park, CA 94025
Phone: 650-4502267 (cell)
Fax: 650-3681101
jcai-at-nanostellar.com
*********************************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 11:23:03 2004

Contents Retrieved from Microscopy Listserver Archives
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Regarding Al and Alzheimer disease, this was done much more convincingly
using a nuclear microprobe - particle induced X-ray emission technique
(PIXE) with matrix corrections using proton backscattering. See publications
by Frank Watt and Geoff Grime + medical collaborators.
Regarding Cd, PIXE would be much better than EDS. Firstly, you should not
use Cd-L lines because of overlaps with potassium K-lines and this is really
a big problem. Therefore EDS is in practice not possible to use, and PIXE
can be used on K lines of Cd. A microprobe based on synchrotron radiation
would be much better indeed (you may call it "x-ray microscopy"?). I suggest
searching papers related to this method (SXRF).

Best regards

xxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxx
Dr Wojciech J. Przybylowicz
Materials Research Group
iThemba LABS
PO Box 722
Somerset West 7129 South Africa
E-mail: przybylowicz-at-tlabs.ac.za
Fax: +27-21-8433543
Phone: +27-21-8431166 (direct); 8431000 (reception)
Cell: +27-82-563 7925
http://www.tlabs.ac.za
xxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxxx

----- Original Message -----
} From: "Mary Mager" {mager-at-interchange.ubc.ca}
To: "Tindall, Randy D." {TindallR-at-missouri.edu}
Cc: "Microscopy" {microscopy-at-MSA.microscopy.com}
Sent: Friday, December 03, 2004 12:20 AM

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Juan Cai wrote:
============================================================================
=
I need suggestions on how to do micro-structure analysis on automotive
emission catalytic converter (honeycomb). Can anyone tell me how to prepare
SEM and TEM samples from the honeycomb? Does the process follow the basic
procedure: cutting, grinding, polishing and ion-milling? Basically, I want
to get noble metal particles' (such as Pt) size and dispersion on the
supports, such as alumina.
============================================================================
=
These systems consist of what is described as a) the honeycomb structure
(which generally consists of low surface area alumina and is generally not
of interest), b) the "wash coating" of high surface area alumina, usually
gamma, on the internal surfaces of the honeycomb and c) the metal catalyst
particles, generally platinum or platinum alloys, dispersed in the coated
layer of high surface area alumina. These are true nanoparticles since they
are rarely larger than 2 nm and usually less. What one generally wants to
see is the degree of dispersion of the nano size metal particles in the high
surface area alumina. We have generally found in our own laboratory, when
we have tried to do these kinds of samples, the "basic procedures" as
outline above generally fail. And the only way that we have ever found that
works reliably is diamond knife thin sectioning on an ultramicrotome.

But this also means that you have to embed a piece of the honey comb
substrate (but only a slight trace of the substrate structure remaining)
that contains the alumina wash coat, keeping track of where you are on the
sample, doing the diamond knife ultramicrotomy, and then examining the
sections by TEM. You can not only image the size and degree of dispersion
of the metal particles but you can also see areas of "hot spotting" which
can have a dramatic effect on the efficiency of the catalyst. Some poisons
such as lead can be imaged this way as well. One note of caution: I have
encountered some workers who literally scrape off some of the high surface
alumina and embed just the fines, an obviously much easier task, but you
lose the all important spatial information when you do it this way. Others
just look at the fines but it is not a very representative sample since the
data comes only from those particles that are small enough to be electron
transparent.

We have found that our own SPI-Pon 812 embedding resin works quite fine for
this application but we would expect that at least some of the "Epon
substitutes" offered by our competitors would work just as well. Cutting
samples of this type is literally "hard" on anyone's diamond knife. We use
the standard 45 degree knives which results in minimum compression. But be
sure you don't waste money on an expensive "life science" knife for this
kind of work since a 45 deg. "materials science" diamond knife will work
just fine. See URL
http://www.2spi.com/catalog/knives/materials.shtml
for more information.

Disclaimer: Our firm does this kind of diamond knife thin sectioning as a
laboratory analytical service for others. We are also suppliers of the
recommended embedding resin and the materials science diamond knives.

Chuck
===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 13:40:12 2004

Contents Retrieved from Microscopy Listserver Archives
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Hello:

We intend to surplus our Philips EM300 that is currently working well
and is under service contract. We are looking for offers to remove and
accept the unit, to make room for a new TEM.

Yours,

Bill Marshall
------------------------------------------------
} {///(°} } {///(°} } {///(°} } {///(°} } {///(°}

^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
William S. Marshall, Ph.D. ° ° °
Professor, Biology Department ° °
St. Francis Xavier University {°)\\\} {
Box 5000 Antigonish NS B2G 2W5
Canada
Phone 902-867-2482 Fax 902-867-2389
*************************************

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 16:07:12 2004

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Dear Listers,

Many thanks for all the suggestions and references! I have passed
everything along to the person needing the information (and learned
quite a bit myself).

Happy Holidays,
Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 16:46:35 2004

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Greetings:

A campus researcher has asked advice about obtaining a new SEM for our lab.

It's been a long time since anyone asked me about this, and I have let my
knowledge of current instruments slide. Besides, it seems like they change
so fast that it would be hard to keep up unless you are ready to get
something new.

I would like to get advice about where to start looking, not which vendors,
I know most of them, but where in the product/feature continuum we should
start.

We have a 1986 vintage ISI WB-6 conventional SEM in the lab now. For the
most part, it does OK. We don't need a large sample chamber or lots of
whistles and bells. Our applications are varied as a central campus lab,
but most are at least semi-biological, no hard core materials types.

The specific application of the inquiring researcher is looking at small
pore patterns in diatoms to confirm species identifications.

I am especially interested in hearing about some of the new developments in
SEM's since we got our ISI machine. Things like 'environmental' SEM, FEG
developments etc. Also any updates on coating techniques beyond our
conventional sputter coater would be useful.

Real world experiences would be great. You know, things like, this sounds
good, but doesn't really add anything or this is a feature I never thought
would be worth anything but I couldn't live without it now, type remarks.

With your help, I will be in a much better position to get the right
instrument for my campus guy and be way better off when talking to vendors.

Thanks

Jon

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 3 17:24:37 2004

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Dear Alwyn,

I feel that my short reply to Andrey’ question was slightly misunderstood…
Let go with the points you raise and your comments on the spatial resolution
of backscattered electrons (BSE) images:

A) “The size of the region from which backscattered electrons come is much
bigger than the resolution in the image”:
If you are talking of the spatial resolution of a backscattered electron
image, I agree partially with this sentence. In my reply to Andrey, I should
have written that the so-called “Surface Radius of BE” histogram generated
by CASINO gives a CONSERVATIVE UPPER LIMIT of the spatial resolution of BSE
images.

B) “The resolution in a secondary electron image corresponds to a distance
much smaller than the size of the area from which the secondary electrons
are emitted”:
I fully agree, except that… I never spoke of secondary electron image in my
reply to Andrey!

C) “If instead the graph is made to plot number of electrons against
position (divide the
first plot by 2pi times the radius) then the situation looks quite
different”:
In fact, you are suggesting to define a parameter J which is proportional to
the true local current density in the region emitting the BSE. In such a
case, one have to divide the number dN of BSE emitted by a surface element
dS. Due to the axial symmetry of the problem, dS = (pi^2)[R(i+1) – Ri] =
(pi^2)(delta R), where (delta R) is the increment of the radial distance Ri.
Note that the term (pi^2) which is different from your 2pi…

With the raw data generated by the free software CASINO
(http://www.gel.usherb.ca/casino/) and imported in a spreadsheet like Excel,
I did this exercise and I have plotted three types of curve:

-- J (= dN/dS) –vs– distance R
-- Cumulative J –vs– R
-- Cumulative dN –vs– R

The “Cumulative J –vs– R” and “Cumulative dN –vs– R” curves are very similar
to the normalised curves presented in figure 3.24 of Goldstein’s book (2nd
edition). If anybody is interested by these results, please contact me off
line and I will send you the figures.

Now the fundamental question is: “How to define the spatial resolution from
these figures”. I agree that J (=dN/dS) is “sharply peaked at the center”,
however one cannot ignore the other BSE coming from the rim around this
peak. One have to make some assumption on the percent of BSE which
significantly contribute to the signal coming from the emitting region and
which are received by a BSE detector such as the solid-state detector.
Conservatively, lets take a criterion of 60%. Andy, try this simple exercise
on figure 3.24 of Goldstein’s book with the values of the Kanaya-Okayama
radius given in table 3.2 of the same book. The results are as follows:

Energy of the primary electrons = 20 keV
Criterion for defining the “spatial resolution” = 60% of the total number of
BSE
“Spatial resolution” for Copper (Z = 29) = 345 nm (nanometer)
“Spatial resolution” for Aluminium (Z = 13) = 1350 nm (nanometer)

In my opinion and as daily demonstrated with any “classic” SEM, such figures
clearly show that the “spatial resolution” of a BSE image will never match
that of a SE image, except if one has the chance to work with special
devices like the energy filtering system developed by Wells and commented in
section 4.6.1 of Goldstein’s book.

Jean-Paul

++++++++++++++++++++++++++++++++++++++
Prof. Jean-Paul Baďlon mailto:jean-paul.bailon-at-polymtl.ca
Génie mécanique Tél: +1(514) 340 4711, p. 4260
École Polytechnique Fax: +1(514) 340 4468
CP 6079, Succursale Centre-Ville
Montréal (QC) Canada H3C 3A7
++++++++++++++++++++++++++++++++++++++

-----Message d'origine-----
De : Alwyn Eades [mailto:jae5-at-lehigh.edu]
Envoyé : 30 novembre, 2004 08:29
Ŕ : Microscopy-at-MSA.Microscopy.Com
Objet : Monte Carlo simulation of backscattered electrons

I think that the recent post on this subject from Jean-Paul BaÔlon is
misleading - sorry Jean-Paul. I started to look into this but have not
had time to finish the investigation but...

The size of the region from which backscattered electrons come is much
bigger than the resolution in the image.

The resolution in a secondary electron image corresponds to a distance
much smaller than the size of the area from which the secondary
electrons are emitted. This is well known. See for example, page 197
of the latest edition of the Goldstein et al book.

Something similar happens with backscattered electrons, though this is
more controversial. The plot that Jean-Paul refers to is a plot of
number of backscattered electrons against distance. If instead the
graph is made to plot number of electrons against position (divide the
first plot by 2pi times the radius) then the situation looks quite
different.

The number of backscattered electrons per unit area from the surface is
sharply peaked at the center and details in the image can be seen at
lengths related to this sharpness rather than the size of the whole area
from which electrons come.

This is the explanation for the fact that backscattered images show
details much smaller than a simple Monte Carlo result would suggest.

Alwyn
--
.........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 4 02:54:06 2004

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I'm not an expert on this ... but I think you'll find the structure
is mechanically quite fragile. To get decent samples, you'll need to
support the structure during preparation.

I'd first cut into smallish (~2 cm across and perhaps ~1 cm thick)
and then embed in resin - I'd have thought a standard epoxy would be
OK. Having done that, you can then proceed with standard
metallurgical preparation techniques. I think you can get the
information you need by SEM, so grinding and polishing is probably
all you need to do.

Keep in mind, commercial auto catalysts contain a wide range of Pt
group metals. If you want to distinguish the different elements, you
will almost certainly need to use WDX, since EDX won't have
sufficient energy resolution.
--
Larry Stoter
JEOL (UK) Ltd
tel: +44-(0)1707-377117, fax: +44-(0)1707-373254, e-mail: larrys-at-jeoleuro.com

PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 4 05:03:01 2004

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Dear Randy,

I hope this will be helpful.

Y. Sumi, Masanori T. Itoh, Takeshi Muraki, Takuro Suzuki (1996).
Histochemical staining of cadmium with
2-(8-quinolylazo)-4,5-diphenylimidazole. Histochemistry and Cell Biology,
Volume 106, Number 2: 223 - 227.

Regards,

Vera Santos
Dental Medical School
Institute of Biomedical Technology (ITB)
University of Lisbon
Portugal

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 4 07:19:02 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (somayyeh_kheiri-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, December 4, 2004 at 05:39:46
---------------------------------------------------------------------------

Email: somayyeh_kheiri-at-yahoo.com
Name: somayyeh

Title-Subject: [Microscopy] [Filtered] karyotype of verbascum

Question: Hello Dear all

I am doing meosic karyotype of Verbascum species on
buds preseved in carnoy solution.
but unfortunately the chromosomes are so little and I have
problem counting them specially in the magnification of 100 LM.
I would appreciate any helps and suggestion.

Thanks alot

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 4 23:24:54 2004

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Have you tried FIB? In Situ liftout FIB should be able to make a
satisfactory specimen of this type of material.

John Mardinly
Intel

-----Original Message-----
} From: Juan Cai [mailto:jcai-at-nanostellar.com]
Sent: Friday, December 03, 2004 9:41 AM
To: Microscopy-at-MSA.Microscopy.Com

Hi,

I need suggestions on how to do micro-structure analysis on automotive
emission catalytic converter (honeycomb). Can anyone tell me how to
prepare
SEM and TEM samples from the honeycomb? Does the process follow the
basic
procedure: cutting, grinding, polishing and ion-milling? Basically, I
want
to get noble metal particles' (such as Pt) size and dispersion on the
supports, such as alumina.

Thanks in advance for your advice. Any suggestion would be highly
appreciated!

*******************************************
Juan Cai, Ph. D.
Scientist
Nanostellar
3603 Haven Avenue, Suite A
Menlo Park, CA 94025
Phone: 650-4502267 (cell)
Fax: 650-3681101
jcai-at-nanostellar.com
*********************************************************

From MicroscopyL-request-at-ns.microscopy.com Sun Dec 5 05:43:55 2004

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Hi,

I'm not sure this will work, but there is a new technology from Aetos called "CytoViva" which drops the limit of resolution of the light microscope from 250nm to below 120nm. It might give you just the edge you need.

Their website is www.CytoViva.com. Their tech apps person is Tom Hasling. I'm sure he'd be happy to run a sample for you. The website has all of their contact info.

Hope this was helpful.

Best regards,
Barbara Foster
Microscopy/Microscopy Education

We've moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
W: www.MicroscopyEducation.com

P. S.
Need a good general reference or light microscopy text? Visit our website to learn more about "Optimizing LIght Microscopy". Copies still available through MME... even for class-room lots ... and we give quantity discounts.

At 07:43 AM 12/4/2004, somayyeh_kheiri-at-yahoo.com wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Sun Dec 5 08:41:05 2004

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Dear All,

Currently, I am organizing and chair a conference with title topic Vision'05
June 20-23, 2005 at LA, USA. The following is the detailed. Interested
please kindly email you full paper to the following address:-
ksism-at-mmu.edu.my or sksbg2003-at-yahoo.com

CALL FOR PAPERS

The 2005 International Conference on Computer Vision
(VISION'05: June 20-23, 2005, Las Vegas, USA)
http://www.world-academy-of-science.org

Title of Approved Session: Microscopy Imaging System

Chair of Session: Dr. Kok-Swee Sim
Multimedia University, Melaka, Malaysia

Conference: The 2005 International Conference on Computer Vision
(VISION'05: June 20-23, 2005, Las Vegas, USA)
http://www.world-academy-of-science.org
Monte Carlo Resort, Las Vegas, Nevada, USA
June 20-23, 2005

Description:
In this session, conference papers that submitted are related to Microscopy
imaging system. The papers can be in the area of Material science microscopy
and microanalysis, Medical applications of scanning microscopy,
Microanalysis in Scanning Electron Microscope (SEM), Microscopy and
microanalysis: theory, instrumentation and techniques, Monte Carlo modeling
for microscopy and microanalysis, Multidimensional microscopy, Museum
applications, Nanotechnology and nanofabrication, Scanning probe
microscopies, Semiconductor devices, materials and process characterization,
X-ray mapping in electron beam instruments.

Dear Colleagues:
You are invited to submit a draft paper (see instructions below) and/or a
proposal to organize a technical session/workshop. All accepted papers will
be published in the conference proceedings.

The International Multiconference in Computer Science and Computer
Engineering is a major annual research event. It assembles a spectrum of
affiliated research conferences into a coordinated research meeting held in
a common place at a common time. This model facilitates communication among
researchers in different fields of computer science and computer
engineering. The last Multiconference attracted over 1,650
computer science and engineering researchers from 78 countries. We expect to
have over 2,000 attendees for this set of conference.

Please regard this announcement as General Guidelines. You are requested to
send your submission to the chair whose address appears below.

Dr. Kok-Swee, Sim
kssim-at-mmu.edu.my or sksbg2003-at-yahoo.com
Tel: (+606) 252-3044
Fax: (+606) 231-6552
E-mail: sksbg2003-at-yahoo.com

SUBMISSION OF PAPERS:

Prospective authors are invited to submit three copies of their draft paper
(about 5 pages - single space, font size of 10 to 12) to KS Sim by the due
date (who may be forwarding the papers to respective conference
chairs/committees). E-mail submissions in MS document or PDF formats are
preferable (Fax submissions are also acceptable.)

The length of the Camera-Ready papers (if accepted) will be limited to
7 (IEEE style) pages. Papers must not have been previously published or
currently submitted for publication elsewhere. The first page of the
draft paper should include: title of the paper, name, affiliation, postal
address, E-mail address, telephone number, & Fax number for each author.
The first page should also include the name of the author who will be
presenting the paper (if accepted) & a maximum of 5 keywords.

IMPORTANT DATES:

Feb. 16, 2005: Submission of papers (about 5 pages)
March 21, 2005: Notification of acceptance
April 20, 2005: Camera-Ready papers & Prereg. due
June 20-23, 2005: The 2005 World Congress in Applied
Computing (WCAC'05) - 14 Joint
Conferences.

Thanks
Ks

From MicroscopyL-request-at-ns.microscopy.com Sun Dec 5 14:26:13 2004

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Hi all,

Can anyone give me the current contact information for whoever is likely
to have replacement parts for a 20year old LKB knifemaker? I need to
replace the scoring wheel in ours.

Thanks,
Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 6 07:31:04 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rvf263-at-chartermi.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Sunday, December 5, 2004 at 21:42:43
---------------------------------------------------------------------------

Email: rvf263-at-chartermi.net
Name: Robert Farris

Organization: Monroe County Community College

Education: Undergraduate College

Location: Newport, Michigan - United States

Question: I'm taking Biology in college now, will be taking Anatomy & Physiology this winter, and Microbiology soon. Can you recommend a decent microscope for me to purchase for use at home?
Thank you very much
Robert

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 6 09:09:25 2004

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Hello group,

We are looking to purchase a new high-vacuum carbon evaporation unit for
our lab.
I have received information on the Cressington 208 and 308 models, the
Denton Bench
Top Turbo IV, and Emitech.

Does anyone have any experience with these units? Can anyone comment on
their
reliability and performance? Anyone have any other recommendations for
coaters?

The coater will be used for SEM/EDS analysis of samples with topography.
We mainly
work on inorganic materials. It may also, in the future, be used for
TEM work.

Thank you in advance for your help.
Amy Bern

^v^
Amy M. Bern
Chemist
EPA, NEIC, Bldg. 25
P.O. Box 25227
Denver, CO 80225
Phone: 303-462-9128

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 6 14:00:46 2004

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Debby,
At Ted Pella Inc, we offer an overhaul service on LKB knifemakers for $500
plus shipping. This includes a new scoring wheel and other consumable parts.
Check it out at: http://www.tedpella.com/glass_html/knifemkr.htm
We do not offer the parts separately.

Regards,
Mark Armogida
VP of Engineering and Production

Phone: 530.243.2200 X212
Fax: 530.243.3761

Ted Pella, Inc.
www.tedpella.com

-----Original Message-----
} From: Debby Sherman [mailto:dsherman-at-purdue.edu]
Sent: Sunday, December 05, 2004 12:54 PM
To: message to: MSA list

I am looking for glue for embedding samples (materials and minerals).
Please advise the glue that is suitable for materials. EpoFix is out of stock
at Electron Microscopy Sciences, so I am looking for a similar one from the
other companies. I am embedding samples for ultramicrotomy.

Thank you,
Hiromi Konishi, Ph.D.
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 6 23:33:02 2004

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} We recondition LKB Knife Makers, including scoring wheel
etc. for $250.00 plus shipping. Turn-around 1 week.
We also recondition Sorval MT-1, MT-2 and 2B Ultra
Microtomes and sell belt kits/ motor mounts for MT-2/2B.
Regards
Markus F. Meyenhofer
Microscopy Labs
Box 338
61 West Street
Red Bank, NJ 07701
732 747 6228
fax 732 758 9142
}
}
} ----------------------------------------------------------
} -------------------- The Microscopy ListServer -- Sponsor:
} The Microscopy Society of America To

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 7 07:56:11 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Stacey.Andringa-at-uc.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, December 6, 2004 at 13:32:34
---------------------------------------------------------------------------

Email: Stacey.Andringa-at-uc.edu
Name: Stacey Andringa

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] staining cicadas

Question: Is there is a stain that will light up mercury in
sectioned tissues (cicadas in this instance)?
Thanks.

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From MicroscopyL-request-at-ns.microscopy.com Tue Dec 7 13:13:40 2004

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STUDENT POSTER COMPETITION ANNOUNCEMENT

To be held in conjunction with the March 24,2005 meeting of the Midwest
Microscopy and Microanalysis Society

Affiliate of the Microscopy Society of America and the Microbeam
Analysis Society of America

!!PLEASE NOTE EXTENDED DEADLINE FOR RECEIPT OF ABSTRACTS!!

ABSTRACT DEADLINE: Abstracts must be received in electronic format by
5PM, WEDNESDAY, DECEMBER 22, 2004.

The first quarter meeting of the Midwest Microscopy and Microanalysis
Society will be held on Thursday, March 24, 2005, in the Pancoe Life
Sciences Building, Northwestern University, Evanston, Illinois. A
student poster competition open to undergraduate and graduate students
will be held in conjunction with the meeting. Posters should illustrate
utilization of microscopy for either biological or materials science
study. Prizes will be awarded as follows:

$300 for 1st place
$200 for 2nd place
$100 for 3rd place

Abstracts must be received in electronic format by 5PM on Wednesday,
December 22, 2004. To be eligible for a prize, you must be first author
on the poster, and you must be present at the meeting. You are
encouraged to submit your entry as early as possible, as space may be
limited. Further details and an explanation of judging criteria will be
provided upon acceptance of your submission.

Please send the following information to the email address below, and
attach your abstract as a Word document:

Name Affiliation
Department Phone number
Email address

Send to:

Elaine Schumacher
MMMS Materials Science Director
McCrone Associates, Inc.
850 Pasquinelli Drive
Westmont, IL 60559-5539
Tel: 630-887-7100 Fax: 630-887-7417
Email: eschumacher-at-mccrone.com

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 7 13:47:17 2004

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ElectroscanE3 for sale as a standing unit or we will part it out. This ESEM
is a working unit though the image quality is poor right now either due to
the scintillator or the column is dirty. Hit stage, tensile stage, and
peltier stage; LaB6 ready.

No offers for the standing unit under $10K, if you need parts we will
discuss the price on an as need basis. Water chiller not included.

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 7 21:41:38 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rebecca.burgin-at-onsemi.com) from http://www.msa.microscopy.org/MicroscopyListserver/MLFormMail.html on Tuesday, December 7, 2004 at 17:26:50
---------------------------------------------------------------------------

Email: rebecca.burgin-at-onsemi.com
Name: Rebecca Burgin

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Does anyone has experience in chemical junction staining on SiC SEM samples? Please advise. Thanks.

Rebecca

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From MicroscopyL-request-at-ns.microscopy.com Tue Dec 7 21:41:15 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (fchu-at-mrl.ubc.ca) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 7, 2004 at 16:25:24
---------------------------------------------------------------------------

Email: fchu-at-mrl.ubc.ca
Name: Fanny Chu

Organization: iCAPTURE Lab, University of British Columbia

Title-Subject: [Microscopy] [Filtered] Epon sections diffused

Question: Somebody in our lab has had sections that will get diffused and dispersed within two seconds staying in the boat. Ironically, all the Epon ingredients were brand new.
Any suggestions what's wrong or can be done about it?

Thanks!

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From MicroscopyL-request-at-ns.microscopy.com Tue Dec 7 22:45:19 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (drbenjy-at-optonline.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Tuesday, December 7, 2004 at 22:36:24
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Email: drbenjy-at-optonline.net
Name: Ben Glassman, MD

Organization: Physician in private practice

Education: Graduate College

Location: Mamaroneck, New York, USA

Question: I have a number of mounted blood smears of unusual anemias. The mountant is yellowing and would like to know if it is possible to salvage these slides. Also ,is it possible to restain them

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From MicroscopyL-request-at-ns.microscopy.com Wed Dec 8 07:38:45 2004

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Fanny
We've all been hit with this phenomenon at some time ...It sounds
like incomplete infiltration and/or polymerization to me. Even with
brand new components, if they are not mixed adequately the resin
won't harden correctly. Also, if the dehydration was not complete
(your absolute ethanol or acetone was not actually absolute) the
resin will not be able to fully infiltrate the tissue and you will
see the effect you've described. I'm afraid there is no salvaging of
those blocks (at least none that I've found). Next time, make sure
that you use a fresh bottle of 100% dehydrating agent, and also take
the time to thoroughly mix the resin components. It may even help to
stir them up, let them sit for 15-30 minutes and stir them again. We
used to do that with Spurr's resin all the time.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 8 07:42:30 2004

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} Question: I have a number of mounted blood smears of unusual
} anemias. The mountant is yellowing and would like to know if it is
} possible to salvage these slides. Also ,is it possible to restain
} them
}
} ---------------------------------------------------------------------------
the histologist who shares my lab space routinely rescues slides from
the medical students' slide collection. She soaks them in a coplin
jar of xylene overnight, or longer, until the old cover glass falls
off. She then restains them if needed and mounts a new cover glass
with Permount. She usually handles paraffin sections and they come
through this procedure very nicely. I'm not sure if blood smears
would restain well. I would try it with you least valuable slide
first as a test specimen.

Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 8 08:39:05 2004

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Any time your section diffuse during microtomy,
it is usually
caused by incomplete infiltration of the tissue.
This will occur
even if your epon ingredients are new. You must
draw out your
infilitration steps, ie: from 2 x 5 min. propylene
oxide, 3:1 P.O.:
epon for 2 hrs then 1:1 P.O.: Epon 2 hrs or
overnight, 1:2 P.O.:
Epon 2 hrs, then 3 fresh Epon changes. Vacuum
infiltration also helps, and Spurrs is a better
infiltrating
resin. Good Luck.

Michael Delannoy
Assist. Director
Johns Hopkins School of Medicine Microscope Facility

----- Original Message -----
} From: fchu-at-mrl.ubc.ca (by way of MicroscopyListserver)

Hello All,
I am posting this ad for Prof. Yang. Please look at the detail below.

The Department of Materials Science and Engineering at the University of
Pittsburgh seeks a post-doctoral research associate for in situ transmission
electron microscopy studies of surface oxidation reactions of metallic
alloys. The successful applicant will utilize primarily a unique in situ
ultra-high vacuum transmission electron microscope that resides within the
Materials Research Laboratory at the University of Illinois at
Urbana-Champaign. The appointment is initially for one year with possible
extension, starting immediately.

Surface oxidation processes play critical roles in environmental stability,
corrosion, electrochemistry, catalysis, gate oxides, fuel reactions, as well
as nanostructures and thin films formed by surface reactions. Furthermore,
as engineered materials approach the nanometer scale, environmental
stability at this scale is critical to the device performance. The objective
of this research program is fundamental understanding of nano-oxidation
reactions via a coordinated experimental effort, with in situ UHV-TEM
(University of Pittsburgh) and synchrotron X-ray diffraction (Argonne
National Laboratory), and theoretical and simulations effort (University of
Florida). The experimentalists and theorists will interact closely.

A Ph.D. in Materials Science and Engineering, Physics, or related field is
necessary. Required experience includes transmission electron microscopy.
Experience with in situ, advanced electron microscopy methods and/or other
characterization methods, such as AFM, and thin film deposition is
advantageous, but not required.

To apply for this position, please send a resume with the names and contact
information for three references, or to obtain more information, please
contact:

Professor Judith Yang

848 Benedum Hall

Materials Science & Engineering Dept.

University of Pittsburgh

Pittsburgh, PA 15261

jyang-at-engr.pitt.edu

(412) 624-8613

Long Li
_________________________________________________________
Materials Science and Engineering Department
University of Pittsburgh
3700 O'Hara St., 848 Benedum Hall
Pittsburgh, PA 15261

Tel: (412) 624-9753
FAX: (412) 624-8069
e-mail: Lil2-at-pitt.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 8 17:07:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (gautam-at-jncasr.ac.in) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Wednesday, December 8, 2004 at 10:01:24
---------------------------------------------------------------------------

Email: gautam-at-jncasr.ac.in
Name: Gautam

Organization: JNCASR

Education: Graduate College

Location: Bangalore, Karnataka, India

Question: Hi. Is it possible that we see a doubling of the lattice spacing in a high-resolution electron microscopy TEM image. If yes, what are the reasons and could you suggest some references?

Thanks.
Gautam.

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From MicroscopyL-request-at-ns.microscopy.com Thu Dec 9 08:51:43 2004

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Greetings Peter,

This depends on the numerical aperture/resolving power of the
objective lens being measured. Ten microns is almost certainly too big
though. To generate a point-spread function dataset you will need to use
beads that are well below the resolution limit of the lens in question.
Molecular probes sells such beads under the brand name "Tetraspeck" (140nm).
Polysciences sells very small fluorescent beads as well (down to 50nm). Quantum dots (~10nm)
are another alternative, however they are somewhat expensive.
-Karl

Peter Lundh wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 9 10:26:49 2004

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Dear All,

Does anyone has the experience on working edge detection imaging technique
on SEM images ? Just curious also, what is the implication of applying edge
detection technique such as canny, sobel and so on onto SEM images.

If anyone has the idea, please kindly share with me.

Many thanks
Kok Swee

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 9 10:28:05 2004

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When I prepare my Epon resin I stir two components together for 5-10
min, add the third, stir for another 5-10 min before adding the
accelerator and stir for 30 min. I get consistent result this way. If
you put all four together and stir, you may get various results.

Ann Fook Yang

-----Original Message-----
} From: Leona Cohen-Gould [mailto:lcgould-at-med.cornell.edu]
Sent: Wednesday, December 08, 2004 9:05 AM
To: by way of MicroscopyListserver; microscopy-at-microscopy.com

Fanny
We've all been hit with this phenomenon at some time ...It sounds
like incomplete infiltration and/or polymerization to me. Even with
brand new components, if they are not mixed adequately the resin
won't harden correctly. Also, if the dehydration was not complete
(your absolute ethanol or acetone was not actually absolute) the
resin will not be able to fully infiltrate the tissue and you will
see the effect you've described. I'm afraid there is no salvaging of
those blocks (at least none that I've found). Next time, make sure
that you use a fresh bottle of 100% dehydrating agent, and also take
the time to thoroughly mix the resin components. It may even help to
stir them up, let them sit for 15-30 minutes and stir them again. We
used to do that with Spurr's resin all the time.
Lee
--
Leona Cohen-Gould, M.S.
Sr. Staff Associate
Director, Electron Microscopy Core Facility
Manager, Optical Microscopy Core Facility
Joan & Sanford I. Weill Medical College
of Cornell University
voice (212)746-6146
fax (212)746-8175

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 10 07:22:59 2004

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Dear All,

I am currently organizing and chair an session for USA conference Vision'05.
Please kindly support by sending me conference paper.

Many thanks
The following is the information:-

CALL FOR PAPERS

The 2005 International Conference on Computer Vision
(VISION'05: June 20-23, 2005, Las Vegas, USA)
http://www.world-academy-of-science.org

Title of Approved Session: Microscopy Imaging System

Chair of Session: Dr. Kok-Swee Sim
Multimedia University, Melaka, Malaysia

Conference: The 2005 International Conference on Computer Vision
(VISION'05: June 20-23, 2005, Las Vegas, USA)
http://www.world-academy-of-science.org
Monte Carlo Resort, Las Vegas, Nevada, USA
June 20-23, 2005

Description:
In this session, conference papers that submitted are related to Microscopy
imaging system. The papers can be in the area of Material science microscopy
and microanalysis, Medical applications of scanning microscopy,
Microanalysis in Scanning Electron Microscope (SEM), Microscopy and
microanalysis: theory, instrumentation and techniques, Monte Carlo modeling
for microscopy and microanalysis, Multidimensional microscopy, Museum
applications, Nanotechnology and nanofabrication, Scanning probe
microscopies, Semiconductor devices, materials and process characterization,
X-ray mapping in electron beam instruments.

Dear Colleagues:
You are invited to submit a draft paper (see instructions below) and/or a
proposal to organize a technical session/workshop. All accepted papers will
be published in the conference proceedings.

The International Multiconference in Computer Science and Computer
Engineering is a major annual research event. It assembles a spectrum of
affiliated research conferences into a coordinated research meeting held in
a common place at a common time. This model facilitates communication among
researchers in different fields of computer science and computer
engineering. The last Multiconference attracted over 1,650
computer science and engineering researchers from 78 countries. We expect to
have over 2,000 attendees for this set of conference.

Please regard this announcement as General Guidelines. You are requested to
send your submission to the chair whose address appears below.

Dr. Kok-Swee, Sim
kssim-at-mmu.edu.my or sksbg2003-at-yahoo.com
Tel: (+606) 252-3044
Fax: (+606) 231-6552
E-mail: sksbg2003-at-yahoo.com

SUBMISSION OF PAPERS:

Prospective authors are invited to submit three copies of their draft paper
(about 5 pages - single space, font size of 10 to 12) to KS Sim by the due
date (who may be forwarding the papers to respective conference
chairs/committees). E-mail submissions in MS document or PDF formats are
preferable (Fax submissions are also acceptable.)

The length of the Camera-Ready papers (if accepted) will be limited to
7 (IEEE style) pages. Papers must not have been previously published or
currently submitted for publication elsewhere. The first page of the
draft paper should include: title of the paper, name, affiliation, postal
address, E-mail address, telephone number, & Fax number for each author.
The first page should also include the name of the author who will be
presenting the paper (if accepted) & a maximum of 5 keywords.

IMPORTANT DATES:

Feb. 16, 2004: Draft papers (about 5 pages) due
March 22, 2004: Notification of acceptance
April 21, 2004: Camera-Ready papers & Prereg. due
June 21-24, 2004: 2004 Int'l Multiconference in CS & CE

----- Original Message -----
} From: "by way of MicroscopyListserver" {jean-paul.bailon-at-polymtl.ca}
To: {microscopy-at-microscopy.com}
Sent: Tuesday, November 30, 2004 7:13 AM

Dear All,

I am currently organizing and chair an session for USA conference Vision'05.
Please kindly support by sending me conference paper.

Many thanks
The following is the information:-

CALL FOR PAPERS

The 2005 International Conference on Computer Vision
(VISION'05: June 20-23, 2005, Las Vegas, USA)
http://www.world-academy-of-science.org

Title of Approved Session: Microscopy Imaging System

Chair of Session: Dr. Kok-Swee Sim
Multimedia University, Melaka, Malaysia

Conference: The 2005 International Conference on Computer Vision
(VISION'05: June 20-23, 2005, Las Vegas, USA)
http://www.world-academy-of-science.org
Monte Carlo Resort, Las Vegas, Nevada, USA
June 20-23, 2005

Description:
In this session, conference papers that submitted are related to Microscopy
imaging system. The papers can be in the area of Material science microscopy
and microanalysis, Medical applications of scanning microscopy,
Microanalysis in Scanning Electron Microscope (SEM), Microscopy and
microanalysis: theory, instrumentation and techniques, Monte Carlo modeling
for microscopy and microanalysis, Multidimensional microscopy, Museum
applications, Nanotechnology and nanofabrication, Scanning probe
microscopies, Semiconductor devices, materials and process characterization,
X-ray mapping in electron beam instruments.

The International Multiconference in Computer Science and Computer
Engineering is a major annual research event. It assembles a spectrum of
affiliated research conferences into a coordinated research meeting held in
a common place at a common time. This model facilitates communication among
researchers in different fields of computer science and computer
engineering. The last Multiconference attracted over 1,650
computer science and engineering researchers from 78 countries. We expect to
have over 2,000 attendees for this set of conference.

Please regard this announcement as General Guidelines. You are requested to
send your submission to the chair whose address appears below.

Dr. Kok-Swee, Sim
kssim-at-mmu.edu.my or sksbg2003-at-yahoo.com
Tel: (+606) 252-3044
Fax: (+606) 231-6552
E-mail: sksbg2003-at-yahoo.com

SUBMISSION OF PAPERS:
Prospective authors are invited to submit three copies of their draft paper
(about 5 pages - single space, font size of 10 to 12) to KS Sim by the due
date (who may be forwarding the papers to respective conference
chairs/committees). E-mail submissions in MS document or PDF formats are
preferable (Fax submissions are also acceptable.)

The length of the Camera-Ready papers (if accepted) will be limited to 7
(IEEE style) pages. Papers must not have been previously published or
currently submitted for publication elsewhere. The first page of the
draft paper should include: title of the paper, name, affiliation, postal
address, E-mail address, telephone number, & Fax number for each author.
The first page should also include the name of the author who will be
presenting the paper (if accepted) & a maximum of 5 keywords.

Feb. 16, 2005: Submission of papers (about 5 pages)
March 21, 2005: Notification of acceptance
April 20, 2005: Camera-Ready papers & Prereg. due
June 20-23, 2005: The 2005 World Congress in Applied
Computing (WCAC'05) - 14 Joint
Conferences.

----- Original Message -----
} From: "by way of MicroscopyListserver" {jean-paul.bailon-at-polymtl.ca}
To: {microscopy-at-microscopy.com}
Sent: Tuesday, November 30, 2004 7:13 AM

Listers,

The Alcatel MDP-5010 molecular drag pump that backs the turbo pump on
our S-900 has died, and the 5010 can no longer be rebuilt. Alcatel
has quit making or providing parts.
So, I'm wondering if anyone has an old Alcatel MDP-5010 lurking
around in working condition (preferably rebuilt, controller not
needed), or has any extra 7+ cfm (170+ L/min) oil-free scroll pumps,
like the Edwards XDS-10. Which latter are rarer than hens' teeth, it
seems.
Thanks for any help.

Phil
--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 11 07:48:44 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Springpaard-at-yahoo.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, December 9, 2004 at 15:34:20
---------------------------------------------------------------------------

Email: Springpaard-at-yahoo.com
Name: springpaard

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: What is the single advantage provided by TIRF microscopy that allows
one to view single molecules?

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 11 07:48:16 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (shuckaby-at-reddyus.com) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, December 9, 2004 at 14:40:56
---------------------------------------------------------------------------

Email: shuckaby-at-reddyus.com
Name: Sondra Huckaby

Organization: Reddy US Therapeutics

Title-Subject: [Microscopy] [Filtered] Use of Alcian Blue for staining of proteoglycans

Question: I hope some one can help me out here. I am trying to use Alcian Blue staing to quantitate matrix proteoglycans. Currently the system i have worked out is to grow tissue culture cells of interest on glass cover glass, fix the cells to the cover glass in 4%formalin/PBS for 20 minutes washed in ddH2O and then stain with 1% Alcian blue(w/v) solution prepared in 3%acetic acid (in water). I allow the staining to progress for 2 hours at room temperature then remove the staining solution, wash the coverglass with the fixed and stained cells and mount onto the slides. I am using a Nikon light microscope and 100x oil imersion lense to see the actual extracellular matrix of the cells. The problem that I am having is that the staining is not very even and I have what look to be large crystals of the blue that are not washed off. I am looking to reduce background due to these large crystals so I can just see nice green-blue matrix. I have tried filtering the dye solution with minimal success. If you have any tips for staining proteoglycans in tissue culutre with Alcian blue please let me know. THANKS!

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 11 07:47:53 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kssim-at-mmu.edu.my) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, December 9, 2004 at 10:26:21
---------------------------------------------------------------------------

Email: kssim-at-mmu.edu.my
Name: kssim

Organization: mmu

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Dear All,

Does anyone has the experience on working edge detection imaging technique
on SEM images ? Just curious also, what is the implication of applying edge
detection technique such as canny, sobel and so on onto SEM images.

If anyone has the idea, please kindly share with me.

Many thanks
Kok Swee

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 11 07:49:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Stacey.Andringa-at-uc.edu) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, December 10, 2004 at 10:04:40
---------------------------------------------------------------------------

Email: Stacey.Andringa-at-uc.edu
Name: Stacey Andringa

Organization: University of Cincinnati

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I have a co-worker looking for a used microtome
part. It is a standard fixed jaw specimen clamp
for an RMC MT-980 (now designated MR3)rotary
microtome. I have done a google search with
little success. If anyone knows a good source
for used parts, please let me know.
Thanks.

Stacey Andringa

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 11 07:50:20 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (qizhang-at-physics.unc.edu) from http://www.msa.microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, December 10, 2004 at 16:10:29
---------------------------------------------------------------------------

Email: qizhang-at-physics.unc.edu
Name: Qi Zhang

Title-Subject: [Microscopy] [Filtered] MListserver: JEM-2010F beam oscillating

Question: Dear colleagues:

Our JEM-2010F microscope has beam oscillating with 2-3 Hz frequency now. I couldnít say when it started. But we didnít have this problem before. Then we took out the gun chamber several times to open the column for mechanical alignment and the polepiece replacement. Now, the voltage stability and emission stability are OK. Does anyone have had this problem or have any comment and suggestion on troubleshooting? Any comment and suggestion will be highly appreciated! Thank you very much!

Regards,
**************************************************
Qi Zhang, Ph.D
164 Phillips Hall, CB#3255
Department of Physics and Astronomy
the University of North Carolina at Chapel Hill
Chapel Hill, NC 27599
Tel: 919-843-2407 (Office)
919-843-0974 (EM Lab)
Fax: 919-962-0480
E-mail: qizhang-at-physics.unc.edu

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 11 07:52:06 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (balbrecht-at-nwicc.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Friday, December 10, 2004 at 12:46:18
---------------------------------------------------------------------------

Email: balbrecht-at-nwicc.edu
Name: Brian Albrecht

Organization: Northwest Iowa Community College

Education: Undergraduate College

Location: Sheldon, Iowa, United States

Question: I'm a science professor here at Northwest Iowa Community College. Our welding instructor, through the Department of Energy, obtained a Leitz Metallurgy microscope. No instructions came with the microscope. We are looking for a way of obtaining an instruction manual. The microscope does not have standard adapters for plugging into the wall. The adapter ends consist of a cylinder which house I believe 5 flat prongs probably no longer than a half an inch and no wider than probably a quater of an inch. The only number that was visible on the scope was 741390. Any assistance would be greatly appreciated. Thank you.

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From MicroscopyL-request-at-ns.microscopy.com Sun Dec 12 23:45:46 2004

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We would like to service and test an old Omar cpd after a couple of years
in a box. Is there a company or facility repairing/servicing/testing such a
unit?

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 08:16:32 2004

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It seems that the $10k asking price for the Electroscan was too rich for
the list. We are willing to take $5K from anyone willing to remove it and
enjoy the wonders of LVSEM! Don't forget about the HT stage, tensile stage
and peltier stage; you can do almost anything with this tool. And if you
just need parts for your ESEM $5K is really fair. Scrap metal prices are
really high now too, we just may take that route if someone doesn't make an
offer, so act now! What about that hard to buy for Uncle this holiday
season? Wouldn't he be surprised when you drop this off on his lawn? The
old guy needed a hobby anyway. The possibilities are endless, act now or
off to Finger Lakes Scrap with it!

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 09:04:09 2004

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Greetings,
Total internal reflectance microscopy (TIRF) provides resolution on the
order of tens of nanometers in the axial dimension. This is because of
a a phenomenon which occurs when the rays of excitation illumination are
glanced off of a reflective interface (an interface between differing
refractive indices) at an angle greater than the second refractive index
will accomodate (in other words, a much higher numerical aperture than
is possible to attain in the second refractive index). When light is
reflected off of an interface in this manner, a very small portion of
the media past the second refractive interface is illuminated by
evanescent waves from the illumination source. The intensity of
evanescent waves decays very rapidly so illumination is only intense
enough to excite fluorochromes to a depth of a few tens of nanometers.
This provides a means of determining that bright spots are localized to
very near the interface with a resolution which surpasses that of
conventional diffraction limited illumination schemes. An example of
this would be viewing the distribution of labeled proteins in the cell
membrane of cultured cells adhering to the coverslip.
To answer your question more directly, the big advantage of TIRF is
very high depth resolution at the coverslip/sample media interface. That
is the single big advantage. This means a very small sample volume can
be monitored and investigators can monitor molecules moving into and out
of this small volume. From these observations, calculations which
provide insight into molecular concentrations, whether or not the
movement of molecules appears to be random, correlation of spatial
relationships between (and colocalization among) different types of
molecules and other parameters can be conducted.
Cheers,
Karl

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 09:10:17 2004

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Attention all Electron Microscopists!

The Laboratory of Developmental Genetics at The Rockefeller
University seeks a full-time electron microscopist to assist in
studies of nervous system development and cell death in the nematode
C. elegans.

Work will involve preparing specimens for TEM, serial sectioning,
and 3-D image reconstructions. The successful candidate will become an
integral part of ongoing scientific efforts in the lab, and could also
pursue independent research. Previous experience with TEM is required,
and experience with serial sectioning experience a plus. Applicants
must hold a minimum of a Bachelor's degree.

We offer a competitive salary, comprehensive benefits, a gracious
working environment, and tuition reimbursement. For immediate
consideration, send resume/C.V. to: Ms. Kara R. Marshak, Senior
Employment Specialist, The Rockefeller University via fax (212)-327-
7079 or email marshak-at-rockefeller.edu. For more information about
ongoing research in this laboratory,please visit our website located
at http://www.rockefeller.edu/labheads/shaham/shaham-lab.php.

An Affirmative Action/Equal Opportunity Employer. The Rockefeller
University appreciates all responses and will contact candidates
selected for further consideration.

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 10:54:29 2004

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I never thought it would happen here but the prospect of inter
-departmental cross charging is being now being discussed. Does
anyone have recent experience of constructing a price list for;
Processing samples? for immunolabelling ? etc etc. Where is the best
place to start? I am not sure if we will have to charge to cover
consumables or entire costs.

Ken Blight
Senior Scientific Officer
Cancer Research UK

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 12:17:24 2004

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Greetings,
I'm looking for an incident fluorescence illumination system to retrofit
an old Olympus BH-2 stand. Any input as to where I might find such
parts in good conditions would be appreciated. Thanks.
Regards,
Karl

--
Karl Garsha
Light Microscopy Specialist
Imaging Technology Group
Beckman Institute for Advanced Science and Technology
University of Illinois at Urbana-Champaign
405 North Mathews Avenue
Urbana, IL 61801
Office: B650J
Phone: 217.244.6292
Fax: 217.244.6219
Mobile: 217.390.1874
www.itg.uiuc.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 15:25:50 2004

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Hi Ken,

I had to do this from scratch when I started here 5 years
ago. It can be quite simple. First, estimate hourly fee
for technical help by dividing average salary of technician
plus benefits by a reasonable estimate of billable hours
that a technician can provide. Don't be over-optimistic -
only a few hours a day can actually be billed for. A lot of
duties that cannot be accounted for (such as administrative
work, ordering, cleaning the lab up, teaching, answering
information requests, lab meetings, etc...). We came up
with a number of $40 an hour, but this is in fact too low
and we will review it upwards soon (should be at least
$50). Then estimate average amount of time required
for the tasks you want to start billing (for example: cryo-
sectioning / 1hour per sample - Immuno-labeling / 2 hours
per run, etc), add some cost for consumables (liquid
nitrogen, coated grids, antibodies, ...) and you can estimate
a reasonable charge.

For sectioning, you also need to take into consideration
the cost for diamond knives. Depending on the experience
of you staff (and the nature of the samples you will be cutting),
estimate how many samples in average you will be sectioning
with one diamond knife before it needs resharpening. People
have different opinions about when a knife needs resharpening,
but in my view if you are going to sell your sections at a hefty
price, they have to be perfect (NO knife marks!). We estimate
a cost of about $5 per sample just for the knife when we do the
cutting, and charge users $20 per hour for knife when they
cut themselves (sometimes literally!!). See it as a form of
insurance.

For instrument rental, we calculate a hourly rate by dividing
service contracts plus technician time required for routine
maintenance, by the total number of hours the instrument
will be used in the year (by our staff or outside users).

Some of our current charges:
Technician time: $41.50/hour
EM time (unassisted): $41.50/hour
EM time (assisted): $83/hour
Microtome rental: $15.50/hour
Cryo-microtome rental: $26/hour
Embedding: $36.50/sample
Sectioning: $52/sample
Cryo-sectioning: $93.50/sample
Single immuno-labeling: $125/run
Double immuno-labeling: $230/run
Prints: $6.50
EM negative: $1.60

We also have a "comprehensive" charge for regular or immuno-EM,
that comprises every step from fixation to the production of
publication-quality pictures. The cost is $155 for regular EM,
and $310 for immuno-EM (per sample).

Hope this helps.

Marc

On Monday, December 13, 2004, at 12:24 PM, Ken Blight wrote:

}
}
} -----------------------------------------------------------------------
} -------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of
} America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -----------------------------------------------------------------------
} --------
}
} I never thought it would happen here but the prospect of inter
} -departmental cross charging is being now being discussed. Does anyone
} have recent experience of constructing a price list for; Processing
} samples? for immunolabelling ? etc etc. Where is the best place to
} start? I am not sure if we will have to charge to cover consumables or
} entire costs.
}
} Ken Blight
} Senior Scientific Officer
} Cancer Research UK
}
}

--
Marc Pypaert
Department of Cell Biology
Center for Cell and Molecular Imaging
Ludwig Institute for Cancer Research
Yale University School of Medicine
333 Cedar Street, PO Box 208002
New Haven, CT 06520-8002
TEL 203-785 3681
FAX 203-785 7446

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 13 20:30:41 2004

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I'm trying to write a batch converter that will convert a Veeco format image
to something more universal, namely TIFF in ImageJ. Does anyone know the
compression used or has anything been done like this before?

Thanks
Thomas Sadowski
Southern Connecticut State University

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 06:42:06 2004

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I would like to know how I can find abstract of Meeting of Microscopy &
Microanalysis. I use Web of Science. However, I cannot find my abstracts. It
seems that Web of Science do not have information on Microscopy &
Microanalysis meeting. What database has the information? Please advise.

Thank you,
Hiromi Konishi
Indiana University

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 08:30:45 2004

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Hi All,

This subject has been discussed a few times here. When I saw the text
below in my latest NASA Tech Briefs INSIDER, I thought it may be of
interest to at least one of the listers, so copied it and am sending it
along. The copyright and subscription info is below, also. Enjoy...

DATA STORAGE
Will records stored on CD or DVD still be retrievable 10 or 20 years from
now?
Researchers at the National Institute of Standards and Technology (NIST)
tested
how well recordable optical disks made with different manufacturing
processes
held up to high temperatures, humidity, and light levels. Results showed
that
some disks perform better than others and that excessive exposure to any of
these conditions can accelerate deterioration.

To address how to identify those high-quality media for archival
applications,
NIST, along with the DVD Association (DVDA) and several government
agencies, has
formed the Government Information Preservation Working Group.

Working with the optical disk industry, the group is setting requirements
for
archival quality CD and DVD recordable media, and specifying the minimum
number
of years that they must last to meet the requirements. NIST is also
developing a
test that manufacturers can use to determine if CDs and DVDs meet the
criteria.

Read the complete story at: http://link.abpi.net/l.php?20041213A6

* * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * *
* *

Please let your colleagues know they too can receive the INSIDER free
of charge simply by sending an e-mail message to the address
Listserv-at-listserv.abpi.net with the text
SUBSCRIBE Insider Firstname Lastname
as the only text on the first line of the message body.

For information on how your company can sponsor future editions of the
INSIDER, e-mail joe-at-abpi.net .

Copyright (c) 2004 Associated Business Publications Intl.

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 12:17:43 2004

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Darrell writes ...

} This subject has been discussed a few times here. ...

It's still an open subject ...

} Read the complete story at: http://link.abpi.net/l.php?20041213A6

There is a PDF available if you follow the hyperlinks at the above URL ...
"Stability Comparison of Recordable Optical Discs - A Study of Error Rates
in Harsh Conditions". However, the disappointing point made in the summary
is:

"It is demonstrated here that CD-R and DVD-R media
can be very stable (sample S4 for CD-R and sample D2
for DVD-R). Results suggest that these media types
will ensure data is available for several tens of years
and therefore may be suitable for archival uses.
Unfortunately, it is very difficult for customers to
identify these more stable media."

Recognizing the better media sometimes requires software to know where the
media was manufactured. Another good source for manufacturer info can be
explored here:
http://www.digitalfaq.com/media/dvdmedia.htm

cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 14:36:39 2004

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Hello Fellow List Members,

I have a Leitz Ergolux microscope with a broken focus mechanism. It's at a
repair facility in Texas. The repair company says that Leica's parts website
reports that they no longer stock the two gears need for the repair of my
scope since the scope is at least 15 years old.

So I'm exploring two routes:

1. Find a used Ergolux body and retrieve the parts I need or swap my
objectives, head, stage, illuminator, etc. to the new body and use it
instead.

2. Either buy of-the-shelf gears from a gear parts company or have custom
gears machined to repair the Ergolux. The second part of this proposition is
the most expensive as it's custom, only yields the two gears I need while a
replacement body might hold other parts for future repairs. I've talked to a
gear manufacturing company in town (Phoenix) and they're saying to reverse
engineer the gears I need from scratch might be in the $500 range, which is
more than I want to pay for two gears less than 1" (25mm) in size.

Do any of you have a used Ergolux body that's collecting dust that you'd
sell for a reasonable price?

Do any of you know if any other Leitz scopes have a matching focus mechanism
where the gears can be interchanged with an Ergolux?

Or do you know of a gear parts company you can recommend that might stock
what I need?

Thanks for your help.

Doug Baldwin

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 15:19:18 2004

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Hello Everyone,

We are in urgent need of two boards for our Hitachi H7000 Transmission
Electron Microscope. Both boards are lens board. One board is called lens
STB, part no. 747-0708 and the other one is DC power supply PC3 (don't
know the part number).

If someone has the boards and is willing to sell them to us please contact
me off line as soon as possible. The scope has been down for about a month
now.

Thanks in advance.

Soumitra

*************************************************************
Soumitra Ghoshroy
College Associate Professor, Biology
Director, Electron Microscopy Lab
Box 3EML
New Mexico State University
Las Cruces, NM 88003
Tel: 505-646-3268 (office), 646-3283 (lab)
Fax: 505-646-3282
e-mail:sghoshro-at-nmsu.edu
http://biology-web.nmsu.edu/ghoshroy/ghoshroy.htm
http://emldata.nmsu.edu/eml/

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 16:49:28 2004

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Greetings

I know finding funding for new instruments is very competative, so if you
don't want to give away any secrets, I understand.

But, I am stuck. Folks are coming into my little multiuser lab and asking
how we can get some new equipment. None of them individually present the
critical mass needed to justify a microscope, but all together maybe they
have a point.

I have looked around and know about the NSF MRI program, but we missed the
deadline for this year and our campus may have different priorities for the
limited number of submissions they can do.

I know about the various NSF equipment programs, has anyone tried to do
this using PI's from multiple disciplines? I have users from Biology, Earth
Science, Chemistry, maybe some others, none which could do it on their own,
but together, maybe.

How about any other leads? As I said, don't give away the farm, but maybe
you could clue me in a little.

Thanks

Jon

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 14 21:33:49 2004

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Kia Ora

We have a researcher who would like to do some transmission electron
microscopy on synovial fluid from the knee. He is looking for debris
in the fluid after a particular surgical procedure. this debris will
not necessarily be cellullar, it may be from the superficial
cartilage layer.

We thought of either spinning the fluid down and processing the
pellet that may result, or perhaps smearing the fluid onto a coated
slide, fixing it and then doing the pop off technique.

Either way I imagine the amount of organic matter we are going to get
will be pretty small.

Has anybody out there got any suggestions or experience with the
transmission electron microscopy of 'clear' body fluids, ie synovial
fluid. I imagine cerebral spinal fluid would be pretty similar in
organic matter content.

I am not sure if we are going to run into problems with high protein
content in these fluids, perhaps masking the debris this researcher
is actually looking for, any thoughts?

Many thanks

Allan

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 06:08:15 2004

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A SEM we are purchasing has an application that does not require optimum gun
brightness, and for the sake of filament longevity (months of 24-7) runs the
filament heat at less than saturation and on top of the 1st peak.

I have always tought that the phenomenon of the 1st peak must be a result of
the Wehnelt's geometry as a function of heating and the zero-to-positive keV
potential moving towards the filament tip ... that is, a phenomenon of note
but not much more of a concern. Now, I find myself wanting of a better
understanding for the sake of beam current stability ... i.e., operating on
the first peak does not seem to be a very stable parameter for stable
emission.

The SEM itself is a FEI Quanta, which apparently has a method of regulating
the emission current. This must also play a role, and I haven't yet found a
explanation of how this works.

Any discussion towards enlightenment much appreciated.

Happy Holidays & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 07:08:53 2004

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------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Greetings

I know finding funding for new instruments is very competative, so if you
don't want to give away any secrets, I understand.

But, I am stuck. Folks are coming into my little multiuser lab and asking
how we can get some new equipment. None of them individually present the
critical mass needed to justify a microscope, but all together maybe they
have a point.

I have looked around and know about the NSF MRI program, but we missed the
deadline for this year and our campus may have different priorities for the
limited number of submissions they can do.

I know about the various NSF equipment programs, has anyone tried to do
this using PI's from multiple disciplines? I have users from Biology, Earth
Science, Chemistry, maybe some others, none which could do it on their own,
but together, maybe.

How about any other leads? As I said, don't give away the farm, but maybe
you could clue me in a little.

Thanks

Jon

Jonathan Krupp
Microscopy & Imaging Lab
University of California
Santa Cruz, CA 95064
(831) 459-2477
jmkrupp-at-cats.ucsc.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 07:55:43 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (Ntores-at-btconnect.com) from on Wednesday, December 15, 2004 at 05:29:58
---------------------------------------------------------------------------

Email: Ntores-at-btconnect.com
Name: Nicholas Tores

Organization: IPS

Title-Subject: [Microscopy] [Filtered] Fofler heating bench ( Heizbank German )

Question: We are looking to purchase a
Kofler Hotbench for thermal treatment of tiny specimens.
Can you help ?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 09:06:15 2004

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Hi All,

I received some nematodes for SEM. They are preserved in 96% ethanol. I have
no experience with this sort of organisms.
Can anyone please tell me how to proceed?

Thanks

-------------------------------------------------------------------------------
Renaat Dasseville
Ghent University - Dept. Biology
Sect. Protistology & Aquatic Ecology
Krijgslaan 281 - S8
B-9000 Gent
Belgium
tel.: +32-9-264.85.05
fax.: +32-9-264.85.99

Protistology website = http://www.pae.ugent.be/
-------------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 09:15:07 2004

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Jon,
The Core Facility Management at M&M 2004 dealt with this topic.
Representatives from NSF and NIH spoke on funding opportunities for major
equipment acquisition. It turns out that there are good opportunities for
both PhD granting and non-PhD granting institutions.

The session was taped and transcribed and the first segment (NIH
opportunities) will be published in Microscopy Today in the January issue.
Other segments will appear over the next few issues. Included will be
Questions & Answers that give a lot of suggestions to help make your grant
more competitive.

The NIH NCRR Major Equipment grant deadline is mid-March so you will see
that article in plenty of time. NSF deadlines for the MUE program (biology)
and the IMR (Instrumentation for materials Research) are in early October.

One thing that was strongly encouraged was to call the NSF program director
where you think you would best fit and talk to that individual. They can
guide you as to what division would be most appropriate for your proposal
and assist in answering many other questions regarding writing a successful
proposal.

One new development that you may not be aware of is that NSF is dropping the
required 30% match for major equipment proposals. They are also increasing
the maximum for the MUE and IMR programs from $400,000 to $500,000. This
should help a lot when you try to round up funds for the more expensive
instruments.

Debby

Debby Sherman, Manager Phone: 765-494-6666
Life Science Microscopy Facility FAX: 765-494-5896
Purdue University E-mail: dsherman-at-purdue.edu
S-052 Whistler Building
170 S. University Street
West Lafayette, IN 47907
http://www3.agriculture.purdue.edu/microscopy

On 12/14/04 6:17 PM, "Jon Krupp" {jmkrupp-at-cats.ucsc.edu} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
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------------------------------------------------------------------------------}
-
}
} Greetings
}
} I know finding funding for new instruments is very competative, so if you
} don't want to give away any secrets, I understand.
}
} But, I am stuck. Folks are coming into my little multiuser lab and asking
} how we can get some new equipment. None of them individually present the
} critical mass needed to justify a microscope, but all together maybe they
} have a point.
}
} I have looked around and know about the NSF MRI program, but we missed the
} deadline for this year and our campus may have different priorities for the
} limited number of submissions they can do.
}
} I know about the various NSF equipment programs, has anyone tried to do
} this using PI's from multiple disciplines? I have users from Biology, Earth
} Science, Chemistry, maybe some others, none which could do it on their own,
} but together, maybe.
}
} How about any other leads? As I said, don't give away the farm, but maybe
} you could clue me in a little.
}
} Thanks
}
} Jon
}
} Jonathan Krupp
} Microscopy & Imaging Lab
} University of California
} Santa Cruz, CA 95064
} (831) 459-2477
} jmkrupp-at-cats.ucsc.edu
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 09:32:23 2004

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Bonjour everyone!
I had a question from a prof I couldn't answer and was wondering if you
could help. He has a couple of diamond knives he wants sharpened
(Diatome). He asked me if he could get the work done in Canada. I
have always sent my knives back to the manufacture. Has anyone out
there ever gotten a knife sharpened in Canada and if yes, let me know
about it....You could also contact me off line if you wish. Merci..

André Dufresne
University of Manitoba
Botany Dept.
Dufresne-at-ms.umanitoba.ca

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 09:54:59 2004

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Allan,

Another option would be to use a cytospin to concentrate the material on the
slide; then invert a beem capsule over it and process for TEM.

Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (W224)
Massachusetts General Hospital
55 Fruit Street
Boston, MA 02114
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-3192 (fax)
msherwood-at-partners.org

-----Original Message-----
} From: Allan Mitchell [mailto:allan.mitchell-at-stonebow.otago.ac.nz]
Sent: Tuesday, December 14, 2004 11:04 PM
To: microscopy-at-msa.microscopy.com

Kia Ora

We have a researcher who would like to do some transmission electron
microscopy on synovial fluid from the knee. He is looking for debris
in the fluid after a particular surgical procedure. this debris will
not necessarily be cellullar, it may be from the superficial
cartilage layer.

We thought of either spinning the fluid down and processing the
pellet that may result, or perhaps smearing the fluid onto a coated
slide, fixing it and then doing the pop off technique.

Either way I imagine the amount of organic matter we are going to get
will be pretty small.

Has anybody out there got any suggestions or experience with the
transmission electron microscopy of 'clear' body fluids, ie synovial
fluid. I imagine cerebral spinal fluid would be pretty similar in
organic matter content.

I am not sure if we are going to run into problems with high protein
content in these fluids, perhaps masking the debris this researcher
is actually looking for, any thoughts?

Many thanks

Allan

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 10:32:43 2004

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Dear Renaat,

If you go to our website at www.wormatlas.org you will see a listing
for "Anatomical Methods" for the study of the nematode. In this
listing, there is a detailed protocol for doing SEM on the nematode,
or even on dissected organs from the nematode.

Other portions of our website will help to inform you about the
various tissues that you might encounter, but you may especially want
to read the "Cuticle" chapter in the Handbook.

Good luck!

Dave Hall
--
David H. Hall, Ph.D.
Center for C. elegans Anatomy
Department of Neuroscience
Albert Einstein College of Medicine
1410 Pelham Parkway
Bronx, NY 10461

www.wormatlas.org
www.aecom.yu.edu/wormem

phone 718 430-2195
fax 718 430-2514

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 10:48:23 2004

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Dear Michael,
When I need long-term SEM gun stability and long filament life, I use a well
under-saturated filament. I don't think the first peak is stable enough. On
my Hitachi instruments, I can use "filament image" mode to see an image of
the filament tip, and back off the heating current until I have a nice
doughnut with a dark centre. You can also use the waveform mode to determine
the zero-emission level and the fully saturated level, then back off about
10 % of that range from the saturation point. This is above the exponential
slope of filament brightness, when the saturation curve starts to curve
over, and is fairly stable over days.
Good luck.
Regards,
Mary Mager
Electron Microscopist
Department of Materials Engineering
University of British Columbia
6350 Stores Road
Vancouver, B.C. V6T 1Z4
CANADA
Tel: 604-822-5648
Fax: 604-822-3619
e-mail: mager-at-interchange.ubc.ca
----- Original Message -----
} From: "michael shaffer" {michael-at-shaffer.net}
To: "Microscopy list" {Microscopy-at-MSA.Microscopy.Com}
Sent: Wednesday, December 15, 2004 4:38 AM

Hello,

We are setting up a modest microscopy suite in our dept and are in need of a used glass knifemaker. Anyone know of a good source, or have a used one for purchase? You may respond to me personally, rather than the list.

Thanks,
Heidi

Heidi A. Kratsch, Ph.D.
Assistant Professor/Extension Ornamental Horticulture Specialist
Utah State University
Department of Plants, Soils & Biometeorology
4820 Old Main Hill
Logan, UT 84322-4820
Phone: 435-797-8124
Mobile: 435-760-5611
Fax: 435-797-3376
Email: heidik-at-ext.usu.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 11:58:01 2004

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Hi Michael,

What you are saying (to use the first peak) is new to me. I have a XL30
ESEM, Quanta's senior generation. Yes, there is a way to limit the
filament current; but you have to adjust it from time to time. I am
talking about the second peak here.
I find that the auto saturation is usually over-done after I have had a
few burned out prematurely.
These days, I let the machine do auto saturation when it is new. I check
it within 10 min to lower the LIMIT setting. The saturation point drops
very quickly for the first few days, so I keep checking it to prolong
it's life. I had one lasted for 6 months; mostly 2-3 months and the rest
can be anywhere down to few days when I neglected to check the filament.
I hope this helps.

Ann Fook Yang

-----Original Message-----
} From: michael shaffer [mailto:michael-at-shaffer.net]
Sent: Wednesday, December 15, 2004 7:39 AM
To: Microscopy list

A SEM we are purchasing has an application that does not require optimum
gun
brightness, and for the sake of filament longevity (months of 24-7) runs
the
filament heat at less than saturation and on top of the 1st peak.

I have always tought that the phenomenon of the 1st peak must be a
result of
the Wehnelt's geometry as a function of heating and the zero-to-positive
keV
potential moving towards the filament tip ... that is, a phenomenon of
note
but not much more of a concern. Now, I find myself wanting of a better
understanding for the sake of beam current stability ... i.e., operating
on
the first peak does not seem to be a very stable parameter for stable
emission.

The SEM itself is a FEI Quanta, which apparently has a method of
regulating
the emission current. This must also play a role, and I haven't yet
found a
explanation of how this works.

Any discussion towards enlightenment much appreciated.

Happy Holidays & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 12:04:41 2004

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Hi Allan

In the early 1970s I worked with the group from St Bartholomew's Hospital,
London, to publish the first papers on crystal deposition disease. Look up
Crocker, Leverson et al for help with the problems that you have. We worked
on synovial fluid from the knee so you should find a good deal of help in
this area.

Regards

Steve Chapman
Senior Consultant Protrain
For electron microscopy consultancy and training world wide
www.emcourses.com tel +44 1280 816512 fax +44 1280 814007

----- Original Message -----
} From: "Allan Mitchell" {allan.mitchell-at-stonebow.otago.ac.nz}
To: {microscopy-at-msa.microscopy.com}
Sent: Wednesday, December 15, 2004 4:03 AM

Hi Michael

The 1950s conventional wisdom as to the setting of the filament was to
move onto the plateau of the heating/signal level graph as the filament
heating current was often unstable. This procedure overcame intensity
changes should the filament heating current change.

As years have gone by and improvements have been made this "overkill",
in more ways than one, has been corrected. Many manufacturers suggest
running at first peak when ever possible and even the purest amongst us
have run for a number of years in this way.

What about stability you may say? Well set a TEM on what would be first
peak (maximum screen intensity when heating the filament) and watch the
virtual source. I think you will become more likely to develop eye
strain than the source will change in form; the stability is amazing!

I back this observation by my experiences with instruments that judge
image brightness in the search for heavy elements in the mining
industry. These automated instruments work 24 hours a day and must
remain stable in order to have a constant probe current and hence a
constant range of grey levels in order to carry out their tasks; the
elemental composition is judged by grey level through BSE.

I would also add that running on first peak on a modern instrument
offers remarkable results; 150,000X being not out of the question (15kV
10mm WD).

I have not and cannot explain first peak but I can say on a modern
instrument it produces a very satisfactory source at } 10kV.

Regards
Steve Chapman
Protrain for Training and Consultancy in Electron Microscopy World Wide
www.emcourses.com

-----Original Message-----
} From: michael shaffer [mailto:michael-at-shaffer.net]
Sent: 15 December 2004 12:39
To: Microscopy list

A SEM we are purchasing has an application that does not require optimum
gun
brightness, and for the sake of filament longevity (months of 24-7) runs
the
filament heat at less than saturation and on top of the 1st peak.

I have always tought that the phenomenon of the 1st peak must be a
result of
the Wehnelt's geometry as a function of heating and the zero-to-positive
keV
potential moving towards the filament tip ... that is, a phenomenon of
note
but not much more of a concern. Now, I find myself wanting of a better
understanding for the sake of beam current stability ... i.e., operating
on
the first peak does not seem to be a very stable parameter for stable
emission.

The SEM itself is a FEI Quanta, which apparently has a method of
regulating
the emission current. This must also play a role, and I haven't yet
found a
explanation of how this works.

Any discussion towards enlightenment much appreciated.

Happy Holidays & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
{www.micro-investigations.com}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 12:38:12 2004

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If you've got enough brightness to spare, why not run it in the valley between the
1st peak and the 'plateau'?

Better stability than the 1st peak, in my JEOL 840 experience (think of the
mechanical analogue), and certainly longer filament life thjan the 'plateau', but I
think both the 1st peak and the valley give a slightly larger spot than the 'plateau'.

cheers

rtch

} From: "michael shaffer" {michael-at-shaffer.net}
To: "Microscopy list" {Microscopy-at-MSA.Microscopy.Com}

} Hello Listers:
}
} I have two multi-packs boxes (250 sheets per pack) of the small sized 6.5
} x 9 cm. 4489 film. It has an expiration of 12/2004 but has been stored in
} a cool dry place. Anyone out there interested in it? Normally it sells
} in the catalogs for $ 97.00 for 100 sheets. I would sell the 250 boxes
} for $50.00 each plus shipping costs. Anyone need film out there?
}
} Karen
}
} Karen L. Bentley, M.S.(previously Jensen)
} Associate Scientist & Project Manager
} Electron Microscope Research Core
} University of Rochester Medical Center
} Rochester, NY 14642
} 585-275-1954
}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 14:12:56 2004

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Jan writes ...

} On our older ISI, the signal is greatly increased when you go
} from the first peak to the edge of the plateau (typical
} saturation point). Even if adequate image brightness is achieved
} on some SEMs at the first peak, am I wrong to think that more
} signal means better S:N ratio, and therefore a better quality
} image? And am I wrong to think that the only advantage to heating
} the filament only to the first peak is increased filament life
} (but at the expense of image quality)? Or are these more modern
} SEMs very different from the older models?

I believe you are correct on both counts ... leastwise, I am not yet
convinced what Steve implies below ... i.e., that emission from the cathode
at 1st peak is equally bright as when saturated. Regarding signal/noise, do
not confuse "spot brightness" with "beam current". For sure, increasing
either results in better s/n ... but brightness is a function of your gun
emission, and once your gun is properly saturated (whatever method), it is
your beam current setting (e.g., spot size) which, in practice, controls
your s/n. (except of course, your choice of final aperture)

cheerios :o)

} Steve Chapman wrote:
} ------------------------------------------------------------------
} ------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ------------------------------------------------------------------
} -------------
}
} Hi Michael
}
} The 1950s conventional wisdom as to the setting of the filament was to
} move onto the plateau of the heating/signal level graph as the filament
} heating current was often unstable. This procedure overcame intensity
} changes should the filament heating current change.
}
} As years have gone by and improvements have been made this "overkill",
} in more ways than one, has been corrected. Many manufacturers suggest
} running at first peak when ever possible and even the purest amongst us
} have run for a number of years in this way.
}
} What about stability you may say? Well set a TEM on what would be first
} peak (maximum screen intensity when heating the filament) and watch the
} virtual source. I think you will become more likely to develop eye
} strain than the source will change in form; the stability is amazing!
}
} I back this observation by my experiences with instruments that judge
} image brightness in the search for heavy elements in the mining
} industry. These automated instruments work 24 hours a day and must
} remain stable in order to have a constant probe current and hence a
} constant range of grey levels in order to carry out their tasks; the
} elemental composition is judged by grey level through BSE.
}
} I would also add that running on first peak on a modern instrument
} offers remarkable results; 150,000X being not out of the question (15kV
} 10mm WD).
}
} I have not and cannot explain first peak but I can say on a modern
} instrument it produces a very satisfactory source at } 10kV.
}
} Regards
} Steve Chapman
} Protrain for Training and Consultancy in Electron Microscopy World Wide
} www.emcourses.com
}
}
} -----Original Message-----
}
} From: michael shaffer [mailto:michael-at-shaffer.net]
}
} Sent: 15 December 2004 12:39
} To: Microscopy list
} Subject: [Microscopy] SEM: gun saturation
}
}
}
} ------------------------------------------------------------------------
} ------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} ------------------------------------------------------------------------
} -------
}
}
} A SEM we are purchasing has an application that does not require optimum
} gun
} brightness, and for the sake of filament longevity (months of 24-7) runs
} the
} filament heat at less than saturation and on top of the 1st peak.
}
} I have always tought that the phenomenon of the 1st peak must be a
} result of
} the Wehnelt's geometry as a function of heating and the zero-to-positive
} keV
} potential moving towards the filament tip ... that is, a phenomenon of
} note
} but not much more of a concern. Now, I find myself wanting of a better
} understanding for the sake of beam current stability ... i.e., operating
} on
} the first peak does not seem to be a very stable parameter for stable
} emission.
}
} The SEM itself is a FEI Quanta, which apparently has a method of
} regulating
} the emission current. This must also play a role, and I haven't yet
} found a
} explanation of how this works.
}
} Any discussion towards enlightenment much appreciated.
}
} Happy Holidays & cheerios ... shAf :o)
} Avalon Peninsula, Newfoundland
} {www.micro-investigations.com}
}
}
}
}
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 14:20:20 2004

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Hello experts. I have an application where I need a very hard resin
formulation. I had been using Mollenhauer Araldite-Epon mixture using
BDMA as the accelerator. This formulation is not hard enough.
I am working with zebrafish which needs a prolonged infiltration schedule.
I cannot use Spurr as I am very allergic to it. I tried the embed-it resin
(a spurr like low viscosity mixture) with unpredictable results.
Can anyone recommend a hard formulation that infiltrates tissue well using
either Epon or Araldite? I plan to try the distilled DDSA that should
infiltrate well.
Thanks for your suggestions.
JoAnn Buchanan

Department of Molecular and Cellular Physiology
Stanford University School of Medicine
Stanford, CA 94305
650-723-5856

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 21:48:32 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mourad.idir-at-synchrotron-soleil.fr) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, December 15, 2004 at 14:14:30
---------------------------------------------------------------------------

Email: mourad.idir-at-synchrotron-soleil.fr
Name: mourad

Title-Subject: [Microscopy] [Filtered] CCD microscopy

Question: Dear All
I had the following questions
1--
Suppose we used A system with a CCD camera with 10 microns pixels size (1000x1000 pixels) and Microscope objective: "10X" with 0.1 NA
This means that we will have a field of view of 1 x 1 mm and an effective pixel size of 1 micron.
NA= 0.2 give a diffraction limited resolution of about 0.61x0.55/0.1=3.355 microns.
If I understand correctly there is no need to have an objective with a x20 but it is better to have an objective with a x10 and higher NA.
If we do the reverse calculation, we nedd two pixels for the resolution (Nyquist theorem) : 2 x10 microns pixel / (x10)=2 microns effective in the object plan so we need a NA of about NA=0.61x 0.5 / 2 = 0.168.
With this I do not need to get a higher magnification because it is the pixel camera who limit the resolution of the image
IS THAT CORRECT?

2--
The Depth of Field in an optical system is lambda/NA^2 = 0.5/(0.2)^2 = 12.50 microns.
So if I have a sample who is emmiting light in 10 microns thickness this will limit the resolution in my image.
This means that the image resolution in our case is limited to this Depth of Field so around 10 µm.

In other word, if we have a sample thickness of 10 µm this will limit the resolution but if we have a sample thickness equal to 2 microns we will have 2 microns resolution
IS THAT CORRECT?
Thanks for you reply
Regards

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 15 21:53:25 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kalyani-at-jncasr.ac.in) from http://www.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Wednesday, December 15, 2004 at 09:11:03
---------------------------------------------------------------------------

Email: kalyani-at-jncasr.ac.in
Name: kalyani

Organization: JNCASR

Education: Graduate College

Location: Bangalore, Karnataka

Question: Sir,

} From an HREM image of a nanowire i am getting a d-spacing which shows up neither in the SAED pattern nor in the XRD pattern. even other HREM images of nanowires of the same sample also show that d-spacing itself. but in the XRD pattern, a peak with half of the d-spacing that is calculated from the HREM image,is present. is there any particular reason for this observation. if yes, could u please give some egs as well as references.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 08:19:22 2004

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}
} Jan writes ...
}
} } On our older ISI, the signal is greatly increased when you
} go from the
} } first peak to the edge of the plateau (typical saturation
} point). Even
} } if adequate image brightness is achieved on some SEMs at the first
} } peak, am I wrong to think that more signal means better S:N
} ratio, and
} } therefore a better quality image? And am I wrong to think that the
} } only advantage to heating the filament only to the first peak is
} } increased filament life (but at the expense of image
} quality)? Or are
} } these more modern SEMs very different from the older models?
}
} I believe you are correct on both counts ... leastwise, I
} am not yet convinced what Steve implies below ... i.e., that
} emission from the cathode at 1st peak is equally bright as
} when saturated. Regarding signal/noise, do not confuse "spot
} brightness" with "beam current". For sure, increasing either
} results in better s/n ... but brightness is a function of
} your gun emission, and once your gun is properly saturated
} (whatever method), it is your beam current setting (e.g.,
} spot size) which, in practice, controls your s/n. (except of
} course, your choice of final aperture)

I believe the quality of the signal and stability from the first peak
depend
very much on instrument in use. But I have not found a single microscope
stable enough on the first peak for prolonged EDS or WDS analysis.
So, while image quality could be satisfactory with the gun at the first
peak, for proper microanalysis gun saturation is a necessity.

} cheerios :o)
}
} } Steve Chapman wrote:
} } ------------------------------------------------------------------
} } ------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of
} } America To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} } http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } ------------------------------------------------------------------
} } -------------
} }
} } Hi Michael
} }
} } The 1950s conventional wisdom as to the setting of the
} filament was to
} } move onto the plateau of the heating/signal level graph as the
} } filament heating current was often unstable. This
} procedure overcame
} } intensity changes should the filament heating current change.
} }
} } As years have gone by and improvements have been made this
} "overkill",
} } in more ways than one, has been corrected. Many
} manufacturers suggest
} } running at first peak when ever possible and even the
} purest amongst
} } us have run for a number of years in this way.
} }
} } What about stability you may say? Well set a TEM on what would be
} } first peak (maximum screen intensity when heating the filament) and
} } watch the virtual source. I think you will become more likely to
} } develop eye strain than the source will change in form; the
} stability
} } is amazing!
} }
} } I back this observation by my experiences with instruments
} that judge
} } image brightness in the search for heavy elements in the mining
} } industry. These automated instruments work 24 hours a day and must
} } remain stable in order to have a constant probe current and hence a
} } constant range of grey levels in order to carry out their
} tasks; the
} } elemental composition is judged by grey level through BSE.
} }
} } I would also add that running on first peak on a modern instrument
} } offers remarkable results; 150,000X being not out of the question
} } (15kV 10mm WD).
} }
} } I have not and cannot explain first peak but I can say on a modern
} } instrument it produces a very satisfactory source at } 10kV.
} }
} } Regards
} } Steve Chapman
} } Protrain for Training and Consultancy in Electron Microscopy World
} } Wide www.emcourses.com
} }
} }
} } -----Original Message-----
} }
} } From: michael shaffer [mailto:michael-at-shaffer.net]
} }
} } Sent: 15 December 2004 12:39
} } To: Microscopy list
} } Subject: [Microscopy] SEM: gun saturation
} }
} }
} }
} }
} ----------------------------------------------------------------------
} } --
} } ------
} } The Microscopy ListServer -- Sponsor: The Microscopy
} Society of America
} } To Subscribe/Unsubscribe --
} } http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help
} http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
} --------------------------------------------------------------
} ----------
} } -------
} }
} }
} } A SEM we are purchasing has an application that does not require
} } optimum gun brightness, and for the sake of filament
} longevity (months
} } of 24-7) runs the
} } filament heat at less than saturation and on top of the 1st peak.
} }
} } I have always tought that the phenomenon of the 1st peak must be a
} } result of the Wehnelt's geometry as a function of heating and the
} } zero-to-positive keV
} } potential moving towards the filament tip ... that is, a
} phenomenon of
} } note
} } but not much more of a concern. Now, I find myself wanting
} of a better
} } understanding for the sake of beam current stability ...
} i.e., operating
} } on
} } the first peak does not seem to be a very stable parameter
} for stable
} } emission.
} }
} } The SEM itself is a FEI Quanta, which apparently has a method of
} } regulating the emission current. This must also play a role, and I
} } haven't yet found a
} } explanation of how this works.
} }
} } Any discussion towards enlightenment much appreciated.
} }
} } Happy Holidays & cheerios ... shAf :o)
} } Avalon Peninsula, Newfoundland
} } {www.micro-investigations.com}
} }
} }
} }
} }
} }
} }
} }
}
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 09:07:07 2004

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Araldite tends to make a softer resin. For hard tissue, I use:

Epon 40g
DDSA 10g
NMA 20g

Infiltrate with this mix for some time with several changes, then add DMP30
2% to the pre-mixed Epon, mix even more thoroughly and infiltrate for a
further period before embedding in fresh Epon + DMP30 mix. The NMA (nadic
methyl anhydride) makes the polymerised resin much harder than normal Epon.

Lesley Weston.

on 15/12/2004 12:50 PM, JoAnn Buchanan at redhair-at-stanford.edu wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe --
} http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
}
----------------------------------------------------------------------------
--} -
}
} Hello experts. I have an application where I need a very hard resin
} formulation. I had been using Mollenhauer Araldite-Epon mixture using
} BDMA as the accelerator. This formulation is not hard enough.
} I am working with zebrafish which needs a prolonged infiltration schedule.
} I cannot use Spurr as I am very allergic to it. I tried the embed-it resin
} (a spurr like low viscosity mixture) with unpredictable results.
} Can anyone recommend a hard formulation that infiltrates tissue well using
} either Epon or Araldite? I plan to try the distilled DDSA that should
} infiltrate well.
} Thanks for your suggestions.
} JoAnn Buchanan
}
} Department of Molecular and Cellular Physiology
} Stanford University School of Medicine
} Stanford, CA 94305
} 650-723-5856
}
}

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 09:20:41 2004

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Hi

I have some nice pictures taken on the first peak where one can see the
same objets twice or three times a bit shifted one from the other. Setting
the filament current to saturation, one see that one image dominate, while
the others are disapering.

The explanation is that there are some hot points on the filament, hot
enough to emit, and so there are two or three emission points. With more
current the filament tip become more homogeneous in temperature, and at
saturation there is only the tip which is the emitting point (in
combination of the wehnelt polarisation). With time, evaporation and
annealing of the W make that the surface of the filament become smoother,
and so these points will desapear.

The ability to work on the first peak or on the plateau depends more of
the quality of the W wire used to make the filament, and of the annealing
effect of a few hours of work, than of the age/generation of the
microscope. It's the same question thant the lifetime of the filaments.
Depends on how the microsope is driven, but on the filament quality too.

On our Auger e-guns, we never work at saturation, and filament hold 10 to
15 years. But there is no image, and the shape of the electron spot
does'nt matter. We need only electrons at ŕ given energy and current.

On the other hand, if the first peak is economically interesting, its
shape, position an intensity often change during the life of the filament.
Sometimes it's very difficult to see it, sometimes it has a very strong
intensity... For a beginner, it can give headache to find it. Saturation
is easier. Over saturation too !

J. Faerber
IPCMS-GSI
(Institut de Physique et Chimie des Matériaux de Strasbourg
Groupe Surface et Interfaces)
23, rue de Loess ; BP43
67034 Strasbourg CEDEX 2
France

Tel 00 33(0)3 88 10 71 01
Fax 00 33(0)3 88 10 72 48
E-mail Jacques.Faerber-at-ipcms.u-strasbg.fr

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 11:52:01 2004

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hello,

according to manufacturer's instruction (SERVA, leaflet dated 1997), the
very hard grade Glycid ether 100 resin (equivatent to the former Epon 812)
is obtained as follows:

52.9 ml of glycid ether
47.1 ml MNA
mix thoroughly, then add 1.5 ml DMP-30 (or 2,4,6 trisphenol...), again mix
thoroughly

polymerisation: 20 h at 45oC, then 24 h at 60oC

I wish you success :-)
Barbara Lotocka

dr Barbara Łotocka
Department of Botany
Faculty of Agriculture and Biology
Warsaw Agricultural University
Nowoursynowska 159
02-776 Warsaw, Poland

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 11:58:11 2004

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Dear Renaat,

What type of info are you looking for from your image?

Last week at Cell Bio, I had a chance to see the new integration of NTMDT's
atomic force microscope with a microtome. Dr. Anton Efimov, the inventor,
had prepared a nematode using the normal freeze substitution protocols for
TEM and then had done a serial section and 3D reconstruction, using a
diamond knife. Because the knife cuts so cleanly, there is no topography
info to be gathered. However, the AFM has the capability to image using
local elasticity. The results were intriguing.

If you are interested in further info, I'd suggest you correspond directly
with Dr. Efimov (efimov-at-ntmdt.ru).

Hope this was helpful,

Best regards,
Barbara Foster
Microscopy/Microscopy Education

We've moved!
313 S Jupiter Rd, Suite 100
Allen, TX 75002
P: 972-954-8011
W: www.MicroscopyEducation.com

P. S.
Need a good general reference or light microscopy text? Visit our website
to learn more about "Optimizing LIght Microscopy". Copies still available
through MME... even for class-room lots ... and we give quantity discounts.

Caveat: MME has financial interest in this product.
At 09:36 AM 12/15/2004, Renaat Dasseville wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 15:58:40 2004

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For others who may have spectrometer interfaces which use the old ISA slots, but
wish to upgrade their computers, Soltek now makes a motherboard (SL-XP865G-
3IG) which uses the Intel 865G chipset, has FSB of 400, 533, or 800MHz,
supports Pentium 4 CPU, and has 4 PCI and 3 ISA slots.

It also has integrated graphics, a LAN port, and 4 integrated USB 2.0 ports, but no
built-in sound.

I have no connection with Soltek or its agents, except as a satisfied customer.

cheers

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 16 17:47:27 2004

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Ritchie Sims wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 04:27:48 2004

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Steve Chapman writes ...

} [...]
} I thought the point of the original question was to determine
} our experiences of using the desaturated filaments and the
} stabilities involved?
} In which case the experiences with these automated instruments
} running desaturated would confirm a high stability over a period
} of up to 24 hours.
} [...]

My original question was for better understanding the phenomenon of the 1st
peak. What's going on with electron emission with changing equipotential
voltage influences? Why don't we see the monotonic rise as described by
"self-biasing", but instead hills and valleys? I was hoping someone had
written it up as something other than a curiosity. For example, modifying
the cathode-Wehnelt distance may have some influence on the 1st peal,
possibly making it a more stable point of heating.

I think most would agree ... putting filament heat on top of the 1st peak is
not the most stable situation for long term electron emission. The
instruments I am just now becoming more familiar with employ the ability to
measure the beam current with regularity, and to digitally optimize the heat
(find the top of the 1st peak), and control the first lens for making the
beam current what it should be. These algorithms takes only a few seconds,
but allow for the gun being almost maintenance-free while emitting
equivelent current. This is somewhat different than relying on the inherent
stability of the emission plateau (saturation) ... and also different from
the method employed by microprobes which compensate with the first lens
only.

I should now remain quiet until I have actually had my hands on with these
SEMs. Still, when I'll need manage and teach these instruments, I'll be
wanting for a better explanation of the "1st peak".

happy holidays & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 06:43:47 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (thokar7-at-in.gr) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Friday, December 17, 2004 at 03:47:14
---------------------------------------------------------------------------

Email: thokar7-at-in.gr
Name: Thomas Karras

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Which is the best optical microscope in market in order to view microstructure of martensitic stainless steel?

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 08:19:40 2004

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Hi Listers,

{tongue-in-cheek mode ON}

I was just browsing through my newly arrived Nov 2004 copy of Microscopy
Today
and found something that has deeply shaken my confidence in my
instrument and
ability to operate it. The back inside cover (an ad for an SEM
manufacturer who
shall remain nameless) displays a very colorful FE-SEM image of Paralia
sulcata (Phytoplankton),
measuring some hundreds of microns across and looking nothing like the
specimens of the same
species I routinely image with my lowly tungsten-based instrument
(see http://www.mta.ca/dmf/wii23.htm for what I'm used to seeing).

It would appear that my SEM is generating not only a thoroughly spurious
image, but also my
magnification calibration is off by a factor of something like 300.

I understand that image quality is a function of the cost of the
instrument, but the differences
here are much more extreme than I ever appreciated. Why, it's like the
two instruments
are not even examining specimens for the same Kingdom! I guess my
problem also
stems from the fact that I can only rely on the 30+ years of expertise
my wife (and collaborator)
has in phytoplankton research, compared to the research budget of a
heavy industry that is
larger than the National Science Foundation. Obviously, I need to invest
in better instrumentation. If one of the vendors will agree to fly me to
Hawaii for the
MSA meeting this summer, I'll almost certainly buy a new FE-SEM from them!

{tongue-in-cheedk mode OFF}

Wishing everyone a Happy (and Accurate) Holiday season,

Jim

--

James M. Ehrman
Digital Microscopy Facility
Mount Allison University
Sackville, NB E4L 1G7
CANADA

phone: 506-364-2519
fax: 506-364-2505
email: jehrman-at-mta.ca
www: http://www.mta.ca/dmf

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 09:18:13 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Listers,
Our facility has an Ilford print processor which is not working. Parts are no longer available and so I'm looking for a replacement. The majority of our users use the digital camera but we have a few holdouts who want film. Can any of you recommend a black and white processor?

Thanks,

Mary Gail Engle
Laboratory Manager
Electron Microscopy & Imaging Facility
University of Kentucky
Lexington, KY 40536

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 09:58:32 2004

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i am no whale expert but the humpback whale in the accompanying photo is
also a tad larger than I would have guessed. The flukes look to span over
20 meters...

At 08:49 AM 12/17/04, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Thomas E. Phillips, PhD
Professor of Biological Sciences
Director, Molecular Cytology Core
3 Tucker Hall
University of Missouri
Columbia, MO 65211-7400

573-882-4712 (office)
573-882-0123 (fax)
PhillipsT-at-missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 10:50:10 2004

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When Jerry Sedgewick's articles first appeared in Microscopy Today, I wrote a
lengthy correction to some of his misinformation and sent it to Ron Anderson.
There was no reply, and nothing appeared in the magazine, but Ron later told
me he had forwarded the letter to Jerry, who has never responded. Realizing
that the magazine is not a referreed journal and probably isn't taken very
seriously anyway, I put the continuing errors in the series of artices in the
category of a minor annoyance.

But in the most recent issue, at the end of Jerry's article, he has inserted
the statement 'Note: More thorough explanations of the concepts presented in
this article can be found in "The Image Processing Handbook" by John Russ.' By
invoking my name and book in an apparent attempt to gain some credibility for
the article, which is almost entirely incorrect and misleading, that statement
requires an answer.

First, the cited book does not discuss the subject of matching the appearance
of images on printouts and the computer screen. I have written in another
book on that topic, but the bible on the subject can be found in David Blatner
and Bruce Fraser's "Real World Photoshop" (Peachpit Press). Another excellent
choice for anyone concerned about doing this right is to get either the
GretagMacbeth Eye-One (my preference) or ColorVision Spyder calibration hardware and
software, and follow the straightforward procedures which will make sure that
your display, printout, and even projector all show the same thing.

The Sedgewick article is completely wrong (as usual). The International Color
Consortium begun by companies like HP and Apple has constructed a technically
sound and easily implemented framework that allows manufacturers of software
(e.g., Photoshop), hardware (display cards, monitors, printers) and
consumables (ink, paper) to provide widely available curves that everyone should use.
Bypassing this (per Jerry's recommendation) and attempting to adjust the image
or the monitor to make images more dramatic is a bad idea. Altering the
contrast of "scientific" images as compared to normal photography is nonsense. Ink
jet printers are fine and have their place, but are certainly not the only way
to get good output. The article has plenty of other, more subtle errors (e.g.,
the dialog shows that sRGB color space is being used, instead of one such as
Adobe 1998 with its greater gamut).

Ignore the article. In fact, ignore all of the Sedgewick articles about
Photoshop. Even in those cases where the instructions are not wrong, they are not
the best way to accomplish a given result. Go read a good book. There are lots
of them, written by people who actually know what they are writing about.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 11:18:29 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello,

We have a See Vac Critical Point Dryer in need of repair. Does anyone
know of a third party company that performs repairs on these devices.

Karl Hagglund
Biological Sciences
Northern Kentucy University

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 11:21:15 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Jim,

You've let the cat out of the bag. That's actually a secret image of
a new, planktonic mutant of Arabidopsis, showing a trichome
engineered to increase the plant's buoyancy.

Phil

} Hi Listers,
}
} {tongue-in-cheek mode ON}
}
} I was just browsing through my newly arrived Nov 2004 copy of Microscopy Today
} and found something that has deeply shaken my confidence in my instrument and
} ability to operate it. The back inside cover (an ad for an SEM
} manufacturer who
} shall remain nameless) displays a very colorful FE-SEM image of
} Paralia sulcata (Phytoplankton),
} measuring some hundreds of microns across and looking nothing like
} the specimens of the same
} species I routinely image with my lowly tungsten-based instrument
} (see http://www.mta.ca/dmf/wii23.htm for what I'm used to seeing).
}
} It would appear that my SEM is generating not only a thoroughly
} spurious image, but also my
} magnification calibration is off by a factor of something like 300.
}
} I understand that image quality is a function of the cost of the
} instrument, but the differences
} here are much more extreme than I ever appreciated. Why, it's like
} the two instruments
} are not even examining specimens for the same Kingdom! I guess my problem also
} stems from the fact that I can only rely on the 30+ years of
} expertise my wife (and collaborator)
} has in phytoplankton research, compared to the research budget of a
} heavy industry that is
} larger than the National Science Foundation. Obviously, I need to invest
} in better instrumentation. If one of the vendors will agree to fly
} me to Hawaii for the
} MSA meeting this summer, I'll almost certainly buy a new FE-SEM from them!
}
} {tongue-in-cheedk mode OFF}
}
} Wishing everyone a Happy (and Accurate) Holiday season,
}
} Jim
}
} --
}
} James M. Ehrman
} Digital Microscopy Facility
} Mount Allison University
} Sackville, NB E4L 1G7
} CANADA
}
} phone: 506-364-2519
} fax: 506-364-2505
} email: jehrman-at-mta.ca
} www: http://www.mta.ca/dmf

--
Philip Oshel
Supervisor, BBPIC microscopy facility
Department of Animal Sciences
University of Wisconsin
1675 Observatory Drive
Madison, WI 53706
voice: (608) 263-4162
fax: (608) 262-5157 (dept. fax)

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 11:26:00 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Jim, & Listers,

[This is getting a bit off-topic of W vs. FE SEM, but...] I had similar
thoughts first time I saw that image. I'll stick my neck out and suggest
that its really a leaf of Arabadopsis, wild type. At least that's the
consensus around here. Any other guesses??

Gib

--
Gib Ahlstrand, Scientist
Electron Optical Facility, University of Minnesota, CBS Imaging Center,
35 Snyder Hall, St. Paul, MN. USA. 55108 (612)624-3454
(612)624-2785 FAX, ahlst007-at-tc.umn.edu
http://www.cbs.umn.edu/ic/

"You can learn a lot by observation - just by lookin'!" - Yogi Berra

} Hi Listers,
}
} {tongue-in-cheek mode ON}
}
} I was just browsing through my newly arrived Nov 2004 copy of Microscopy
} Today
} and found something that has deeply shaken my confidence in my
} instrument and
} ability to operate it. The back inside cover (an ad for an SEM
} manufacturer who
} shall remain nameless) displays a very colorful FE-SEM image of Paralia
} sulcata (Phytoplankton),
} measuring some hundreds of microns across and looking nothing like the
} specimens of the same
} species I routinely image with my lowly tungsten-based instrument
} (see http://www.mta.ca/dmf/wii23.htm for what I'm used to seeing).
}
} It would appear that my SEM is generating not only a thoroughly spurious
} image, but also my
} magnification calibration is off by a factor of something like 300.
}
} I understand that image quality is a function of the cost of the
} instrument, but the differences
} here are much more extreme than I ever appreciated. Why, it's like the
} two instruments
} are not even examining specimens for the same Kingdom! I guess my
} problem also
} stems from the fact that I can only rely on the 30+ years of expertise
} my wife (and collaborator)
} has in phytoplankton research, compared to the research budget of a
} heavy industry that is
} larger than the National Science Foundation. Obviously, I need to invest
} in better instrumentation. If one of the vendors will agree to fly me to
} Hawaii for the
} MSA meeting this summer, I'll almost certainly buy a new FE-SEM from them!
}
} {tongue-in-cheedk mode OFF}
}
} Wishing everyone a Happy (and Accurate) Holiday season,
}
} Jim

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 11:46:59 2004

Contents Retrieved from Microscopy Listserver Archives
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Group,

Looking for labs that have access to LAICP mass spec or NAA to look at trace rare earth elements in apatite and tourmaline mineral samples. Need quantification so not sure if you folks in the SIMS area can help but thought I would ask. If you have any ideas please respond directly with contact info, resource to be used, and poor university pricing. Will consider commercial labs.

Thanks

Roy Beavers

Southern Methodist University
Department of Geological Sciences
P.O. Box 750395
Dallas, TX 75275
Voice: 214-768-2756
Fax: 214-768-2701
Email: rbeavers-at-mail.smu.edu

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 13:34:17 2004

Contents Retrieved from Microscopy Listserver Archives
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EMS now does this kind of things - see http://www.emsdiasum.com/default.htm

At 12:48 PM 12/17/2004, Karl Hagglund wrote:

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From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 13:47:37 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I should offer at least one tale of warning in connection with ISA cards.

We had an EDS computer for one of our SEMs. The EDS system (Oxford ISIS)
required 1 ISA slot for its interface and we had an older PCI image capture
system on the same computer and that required two ISA slots. We upgraded
the motherboard over the years from a 486-50 to a Pentium 90, to a Pentium
200 Overdrive processor, to an AMD 500. That all went well as we always
ordered motherboards with 3 (or more) ISA slots.

When it came time to make the next jump, we could not find a motherboard
with three slots. I found a Biostar board with 1 slot. We bit the bullet
and spent the money to upgrade the PCI system to a single PCI card and
tried to keep the ISIS running on the ISA card. That did NOT work.

We ran into a variety of problems, probably related to timing issues. We
had not changed any software except a few drivers for the motherboard. We
could switch back to the old motherboard and things would work fine, but
swap in the new motherboard and things got weird again. Consultation with
the staff at Oxford confirmed the timing suspicion. We determined the best
course would be to upgrade the ISIS board from ISA to PCI.

However, even that did not work completely smoothly. We had upgraded from
Windows 3.11 through Windows 95 to Windows 98se over the years with no
problem. The driver needed for the new PCI card only worked properly under
Windows 2000 or XP. Upgrading to 2000 solved the problem and our system has
been running fine for the last two years.

I may add that we tried to upgrade to Windows XP, but that led to other
problems. XP does not work with one an image library (KNIFE.VBX) that is
required for one piece of our software.

The moral of the story seems to be that upgrades are not always as painless
as we would like them to be. While we were able to change out motherboards
and upgrade Windows several times, there can be problems waiting at the
next upgrade. I am happy to see the availability of motherboard that again
includes ISA slots, but I would recommend caution when trying to upgrade
with it. The specialized cards that we use are not so common and not so
universally tested as a sound or network card. Problems could be lurking.

Disclaimer: The folks at Oxford were reasonably helpful and pleasant
throughout this process. I can imagine the anxiety on the part of a tech
support person when a user says they are about to embark on a upgrade. The
process is not under the control of tech support and a lot of things that
can (and do) go wrong. Oxford has been fair to point out that they could
not guarantee the outcome of any of our upgrades, but they have helped us
as they could.

Warren

At 04:28 PM 12/16/04, you wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 14:12:45 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hi all,

Fred Schamber wrote a series of articles in Microscopy Today (Sep - Nov
1999) on triode electron guns. I scanned them in and use it for my class
(with permission). You can find it at

ftp://hoc2.ceof.ohio-state.edu/MSE741/PowerPoint/Lecture%201/Schamber%20-%20emission%20myths.pdf

In my discussions with Fred, we talked a little about the first ("false")
peak. The first peak does not show up in all guns and seems to be a
function of the gun design. It seems to more prevalent in older designs
than in the newer guns. Fred indicated that he did not see it in the
Personal SEM (TM) gun he designed. Our speculation at the time was that
the false peak could be due to emission from the sides of the W loop
filament. This was based on my experience with looking at TEM filament
images.

If you talk with Fred, he will discuss the equipotential lines as the
wehnelt bias is varied. I usually visualize the wehnelt as an
electrostatic lens. As the potential (bias) is increased, the focal length
is shortened. Saturation occurs when the focal length is such that you are
looking at just the tip of the filament. At the lower bias voltages, you
tend to see the halo around the central image of the tip. These seem to be
coming from the "side" faces of the wire loop. I suspect that these
electrons are responsible for the false peak. However if Fred wishes to
jump into this thread, I'll certainly defer to him!

Cheers,
Henk

At 05:57 AM 12/17/04, michael shaffer wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

Hendrik O. Colijn colijn.1-at-osu.edu
Campus Electron Optics Facility Ohio State University
(614) 292-0674 http://www.ceof.ohio-state.edu
Time is that quality of nature which keeps events from happening all at
once. Lately it doesn't seem to be working.

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 14:35:39 2004

Contents Retrieved from Microscopy Listserver Archives
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I'm sorry John, but I can't let this slip away.

First, let me say that I do not have any issues with the technical issues that you put in response to Jerry's article because I do not consider myself an expert and do consider you one. When you write an article or submit something on the listserver, my ears perk up and I read it. I have personally benefited from your generosity in discussing and helping me with stereological problems. However, there are a number of points that you raise that I think that should be addressed.

You are correct that MT is not a refereed journal, but I don't think that your assessment that people don't take it seriously is correct. Ron is an experienced microscopist and does a very good job of putting solid articles together in a coherent fashion. For the most part, the articles are by people that are well-respected. I have written a few articles for MT (not that I am well-respected, LOL) and I am careful to try not to put anything that is incorrect in there because I realize that it is not refereed. It also takes a bit of time to put an article together and I thank the efforts of those who have written for MT. I have talked to others who have written articles and for the most part, they have taken similar care. If you have technical exceptions to an article that someone has written, I would bet that Ron would be willing to include those if they were written in an objective mode.

Next, the Listserver is for discussion. Your points with respect to the MT article are valid and are on subject and definitely should generate discussion. However, I think that your delivery was a bit personal and rather scathing. That wasn't appropriate for the listserver and was against the rules. John, forgive me for saying this, but it looks unprofessional and lacked tact. It looked as if you were frustrated with nobody listening to you. Believe me that that is not the case when you talk about imaging. I just was not comfortable reading your submission because of the personal attack that it had.

I wrote this because I don't want people afraid to submit either to the listserver or MT for fear of personal attacks by well-known people in the field. I hope that this has not jeopardized our friendship in any way. These are my opinions alone.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Friday, December 17, 2004 12:20 PM
To: Microscopy-at-msa.microscopy.com

------------------------------------------------------------------------------
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

When Jerry Sedgewick's articles first appeared in Microscopy Today, I wrote a
lengthy correction to some of his misinformation and sent it to Ron Anderson.
There was no reply, and nothing appeared in the magazine, but Ron later told
me he had forwarded the letter to Jerry, who has never responded. Realizing
that the magazine is not a referreed journal and probably isn't taken very
seriously anyway, I put the continuing errors in the series of artices in the
category of a minor annoyance.

But in the most recent issue, at the end of Jerry's article, he has inserted
the statement 'Note: More thorough explanations of the concepts presented in
this article can be found in "The Image Processing Handbook" by John Russ.' By
invoking my name and book in an apparent attempt to gain some credibility for
the article, which is almost entirely incorrect and misleading, that statement
requires an answer.

First, the cited book does not discuss the subject of matching the appearance
of images on printouts and the computer screen. I have written in another
book on that topic, but the bible on the subject can be found in David Blatner
and Bruce Fraser's "Real World Photoshop" (Peachpit Press). Another excellent
choice for anyone concerned about doing this right is to get either the
GretagMacbeth Eye-One (my preference) or ColorVision Spyder calibration hardware and
software, and follow the straightforward procedures which will make sure that
your display, printout, and even projector all show the same thing.

The Sedgewick article is completely wrong (as usual). The International Color
Consortium begun by companies like HP and Apple has constructed a technically
sound and easily implemented framework that allows manufacturers of software
(e.g., Photoshop), hardware (display cards, monitors, printers) and
consumables (ink, paper) to provide widely available curves that everyone should use.
Bypassing this (per Jerry's recommendation) and attempting to adjust the image
or the monitor to make images more dramatic is a bad idea. Altering the
contrast of "scientific" images as compared to normal photography is nonsense. Ink
jet printers are fine and have their place, but are certainly not the only way
to get good output. The article has plenty of other, more subtle errors (e.g.,
the dialog shows that sRGB color space is being used, instead of one such as
Adobe 1998 with its greater gamut).

Ignore the article. In fact, ignore all of the Sedgewick articles about
Photoshop. Even in those cases where the instructions are not wrong, they are not
the best way to accomplish a given result. Go read a good book. There are lots
of them, written by people who actually know what they are writing about.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 15:41:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I have been relatively quiet about postings lately. But I posted today and
received the normal "prize" for my offering - multiple out-of-the-office
notices.

Since many of us will be taking time off in the next couple of weeks,
please allow me to preempt Nestor and remind you all of the guidelines in
the list FAQ. They are reproduced below. Please do not enable the
out-of-office reply without unsubscribing from the list.

Thank you and happy holidays.

Warren

http://microscopy.com/MicroscopyListserver/FAQ.html

Are There Any Special Settings on my Email Program?

----------
Yes.

1.) Please insure that your correct Email address is listed in the FROM:
record. You may need to enter this in the Preferences option of your Email
program. Contact your system administrator if your not sure what to do here.

2.) DO NOT set your Email Program to automatically reply to all messages,
or to request a return receipt. If either of these are done, you run the
risk of creating an Email loop within the system. This may result in a
message bouncing through the system for several days, filling up everyone's
mail box!

3.) Generally it is best to terminate each line of your message at less
than 80 characters. This avoids the occasional problem of messages getting
chopped up. Some mail routers, limit the number of characters per line. If
you exceed 80 characters it is sometimes possible that your message will
become randomly truncated. If your not sure, then simply enter a (Carriage
Return) at the end of each line of text you type (i.e., don't let your
system automatically word wrap) and things should be fine.

4.) Make sure you do not send attachments of any type. (see above)

5.) Do not set your Email program to deliver "out of the office/vacation"
messages. If you will be gone, you should unsubscribe from the list and
subscribe again when you return.

6.) It is not out of line to provide your company name, Email address or
WWW site as part of your signoff/signature line, at the end of ANY message
you post to this system. Anonymous posting of Email is frowned upon.

-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking
-------------------------------------------
No files should be attached to this message
-------------------------------------------
Warren E. Straszheim, Ph.D.
Materials Analysis and Research Lab
Iowa State University
46 Town Engineering
Ames IA, 50011-3232

Ph: 515-294-8187
FAX: 515-294-4563

E-Mail: wesaia-at-iastate.edu
Web: www.marl.iastate.edu

Scanning electron microscopy, x-ray analysis, and image analysis of materials
Computer applications and networking

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 15:42:05 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Scott

I've responded to you privately about some of the points in your posting. For
the public record, let me say that I do not mean to imply in any way that
everything in the magazine is of poor quality - much of it is quite good. And
I've written articles for it myself. But the quality depends on the efforts of
the submitter, not on any review process, so readers need to exercise some
judgment.

My posting was not intended as a personal attack on either Jerry or Ron. Ron
has to fill the magazine for each issue and must depend on whatever people are
willing to send him. The simple fact is that the Sedgewick articles on
Photoshop (and his book put out by Plenum) contain many, many errors, both on image
processing in general and Photoshop in particular. I don't intend to try to
correct them point by point. There are plenty of texts on both image processing
and on Photoshop that get it right, and people should be warned to read them.

I have not responded publicly in the past to the errors in the articles, but
this time the fact that my name and book were referenced inappropriately and
incorrectly in the article required some kind of corrective response. Sorry if
I offended you....

John Russ

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 22:02:10 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Karl Hagglund wrote:
================================================================
} Hello,
}
} We have a See Vac Critical Point Dryer in need of repair. Does anyone
} know of a third party company that performs repairs on these devices.
================================================================
The See Vac firm went out of existence around 1983 or 1984 (if I remember
correctly). The owner and president, Blair Seese, passed away about ten or
twelve years ago from cancer.

We ended up with a box of spare parts, mainly for the Seevac manufacturered
sputter coaters and also some of the other equipment items they made,
including the CPD unit. The CPD unit has not been made since the early
1980's. If you could contact me off-line and tell me what parts you think
you need, I could see if we have them.

The system you have is roughly 25 years old. You might want to talk to your
safety people and get their opinion on the need to get it safety re-tested.
There are special laboratories who do that sort of thing, we are not one of
them.

Chuck
===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 17 22:28:43 2004

Contents Retrieved from Microscopy Listserver Archives
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Hi All:

I am a beginner in using TEM. I am currently in
investigating
nano-particles of 20nm and below. However, I have
difficulty in getting the
diffraction pattern in TEM. May I know if i can have
some advice on this
issue? Thanks a lot!

Regards,
Yee Yan
Postgraduate
Nanyang Technological University
Singapore

__________________________________________________
Do You Yahoo!?
Download the latest ringtones, games, and more!
http://sg.mobile.yahoo.com

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 18 07:25:42 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (mgrace-at-fit.edu) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html#form on Friday, December 17, 2004 at 12:40:39
---------------------------------------------------------------------------

Email: mgrace-at-fit.edu
Name: Michael Grace

Organization: Florida Institute of Technology

Education: Graduate College

Location: Melbourne, FL USA

Question: I am purchasing a digital imaging system for a film-based TEM (Zeiss EM900), and am trying to decide on a camera. Questions:

1. I am currently considering the SIS MegaView and Morada, and the AMT XR40/XR60. Does anyone have experience with these? Recommendations?

2. One ultimate goal is to have high quality digital images for publication. How much resolution in a system is enough? Pixel size/number info is difficult (for me, at least) to understand and to relate to actual output resolution.

Thanks!

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 18 07:26:15 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (zohrehhamnabard-at-yahoo.com) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Saturday, December 18, 2004 at 01:38:06
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Email: zohrehhamnabard-at-yahoo.com
Name: zohreh hamnabard

Organization: materials energy research center

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: dear sir/madam,
I have some glass-ceramic samples(phlogopite system) and I am going to investigate them through SEM. How can I etch these samples and what etchants can I use for this purpose to get best results and high degree photos.

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From MicroscopyL-request-at-ns.microscopy.com Sat Dec 18 10:33:58 2004

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I am looking for FIB services for TEM samples (universities or companies). I
prefer a training course of FIB where I can bring my own samples, depending on
the cost. If there are such services (training, sample preparation services,
or just free testing my samples), please advise.

Thank you,
Hiromi Konishi, Ph.D.

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 03:23:34 2004

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Dear Yee-Yan,
This is not exactly a beginner's problem and is in fact quite hard. If
you want powder diffraction patterns, then put a large SA aperture in
and hit Diffraction, easy enough. If you want single particle
diffraction patterns, then SA will probably not give sufficient
intensity from such small particles. You will probably have to use some
form of convergent beam diffraction. Whether this is done in
conventional imaging mode, or using a nanodiffraction mode is up to you
and your microscope. Whatever, you need a focussed probe with small
spot size, sufficient intensity to see a diffraction pattern without
roasting the particle, and a convergence angle low enough to separate
the diffraction spots (may need to change the C2 aperture). Then press
diffraction. This is fiddly but should work. The really tricky bit is
if you then need to tilt the particle to a specific orientation. I can
only say, be patient! And don't expect anything nice like Kikuchi bands
to help you, it is too thin.

Best wishes

Ian

} I am a beginner in using TEM. I am currently in
} investigating
} nano-particles of 20nm and below. However, I have
} difficulty in getting the
} diffraction pattern in TEM. May I know if i can have
} some advice on this
} issue? Thanks a lot!
}

--
Ian MacLaren
Department of Physics and Astronomy
University of Glasgow
Glasgow G12 8QQ
Scotland
http://www.ssp.gla.ac.uk/

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 08:04:05 2004

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Did anyone ask if Yee-Yan's particles are crystalline? Properly recording
and interpreting the results aside, E.D. is simple enough that anyone with
an instruction book or a colleague nearby can work the controls of a TEM to
get some sort of a diffraction pattern on the screen.

Yee-Yan: if you illuminated some of your particles with an electron beam in
a TEM set in diffraction mode, and all you see is a single bright spot
centered on a featureless, diffuse background, it could be that your
particles are amorphous (or nearly so).

Ron Anderson

-----Original Message-----
} From: Ian MacLaren [mailto:i.maclaren-at-physics.gla.ac.uk]
Sent: Monday, December 20, 2004 4:22 AM
To: Tay Yee Yan
Cc: Microscopy-at-msa.microscopy.com

Dear Yee-Yan,
This is not exactly a beginner's problem and is in fact quite hard. If
you want powder diffraction patterns, then put a large SA aperture in
and hit Diffraction, easy enough. If you want single particle
diffraction patterns, then SA will probably not give sufficient
intensity from such small particles. You will probably have to use some
form of convergent beam diffraction. Whether this is done in
conventional imaging mode, or using a nanodiffraction mode is up to you
and your microscope. Whatever, you need a focussed probe with small
spot size, sufficient intensity to see a diffraction pattern without
roasting the particle, and a convergence angle low enough to separate
the diffraction spots (may need to change the C2 aperture). Then press
diffraction. This is fiddly but should work. The really tricky bit is
if you then need to tilt the particle to a specific orientation. I can
only say, be patient! And don't expect anything nice like Kikuchi bands
to help you, it is too thin.

Best wishes

Ian

} I am a beginner in using TEM. I am currently in
} investigating
} nano-particles of 20nm and below. However, I have
} difficulty in getting the
} diffraction pattern in TEM. May I know if i can have
} some advice on this
} issue? Thanks a lot!
}

--
Ian MacLaren
Department of Physics and Astronomy
University of Glasgow
Glasgow G12 8QQ
Scotland
http://www.ssp.gla.ac.uk/

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 08:24:03 2004

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Roy,

We have a LA-ICP-MS, but not for commercial use. Two companies that you can
check out include Balazs (there is a local office in the DFW area, but the
lab is in California) and Shiva in New York, but they do Glow Discharge MS.
Both are pretty good companies (we still do business with both
companies)...with one strong caveat. Both companies apparently believe that
their trace analysis capability with the instrumentation cited does not need
need a matrix-matched standard or reference material. Their explanations
for no need of reference materials are, I believe, nothing but smoke and
mirrors. In order to get results that are dependable, a standard that is a
well characterized apatite or tourmaline...or close analogue is needed. We
don't believe one can calibrate either instrument with, say, a NIST glass
reference, and then expect to get good results analyzing SiC.

Contact me off-line if you wish.

Chuck Butterick
Analytical Laboratory Supervisor
Poco Graphite, Inc.
300 Old Greenwood Road
Decatur, TX 76234
(940) 393-4287 (Phone)
(940) 393-8383 (Fax)
CButterick-at-poco.com

-----Original Message-----
} From: Beavers, Roy [mailto:rbeavers-at-mail.smu.edu]
Sent: Friday, December 17, 2004 12:17 PM
To: microscopy-at-microscopy.com

Group,

Looking for labs that have access to LAICP mass spec or NAA to look at trace
rare earth elements in apatite and tourmaline mineral samples. Need
quantification so not sure if you folks in the SIMS area can help but
thought I would ask. If you have any ideas please respond directly with
contact info, resource to be used, and poor university pricing. Will
consider commercial labs.

Thanks

Roy Beavers

Southern Methodist University
Department of Geological Sciences
P.O. Box 750395
Dallas, TX 75275
Voice: 214-768-2756
Fax: 214-768-2701
Email: rbeavers-at-mail.smu.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 11:50:22 2004

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On Dec 17, 2004, at 8:59 PM, Tay Yee Yan wrote:

} I am a beginner in using TEM. I am currently in
} investigating
} nano-particles of 20nm and below. However, I have
} difficulty in getting the
} diffraction pattern in TEM. May I know if i can have
} some advice on this
} issue? Thanks a lot!
}
Dear Yee Yan,
One problem you might have is that such small particles make up a very
small fraction of the area seen in even the smallest selected area
aperture you have in your scope. Unless the particles constitute a
reasonable fraction of the scattering, the pattern will be lost in the
power spectrum of the substrate in the selected area. My advice is to
use the thinnest possible support film, make that film from low-Z
material (carbon is probably best), increase the concentration of
nanoparticles in your prep, and put a very small aperture (5 or 10 um)
in the SA aperture holder and use it to restrict the area. You will
probably see only diffraction rings, since the hoped-for many particles
in the selected area will not, in general, be oriented in the same
direction. Good luck.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 13:54:32 2004

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} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America

You also need to keep in mind that with SA diffraction, spherical
aberation limits how precisely you can define the area from which you
get diffraction. The error is of the order of 500 nm.

Typically, the smallest practical SA aperture will be ~5 um which
results in a selected area of ~ {500 nm. Consequently, if you really
push SA diffraction and succeed in getting a pattern, it is likely to
be from a region different from where you think it is coming from.

Best regards,
--
Larry Stoter
JEOL (UK) Ltd
tel: +44-(0)1707-377117, fax: +44-(0)1707-373254, e-mail: larrys-at-jeoleuro.com

PLEASE NOTE
1. Any mail other than plain text will be automatically deleted.
2. Any mail, legitimate or not, apparently or actually from hotmail,
netscape, yahoo or excite will automatically be deleted.
3. Mail with no subject or without a clear subject will be ignored :-)

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 13:59:48 2004

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Hi Listers:

The 4489 film I mentioned last week has been sold to the first responder to
my email. Thanks for all of your inquiries!

Happy Holidays to everyone who replied!

Karen Bentley

Karen L. Bentley, M.S.(previously Jensen)
Associate Scientist & Project Manager
Electron Microscope Research Core
University of Rochester Medical Center
Rochester, NY 14642
585-275-1954

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 17:18:52 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (kjl226-at-vt.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, December 20, 2004 at 15:05:08
---------------------------------------------------------------------------

Email: kjl226-at-vt.edu
Name: Kathy

Organization: Virginia Tech

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Has anyone out there had any expereince working with the Zeiss EVO40 SEM? I would like to get opinions on what you think of the instrument. Our Department purchased a EVO40 about 6 months ago and have had several serious problems. We are wondering if we have purchased a lemon.

Kathy Lowe

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From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 18:30:00 2004

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=======================================
First Notice of Microscopy Listserver DataBase Update:
=======================================
Dec. 21, 2004

Colleagues....

After nearly a dozen years of operation, the master database of the
Microscopy Listserver needs a serious reworking and purging. I have done
the hard work of restructuring the software model but now the
database needs to be "repopulated" with updated/new user information.

The easiest way for me to accomplish this is to simply purge the entire database,
and have each of you resubscribe as if you are a new user.

As a result, I'm asking EACH and EVERY ONE of you to visit the following WWW site
and fill out the new subscription form. Here is the URL:

http://www.microscopy.com/MicroscopyListserver/SubscribeMicroscopy.html

You can do this beginning immediately, the changes will be stored and
I will implement the new system on or about the second week of Jan. 2005.
If all goes well, resubscribing should only take a few minutes of your time,
so please do it as soon as possible.

For the balance of 2004 the old database will remain in use, but
if you have not resubscribed by ~ the first week of Jan 2005,
you will no longer receive Listserver Email as I will cease using the
old database and only forward Listserver Email to those individuals who have
subscribed and are recorded in the new system.

I'll post this message every Monday through Jan 3, as a reminder and shortly thereafter will
transition away from the old database to the new one.

Thanks in advance for your patience and cooperation.

Nestor
Your Friendly Neighborhood SysOp.

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 20 23:31:20 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jmo12505-at-yahoo.com) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Monday, December 20, 2004 at 22:33:37
---------------------------------------------------------------------------

Email: jmo12505-at-yahoo.com
Name: Judy Ogilvie

Organization: Saint Louis University

Title-Subject: [Microscopy] [Filtered] LM - advice on embedding plastic

Question: I have been using Epon Araldite plastic for many years for both EM & LM (1 micron) sectioning. I am gearing up for a new project that will involve embedding and sectioning of a fairly large number of mouse brains. I will not need to do any EM on this tissue. I also have undergraduates who are interested in participating in the project but have no prior histology experience. Are any of the newer plastics easier to work
with for embedding and sectioning?

Judy Ogilvie

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From MicroscopyL-request-at-ns.microscopy.com Tue Dec 21 01:29:20 2004

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Dr Jim:

My school has a Jeol JEM 2010 TEM running at 200kV.
Thanks a lot!

And the rest:

Very grateful for giving me so much useful advices! I
am currently waiting my turn for next session of TEM
to try and experiment again!!!!! Will update any
result if possible!

Regards,
Yee Yan
Nanyang Technological University

--- Jim Quinn {jquinn-at-www.matscieng.sunysb.edu} wrote:

} You may want to repost
} with the make and model
} number of your TEM.
} In that manner, people
} can give you specific
} answers.
}
} regards,
}
} Jim
}
}
} } From MicroscopyL-request-at-ns.microscopy.com Sat
} Dec 18 02:27:48 2004
} } X-Authentication-Warning: ns.microscopy.com: mail
} set sender to MicroscopyL-request-at-ns.microscopy.com
} using -f
} } Date: Sat, 18 Dec 2004 12:59:01 +0800 (CST)
} } From: Tay Yee Yan {one_twinklestar-at-yahoo.com.sg}
} } Subject: [Microscopy] Diffraction Pattern for
} nano-particle/quantum dots in TEM
} } To: Microscopy-at-msa.microscopy.com
} } MIME-Version: 1.0
} } Content-Type: text/plain; charset=iso-8859-1
} } Content-Transfer-Encoding: 8bit
} }
} }
} }
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}
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} Microscopy Society of America
} } To Subscribe/Unsubscribe --
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} } On-Line Help
}
http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} }
}
-------------------------------------------------------------------------------
} }
} } Hi All:
} }
} } I am a beginner in using TEM. I am currently in
} } investigating
} } nano-particles of 20nm and below. However, I have
} } difficulty in getting the
} } diffraction pattern in TEM. May I know if i can
} have
} } some advice on this
} } issue? Thanks a lot!
} }
} } Regards,
} } Yee Yan
} } Postgraduate
} } Nanyang Technological University
} } Singapore
} }
} }
} __________________________________________________
} } Do You Yahoo!?
} } Download the latest ringtones, games, and more!
} } http://sg.mobile.yahoo.com
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}

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From MicroscopyL-request-at-ns.microscopy.com Tue Dec 21 05:45:05 2004

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We have recently moved over to a Gatan digital system for our TEM and now
no longer use cut film.

We have 5 sealed boxes of KODAK 4489 (new formulation) - 83mm x 102mm (3.25
x 4") film. (100sheets/box)

3 boxes 2004 - 06
1 box 2004 - 09
1 box 2004 - 12

These are available at Ł35 a box.

Contact me if you are interested or require more information.

Kevin

------------

Kevin Mackenzie
Histology and EM Core Facility
Institute of Medical Sciences
University of Aberdeen
Foresterhill

k.s.mackenzie-at-abdn.ac.uk

01224 555822

www.abdn.ac.uk/ims/h-em

http://www.abdn.ac.uk/ims/imaging/

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 21 08:27:55 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (neil-at-young8696.freeserve.co.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 21, 2004 at 05:52:35
---------------------------------------------------------------------------

Email: neil-at-young8696.freeserve.co.uk
Name: Neil P. Young

Organization: University of Birmingham, England

Title-Subject: [Microscopy] [Filtered] STEM and beam induced contamination

Question: Dear all, I am a new TEM/STEM user. My machine is an FEI Tecnai F20 with STEM facility operating at 200kV. I am interested in looking at metal nanoparticles, diameter {20nm. I have deposited such particles (Au) upon carbon support films (Agar Scientific). I am having many problems with beam induced contamination of the carbon support, making imaging of the nanoparticles impossible with STEM. I am investigating ways of cleaning the supports before depositing nanoparticles. I wonder if such contamination problems are common with STEM and would be interested in possible solutions to the problem. I am currently investigating cleaning with organic solvents and heating or irradiation with UV.
regards

Neil Young
University of Birmingham

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 21 10:57:08 2004

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Dear Neil,

There are those much better qualified to answer this than
me but I'll give an answer as a 'neighbour' with some
experience of it.

Yes, contamination is a problem with STEM. It is with all
small probe modes, especially as you use higher and higher
beam currents. You will see contamination in a FEG STEM
when your specimen looks OK in every other machine.

First you need to identify the source of the contamination.
It is, as you say, most likely to be from your specimen. Do
other users have contamination free STEM sessions with the
same holder? If so then you can rule out the column or
holder cleanliness, if not then maybe there is a problem
there.

If you 'flood' the specimen does it reduce the
contamination rate for a while? If so then the major
contamination source is your specimen, if not the
contamination is coming from the vacuum. To flood the
specimen use a large C aperture and spot size and keep the
beam on an area larger than a grid square (~200um dia) for
15 minutes. Check the contamination rate in the centre of
the area before and after flooding.

If it is the C filmed grids giving rise to the
contamination we have found that annealing them in a
(clean) vacuum is a very efficient way of cleaning them,
about 200C for 10-15 minutes is usually enough. The Cu
tends to get annealed if the temperature is too high, not a
real problem it just makes handling them more difficult.

Plasma cleaning can also be used, if you have access to a
plasma cleaner, but it will also dissolve your film.

Ensure your method of depositing gold is clean or else
you've wasted your time cleaning the C film. If is is a
diffusion pumped vacuum then it should be trapped to
prevent backstreaming of oil. If it is a chemical or
solvent then it needs to be clean and pure, fresh from the
container into cleaned glass not from a plastic washbottle.

Ensure your method of storing specimens is clean. Avoid
contact with plastic containers - gelatine capsules should
be thrown away and never used. Keep specimens under clean
vacuum or in a dry container.

If no-one has clean specimens and flooding does not improve
the contamination rate it is probably your specimen holder
(clean it properly) or column (bake it out) causing the
problem.

If the contamination rate from your sample is small you may
be able to use the flooding method to prevent contamination
build up for long enough to run your experiment.

Good luck,
Ron

On Tue, 21 Dec 2004 08:27:37 -0600 by way of
MicroscopyListserver {neil-at-young8696.freeserve.co.uk} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
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} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (neil-at-young8696.freeserve.co.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 21, 2004 at 05:52:35
} ---------------------------------------------------------------------------
}
} Email: neil-at-young8696.freeserve.co.uk
} Name: Neil P. Young
}
} Organization: University of Birmingham, England
}
} Title-Subject: [Microscopy] [Filtered] STEM and beam induced contamination
}
} Question: Dear all, I am a new TEM/STEM user. My machine is an FEI Tecnai F20 with STEM facility operating at 200kV. I am interested in looking at metal nanoparticles, diameter {20nm. I have deposited such particles (Au) upon carbon support films (Agar Scientific). I am having many problems with beam induced contamination of the carbon support, making imaging of the nanoparticles impossible with STEM. I am investigating ways of cleaning the supports before depositing nanoparticles. I wonder if such contamination problems are common with STEM and would be interested in possible solutions to the problem. I am currently investigating cleaning with organic solvents and heating or irradiation with UV.
} regards
}
} Neil Young
} University of Birmingham
}
} ---------------------------------------------------------------------------
}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 21 15:42:50 2004

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Hi all,
I'm posting these job announcements for a friend, Robby Roberson.
Please contact Robby (not me) if you need more information.
robby2-at-asu.edu

happy holidays,
Beth
*****
As you may know there are three bioimaging positions in the School of
Life Sciences at Arizona State University (ASU): 1) Bioimaging
Laboratory Director to be appointed as a tenure-track Associate or Full
Professor, 2) Bioimaging Lab Manager (2 positions): responsible for
user training/interaction, equipment maintenance, etc. (position
announcement attached as advertised in Science).

The W.M. Keck Bioimaging Laboratory and the Life Sciences Electron
Microscopy Laboratory at Arizona State University will soon be merged
and administered by a new faculty Director and two Laboratory Managers.
For Director we are intending to appoint a senior, tenured faculty
member who maintains an active, well funded research program in cell or
molecular biology, preferably a program that incorporates bioimaging
techniques as an important feature. The other fifty percent of the
Directors workload, including all teaching and service, would be
directed toward the bioimaging laboratory. Teaching would likely
consist of bioimaging courses and laboratories at the graduate level
although there is flexibility here. Service would include management
and development of the bioimaging laboratory. These activities would
likely include supervision of two laboratory managers, preparation of
community-use equipment grants for external funding agencies,
organization of bioimaging workshops, development of laboratory policy,
and interaction with other units and research programs that use the
bioimaging laboratory. We hope to hire a Director that sees
development of the Bioimaging Laboratory as being a means to strengthen
their own research program.

The Lab Managers (service professionals in ASU terminology) will
oversee the daily activities of the laboratory, with the anticipation
that one manager will have expertise in electron microscopy and the
other expertise in light microscopy. The Bioimaging Laboratories are a
University-wide resource and as such the personnel hired must be
capable of interacting with faculty, staff, students and collaborating
scientists from a broad range of fields.

As stated in the ad, the Laboratory currently provides bioimaging
services in electron microscopy, cryofixation, freeze fracture,
laser-scanning confocal microscopy (single and multi-photon), video
microscopy, live cell imaging, single-molecule fluorescence microscopy,
and atomic force microscopy. ASU has an established history of
excellence in imaging with its Center for High Resolution Electron
Microscopy and its Centers for Optical Biotechnology and Molecular
Biophysics. This present hiring initiative is meant to maintain and
strengthen this emphasis in imaging. ASU is currently expanding in
biomedical and applied molecular research with the formation of the
Biodesign Institute and in growing relationships with Phoenix-area
biomedical and agricultural research institutes.

Formal applications can be sent to: Chair, Bioimaging Search Committee,
School of Life Sciences, PO Box 874501, Arizona State University,
Tempe, AZ 85287-4501. Initial closing date for applications is
December 28, 2004; if not filled, subsequent applications will be
reviewed weekly thereafter until the search is closed.

Thanks tons,
Robby and Doug (Chandler)
Co-Chairs, Bioimaging Search Committee
E-Mail: robby2-at-asu.edu

PS... happy solstice

**********************************************************************
Beth Richardson
EM Lab Coordinator
Plant Biology Department
University of Georgia
Athens, GA 30602-7271

Phone - (706) 542-1790 & FAX - (706) 542-1805
http://www.plantbio.uga.edu/emlab

"Between the two evils,
I always pick the one I never tried before". Mae West (1893-1980)
*******************************************************************

"And it's only the giving that makes you what you are".
Wond'ring Aloud, Jethro Tull (Aqualung)

************************************************************************
***

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 21 16:18:31 2004

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Niel

I'll echo Ron Doole's comments.

You can also access the information on Plasma Cleaning at this WWW
Site.

http://www.amc.anl.gov/Docs/ANL/TechTrans/PlasmaCleaning.html

There are some articles and a Book Chapter I wrote at that site. A number of
Vendors also market plasma cleaners including: SouthBay Technology,
XEI, Fischione,
and SPI.

Disclaimer:

ANL/University of Chicago holds the original patent on Plasma
Cleaning for AEM applications
and I did a modicum of that work.

Nestor
Your Friendly Neighborhood SysOp

--
===========================================
Dr. Nestor J. Zaluzec
Argonne National Lab
Materials Science Division/Bldg 212
9700 S. Cass Ave
Argonne, Illinois 60439 USA
Tel: 630-252-7901, Fax: 630-252-4798
Email: Zaluzec-at-aaem.amc.anl.gov
===========================================
TPMLab: http://tpm.amc.anl.gov
NEESLab: http://neestpm.mcs.anl.gov
MMSite: http://www.amc.anl.gov
===========================================

The box said ...
"This program requires Win 95/98/NT or better..."
So I bought a G3 Mac !

===========================================

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 06:20:57 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Hello to all:

I am glad to see a resolution to a topic that I too thought it was rather
harshly or inappropriately attacked.

Dear Dr. John Russ as Scott as well stated I too look to you for answers
when it comes to image analysis. I think the country looks to you for image
analysis. I have taken image analysis courses from you. Again as Scott said
I see your name on the listserver, I read it carefully. In our Microscopy
Lab I have two colleagues that have taken microscopy course/s from a
legendary man named Dr. Walter McCrone and they thought of him as if the
Webster Dictionary described the word microscopy as Dr. Walter McCrone. So,
it sounds like I am not alone to think that you must be a description in the
Webster Dictionary under image analysis. However, it takes people such as
you to bring out the best in the rest of us. I have yet to publish any
paper/article related to image analysis just because of being afraid to make
a mistake. I am glad to see the professionalism in you to re-assure the rest
of us (at least me) that mistakes can be made and maybe even corrected in a
professional manner. I assure you that this is to remind myself and others
like me that one can write articles/papers on image analysis and not be
ridiculed by the community.

I believe that a great teacher goes on teaching even when he/she is not
teaching.

Merry Christmas and Happy New Year to all.

Nicola Ranieri, Microscopy/Image Analysis
US FDA Forensic Chemistry Center
6751 Steger Drive
Cincinnati, Ohio 45237-3097
(513) 679-2700 X253
(513) 679-2761 FAX
nranieri-at-ora.fda.gov

-----Original Message-----
} From: Walck, Scott D. [mailto:walck-at-ppg.com]
Sent: Friday, December 17, 2004 4:04 PM
To: MicroscopyListserver (E-mail)

I'm sorry John, but I can't let this slip away.

First, let me say that I do not have any issues with the technical issues
that you put in response to Jerry's article because I do not consider myself
an expert and do consider you one. When you write an article or submit
something on the listserver, my ears perk up and I read it. I have
personally benefited from your generosity in discussing and helping me with
stereological problems. However, there are a number of points that you
raise that I think that should be addressed.

You are correct that MT is not a refereed journal, but I don't think that
your assessment that people don't take it seriously is correct. Ron is an
experienced microscopist and does a very good job of putting solid articles
together in a coherent fashion. For the most part, the articles are by
people that are well-respected. I have written a few articles for MT (not
that I am well-respected, LOL) and I am careful to try not to put anything
that is incorrect in there because I realize that it is not refereed. It
also takes a bit of time to put an article together and I thank the efforts
of those who have written for MT. I have talked to others who have written
articles and for the most part, they have taken similar care. If you have
technical exceptions to an article that someone has written, I would bet
that Ron would be willing to include those if they were written in an
objective mode.

Next, the Listserver is for discussion. Your points with respect to the MT
article are valid and are on subject and definitely should generate
discussion. However, I think that your delivery was a bit personal and
rather scathing. That wasn't appropriate for the listserver and was against
the rules. John, forgive me for saying this, but it looks unprofessional
and lacked tact. It looked as if you were frustrated with nobody listening
to you. Believe me that that is not the case when you talk about imaging.
I just was not comfortable reading your submission because of the personal
attack that it had.

I wrote this because I don't want people afraid to submit either to the
listserver or MT for fear of personal attacks by well-known people in the
field. I hope that this has not jeopardized our friendship in any way.
These are my opinions alone.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: DrJohnRuss-at-aol.com [mailto:DrJohnRuss-at-aol.com]
Sent: Friday, December 17, 2004 12:20 PM
To: Microscopy-at-msa.microscopy.com

----------------------------------------------------------------------------
--
The Microscopy ListServer -- Sponsor: The Microscopy Society of America

When Jerry Sedgewick's articles first appeared in Microscopy Today, I wrote
a
lengthy correction to some of his misinformation and sent it to Ron
Anderson.
There was no reply, and nothing appeared in the magazine, but Ron later told

me he had forwarded the letter to Jerry, who has never responded. Realizing
that the magazine is not a referreed journal and probably isn't taken very
seriously anyway, I put the continuing errors in the series of artices in
the
category of a minor annoyance.

But in the most recent issue, at the end of Jerry's article, he has inserted

the statement 'Note: More thorough explanations of the concepts presented in

this article can be found in "The Image Processing Handbook" by John Russ.'
By
invoking my name and book in an apparent attempt to gain some credibility
for
the article, which is almost entirely incorrect and misleading, that
statement
requires an answer.

First, the cited book does not discuss the subject of matching the
appearance
of images on printouts and the computer screen. I have written in another
book on that topic, but the bible on the subject can be found in David
Blatner
and Bruce Fraser's "Real World Photoshop" (Peachpit Press). Another
excellent
choice for anyone concerned about doing this right is to get either the
GretagMacbeth Eye-One (my preference) or ColorVision Spyder calibration
hardware and
software, and follow the straightforward procedures which will make sure
that
your display, printout, and even projector all show the same thing.

The Sedgewick article is completely wrong (as usual). The International
Color
Consortium begun by companies like HP and Apple has constructed a
technically
sound and easily implemented framework that allows manufacturers of software

(e.g., Photoshop), hardware (display cards, monitors, printers) and
consumables (ink, paper) to provide widely available curves that everyone
should use.
Bypassing this (per Jerry's recommendation) and attempting to adjust the
image
or the monitor to make images more dramatic is a bad idea. Altering the
contrast of "scientific" images as compared to normal photography is
nonsense. Ink
jet printers are fine and have their place, but are certainly not the only
way
to get good output. The article has plenty of other, more subtle errors
(e.g.,
the dialog shows that sRGB color space is being used, instead of one such as

Adobe 1998 with its greater gamut).

Ignore the article. In fact, ignore all of the Sedgewick articles about
Photoshop. Even in those cases where the instructions are not wrong, they
are not
the best way to accomplish a given result. Go read a good book. There are
lots
of them, written by people who actually know what they are writing about.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 09:11:48 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (R_Chen-at-fccc.edu) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, December 22, 2004 at 09:00:18
---------------------------------------------------------------------------

Email: R_Chen-at-fccc.edu
Name: Rongji Chen

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: We are trying to image DNA and dsRNA using Cytochrom C or BAC spreding/rotary shadowing techniques. While we were ble to reach reasonable contrast, we still have problems with longer DNA (say, 40 kb) - despite our efforts, the filaments usually remind more a complex bundle of knotted string than anything else. Any bright suggestions?

Thanks, Rongji Chen

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 09:53:13 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

John Russ writes ...
regarding the MT Sedgewick article

} [...[
} the dialog shows that sRGB color space is being used,
} instead of one such as Adobe 1998 with its greater gamut.
}
} Ignore the article. [...] Go read a good book. There are
} lots of them, [...]

Just as another note regarding Photoshop and color spaces (e.g., sRGB,
AdobeRGB). I would suggest another book, "Real World Color Management"
(Fraser, et al, Peach Press). Scientific imagery and Photoshop don't
necessary mix because recent versions of PS will insist on a working color
space (i.e., a work-around isn't easy to find). Given a general
installation of PS, and PS's default insistance on a working space, you can
end up with different color, or you can end up with different RGB data.
Either of the "Real World" books will make you aware of, and how to avoid
either, depending on the task at hand.

The general implication is understanding Photoshop is a significant study.
Unless you know what you're doing, you should use PS for presentation only
.. while keeping your original image files archived and intact.

Happy Holidays!!! ...

my CA$0.02 & cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 11:05:43 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

In a message dated 12/22/04 11:46:59 AM, michael-at-shaffer.net writes:

} Just as another note regarding Photoshop and color spaces (e.g., sRGB,
}
} AdobeRGB). I would suggest another book, "Real World Color Management"
}
} (Fraser, et al, Peach Press).

I agree with Michael that all of Bruce Fraser's books on Photoshop are
excellent sources of correct information. Another good one to consider is Michael
Kieran "Photoshop Color Correction" (Peachpit Press). I refer to the Kieran and
Fraser books regularly. Somewhat different in focus is Dan Margulis
"Professional Photoshop" (Wiley) which is mostly concerned with CMYK color spaces used
in printing but offers a useful point of view.

John Russ

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 12:17:08 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear Neil:

Plasma Cleaning of your support films would be the answer. I have some
documentation on this being done with our PC2000 Plasma Cleaner and would be pleased to send it along to you if you think it would be useful. Please contact me off-line for details.

Best regards-

David

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

by way of MicroscopyListserver wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- {http://www.msa.microscopy.com/MicroscopyListserver http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help {http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by ( {mailto:neil-at-young8696.freeserve.co.uk neil-at-young8696.freeserve.co.uk) from {http://microscopy.com/MicroscopyListserver/MLFormMail.html http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 21, 2004 at 05:52:35
} ---------------------------------------------------------------------------
}
} Email: {mailto:neil-at-young8696.freeserve.co.uk neil-at-young8696.freeserve.co.uk
} Name: Neil P. Young
}
} Organization: University of Birmingham, England
}
} Title-Subject: [Microscopy] [Filtered] STEM and beam induced contamination
}
} Question: Dear all, I am a new TEM/STEM user. My machine is an FEI Tecnai F20 with STEM facility operating at 200kV. I am interested in looking at metal nanoparticles, diameter {20nm. I have deposited such particles (Au) upon carbon support films (Agar Scientific). I am having many problems with beam induced contamination of the carbon support, making imaging of the nanoparticles impossible with STEM. I am investigating ways of cleaning the supports before depositing nanoparticles. I wonder if such contamination problems are common with STEM and would be interested in possible solutions to the problem. I am currently investigating cleaning with organic solvents and heating or irradiation with UV.
} regards
}
} Neil Young
} University of Birmingham
}
--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 12:19:51 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

Ron:

A very thorough response and some excellent suggestions. One correction
that I would like to make is that carbon support films can be cleaned in
a plasma cleaner without dissolving the film. In fact, this was tested
on our plasma cleaner and documented by our friendly neighborhood sysop
- Nestor Zaluzec. Perhaps the plasma cleaner you used did not have the
flexibilty to adjust the parameters appropriately to clean without
dissolving the film. I am away from the office now, but when I return I
would be happy to send you the reference if you have an interest. In
any case, it most certainly can be done with our PC2000.

Best regards-

David

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com
Ron Doole wrote:

} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} -------------------------------------------------------------------------------
}
} Dear Neil,
}
} There are those much better qualified to answer this than
} me but I'll give an answer as a 'neighbour' with some
} experience of it.
}
} Yes, contamination is a problem with STEM. It is with all
} small probe modes, especially as you use higher and higher
} beam currents. You will see contamination in a FEG STEM
} when your specimen looks OK in every other machine.
}
} First you need to identify the source of the contamination.
} It is, as you say, most likely to be from your specimen. Do
} other users have contamination free STEM sessions with the
} same holder? If so then you can rule out the column or
} holder cleanliness, if not then maybe there is a problem
} there.
}
} If you 'flood' the specimen does it reduce the
} contamination rate for a while? If so then the major
} contamination source is your specimen, if not the
} contamination is coming from the vacuum. To flood the
} specimen use a large C aperture and spot size and keep the
} beam on an area larger than a grid square (~200um dia) for
} 15 minutes. Check the contamination rate in the centre of
} the area before and after flooding.
}
} If it is the C filmed grids giving rise to the
} contamination we have found that annealing them in a
} (clean) vacuum is a very efficient way of cleaning them,
} about 200C for 10-15 minutes is usually enough. The Cu
} tends to get annealed if the temperature is too high, not a
} real problem it just makes handling them more difficult.
}
} Plasma cleaning can also be used, if you have access to a
} plasma cleaner, but it will also dissolve your film.
}
} Ensure your method of depositing gold is clean or else
} you've wasted your time cleaning the C film. If is is a
} diffusion pumped vacuum then it should be trapped to
} prevent backstreaming of oil. If it is a chemical or
} solvent then it needs to be clean and pure, fresh from the
} container into cleaned glass not from a plastic washbottle.
}
} Ensure your method of storing specimens is clean. Avoid
} contact with plastic containers - gelatine capsules should
} be thrown away and never used. Keep specimens under clean
} vacuum or in a dry container.
}
} If no-one has clean specimens and flooding does not improve
} the contamination rate it is probably your specimen holder
} (clean it properly) or column (bake it out) causing the
} problem.
}
} If the contamination rate from your sample is small you may
} be able to use the flooding method to prevent contamination
} build up for long enough to run your experiment.
}
} Good luck,
} Ron
}
} On Tue, 21 Dec 2004 08:27:37 -0600 by way of
} MicroscopyListserver {neil-at-young8696.freeserve.co.uk wrote:
}
}
}
}
}
} } ------------------------------------------------------------------------------
} } The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} } To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
} } On-Line Help http://www.msa.microscopy.com/MicroscopyListserver/FAQ.html
} } -------------------------------------------------------------------------------
} }
} } Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (neil-at-young8696.freeserve.co.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 21, 2004 at 05:52:35
} } ---------------------------------------------------------------------------
} }
} } Email: neil-at-young8696.freeserve.co.uk
} } Name: Neil P. Young
} }
} } Organization: University of Birmingham, England
} }
} } Title-Subject: [Microscopy] [Filtered] STEM and beam induced contamination
} }
} } Question: Dear all, I am a new TEM/STEM user. My machine is an FEI Tecnai F20 with STEM facility operating at 200kV. I am interested in looking at metal nanoparticles, diameter {20nm. I have deposited such particles (Au) upon carbon support films (Agar Scientific). I am having many problems with beam induced contamination of the carbon support, making imaging of the nanoparticles impossible with STEM. I am investigating ways of cleaning the supports before depositing nanoparticles. I wonder if such contamination problems are common with STEM and would be interested in possible solutions to the problem. I am currently investigating cleaning with organic solvents and heating or irradiation with UV.
} } regards
} }
} } Neil Young
} } University of Birmingham
} }
} } ---------------------------------------------------------------------------
} }
} }
} }
} }
} }
} }
}
} ----------------------
} Mr. R.C. Doole
} Department of Materials,
} University of Oxford.
} Parks Road, Oxford. OX1 3PH. UK.
} Phone +44 (0) 1865 273701
} Fax +44 (0) 1865 283333
} ron.doole-at-materials.ox.ac.uk
} http://www-em.materials.ox.ac.uk/
} *********************************
}
}
}
}
}
}
}
}
}

--
David Henriks
Vice President

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed.
If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and
delete this message from your system.

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

--
David Henriks

South Bay Technology, Inc.
1120 Via Callejon
San Clemente, CA 92673 USA

TEL: +1-949-492-2600
Toll-free in the USA: +1-800-728-2233
FAX: +1-949-492-1499

email: henriks-at-southbaytech.com

Celebrating 40 years of providing Materials Processing Solutions for Metallogaphy, Crystallography and Electron Microscopy.

Please visit us online at www.southbaytech.com.

The information contained in this message and any attachments is privileged and confidential. This message is intended for the individual or entity addressed. If you are not the intended recipient, please do not read, copy or disclose this communication. Notify the sender of the mistake by calling +1-949-492-2600 and delete this message from your system.

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 22 13:21:04 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

I would like to add my two cents into this discussion regarding carbon contamination. This is in regard to observations that I have had using carbon films, FEG TEMs, and plasma cleaners. I have anecdotal information on carbon films and plasma cleaning of coated samples that I would like to share.

General Claim: The type of carbon that you have is going to play a role in "contamination" effects and the effectiveness in carbon removal with plasma cleaners.

When I was working at Wright Patterson Air Force Base, we were looking at pulsed laser deposited (PLD) diamond-like carbon (DLC) films. First, it is well-known in the literature that the way the DLC films are prepared and their inherent chemistry plays a major role in their tribological properties as well as their reaction to environmental factors. The films that we grew by PLD showed a layered pattern of alternating regions of amorphous DLC that varied in the ratio of sp3 to sp2 bonds, i.e. the darker bands were more diamond-like and the lighter bands were more graphite-like. When a focused FEG probe was used to acquire EELS spectra, the dark bands would show all SP3 bonding initially but immediately start showing or growing the SP2 structure during beam exposure within seconds. The light bands would do it also, but the rate of build-up was comparatively slower (never measured -only observed). Since the films were grown on silicon substrates, I prepared these samples by the
small angle cleavage technique. This gave great, very thin carbon films, and SACT is very good for minimizing, if not eliminating, contamination problems. If the beam was not converged on the PLD-DLC coating, but was used in the normal imaging mode, no contamination build-up was seen, regardless of how much time the sample was under the beam. If the converged beam was moved to the substrate, the beam could be in position for up to 5 minutes with no noticeable contamination. I concluded that the beam was converting the carbon type when converged on the coating and that it was not contamination.

When I first came to PPG, we had a JEOL 1200EX that operated at 120 kV. At this voltage, the glass is softened because of the energy that is deposited in the glass. When the samples were taken to a 200 or 300 kV machine (outside lab with FEG or LaB6), we did not see the softening effect. To help the problem when imaging at 120 kV, I found that a very light evaporated carbon layer helped dissipate the heat as well as eliminate charging effects. The evaporator was a diffusion pumped system and pretty dirty. I worried about contamination problems in the FEG machines if I used the samples coated with this carbon in these better FEG machines. To help minimize charging in samples taken to other sites with FEG, I developed a way of sputter coating carbon films destined for use in the good machines with my Bal-Tec RES 100 ion mill. Well the situation arose where I didn't have one of the "clean" carbon sputtered samples and only had the 120 kV carbon evaporated films. I thought that I
could plasma clean (EAF Fishcione unit) the samples for a very short time and partially remove the carbon and have a light, but sufficiently conducting film for the FEG use. What I found was that the evaporated carbon resisted removal by plasma cleaning. Playing around a bit, I found that the sputter coated carbon films could be removed by plasma cleaning.

There are other behavior of carbon films with plasma cleaners that was written about in several publications in which I was a co-author. Those publication are available at the South Bay Technology web site for downloading as was mentioned by another posting. I think that an image of the SACT prepared PLD-DLC film on silicon with the EELS spectra is also available from their site.

My point in submitting these observations is that the behavior of the carbon films both under the beam and with plasma cleaning will differ depending on the state of the carbon which is determined by the deposition parameters.

-Scott

Scott D. Walck, Ph.D.
PPG Industries, Inc.
Glass Technology Center
P. O. Box 11472 (letters)
Guys Run Rd. (packages)
Pittsburgh, PA 15238-0472
Walck-at-PPG.com
(412) 820-8651 (office)
(412) 820-8515 (fax)

-----Original Message-----
} From: Ron Doole [mailto:ron.doole-at-materials.oxford.ac.uk]
Sent: Tuesday, December 21, 2004 11:58 AM
To: by way of MicroscopyListserver
Cc: microscopy-at-microscopy.com

Dear Neil,

There are those much better qualified to answer this than
me but I'll give an answer as a 'neighbour' with some
experience of it.

Yes, contamination is a problem with STEM. It is with all
small probe modes, especially as you use higher and higher
beam currents. You will see contamination in a FEG STEM
when your specimen looks OK in every other machine.

First you need to identify the source of the contamination.
It is, as you say, most likely to be from your specimen. Do
other users have contamination free STEM sessions with the
same holder? If so then you can rule out the column or
holder cleanliness, if not then maybe there is a problem
there.

If you 'flood' the specimen does it reduce the
contamination rate for a while? If so then the major
contamination source is your specimen, if not the
contamination is coming from the vacuum. To flood the
specimen use a large C aperture and spot size and keep the
beam on an area larger than a grid square (~200um dia) for
15 minutes. Check the contamination rate in the centre of
the area before and after flooding.

If it is the C filmed grids giving rise to the
contamination we have found that annealing them in a
(clean) vacuum is a very efficient way of cleaning them,
about 200C for 10-15 minutes is usually enough. The Cu
tends to get annealed if the temperature is too high, not a
real problem it just makes handling them more difficult.

Plasma cleaning can also be used, if you have access to a
plasma cleaner, but it will also dissolve your film.

Ensure your method of depositing gold is clean or else
you've wasted your time cleaning the C film. If is is a
diffusion pumped vacuum then it should be trapped to
prevent backstreaming of oil. If it is a chemical or
solvent then it needs to be clean and pure, fresh from the
container into cleaned glass not from a plastic washbottle.

Ensure your method of storing specimens is clean. Avoid
contact with plastic containers - gelatine capsules should
be thrown away and never used. Keep specimens under clean
vacuum or in a dry container.

If no-one has clean specimens and flooding does not improve
the contamination rate it is probably your specimen holder
(clean it properly) or column (bake it out) causing the
problem.

If the contamination rate from your sample is small you may
be able to use the flooding method to prevent contamination
build up for long enough to run your experiment.

Good luck,
Ron

On Tue, 21 Dec 2004 08:27:37 -0600 by way of
MicroscopyListserver {neil-at-young8696.freeserve.co.uk} wrote:

}
}
} ------------------------------------------------------------------------------
} The Microscopy ListServer -- Sponsor: The Microscopy Society of America
} To Subscribe/Unsubscribe -- http://www.msa.microscopy.com/MicroscopyListserver
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} Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (neil-at-young8696.freeserve.co.uk) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 21, 2004 at 05:52:35
} ---------------------------------------------------------------------------
}
} Email: neil-at-young8696.freeserve.co.uk
} Name: Neil P. Young
}
} Organization: University of Birmingham, England
}
} Title-Subject: [Microscopy] [Filtered] STEM and beam induced contamination
}
} Question: Dear all, I am a new TEM/STEM user. My machine is an FEI Tecnai F20 with STEM facility operating at 200kV. I am interested in looking at metal nanoparticles, diameter {20nm. I have deposited such particles (Au) upon carbon support films (Agar Scientific). I am having many problems with beam induced contamination of the carbon support, making imaging of the nanoparticles impossible with STEM. I am investigating ways of cleaning the supports before depositing nanoparticles. I wonder if such contamination problems are common with STEM and would be interested in possible solutions to the problem. I am currently investigating cleaning with organic solvents and heating or irradiation with UV.
} regards
}
} Neil Young
} University of Birmingham
}
} ---------------------------------------------------------------------------
}
}

----------------------
Mr. R.C. Doole
Department of Materials,
University of Oxford.
Parks Road, Oxford. OX1 3PH. UK.
Phone +44 (0) 1865 273701
Fax +44 (0) 1865 283333
ron.doole-at-materials.ox.ac.uk
http://www-em.materials.ox.ac.uk/
*********************************

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 23 05:41:10 2004

Contents Retrieved from Microscopy Listserver Archives
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Dear listers,
I now have a working Micrion 2500 FIB system (lovely) and made my first TEM specimen yesterday, a nice Christmas present! I am now looking at micromanipulators for lift-out TEM specimen prep. I would be very grateful to hear from anyone who has recently purchased a micromanipulator for this purpose, either in-situ or ex-situ, what are the pros and cons of each, and of course how much it is likely to cost. Manufacturers are welcome to respond off-line.

Although not microscopy-related per se, I have a Philips HRD five-crystal X-ray diffraction kit for disposal. The HT generator is no longer working (I can give more details to anyone who is interested). A very nice machine with a good solid goniometer. It would be nice to find a home for this, as usual I hate to see good machines going into landfill. I don't want any money for it, but if you take it you will pay for any shipping costs.

Season's greetings to all,

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

=======================================================================
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From MicroscopyL-request-at-ns.microscopy.com Thu Dec 23 08:27:17 2004

Contents Retrieved from Microscopy Listserver Archives
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Yes, you can go to a conference in Cuba!

The

8th InterAmerican Congress of Electron Microscopy,

will be held in Havana, Cuba, from 25 to 30 September 2005.

Despite the restrictions on travel to Cuba by citizens and residents of
the USA, full-time professional microscopists are allowed to travel to
Cuba for this meeting. Details are given along with other valuable
information on the conference web site:

http://ciasem2005.cigb.edu.cu/

Bookmark this site, which will be kept up to date as new information
becomes available.

The conference is sponsored by CIASEM, the
InterAmerican Committee of Electron Microscopy Societies
http://www.ciasem.com/

..........
Alwyn Eades
Department of Materials Science and Engineering
Lehigh University
5 East Packer Avenue
Bethlehem
Pennsylvania 18015-3195
Phone 610 758 4231
Fax 610 758 4244
jae5-at-lehigh.edu

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 23 11:40:27 2004

Contents Retrieved from Microscopy Listserver Archives
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richard,
we have a fei db235, in service for about 3 years. we purchased the in-situ omniprobe plucker with the initial installation. it works well, but is somewhat tricky to align the tips. in our version, the coordinate system for the plucker and the sample are different, meaning a z move with the plucker, moves x,y,z, in relation to the sample. i think omniprobe has a much better system available, but at a cost. ours was around $80K as i recall, much more for their newer system. we have recently acquired a zyvex s100 manipulator for in-situ probe measurements, manipulation, and tem lift out. priced at $180K. it was just installed, and we have not fully tried it, but it looks very nice. with either system we would like to have sharper probe tips. we currently use two sources for tips with the omniprobe: micromanipulator company, 7x (.1 micron radius) and omniprobe tips.

mike

Michael T. Marshall
Research Engineer
University of Illinois
Frederick Seitz Materials Research Laboratory
104 South Goodwin Avenue
Urbana, IL 61801
Voice: 217/265-5380 Fax: 217/244-2278
marshall-at-mrl.uiuc.edu

-----Original Message-----
} From: Richard Beanland [mailto:richard.beanland-at-bookham.com]
Sent: Thursday, December 23, 2004 5:40 AM
To: Microscopy Listserver (E-mail)

Dear listers,
I now have a working Micrion 2500 FIB system (lovely) and made my first TEM specimen yesterday, a nice Christmas present! I am now looking at micromanipulators for lift-out TEM specimen prep. I would be very grateful to hear from anyone who has recently purchased a micromanipulator for this purpose, either in-situ or ex-situ, what are the pros and cons of each, and of course how much it is likely to cost. Manufacturers are welcome to respond off-line.

Although not microscopy-related per se, I have a Philips HRD five-crystal X-ray diffraction kit for disposal. The HT generator is no longer working (I can give more details to anyone who is interested). A very nice machine with a good solid goniometer. It would be nice to find a home for this, as usual I hate to see good machines going into landfill. I don't want any money for it, but if you take it you will pay for any shipping costs.

Season's greetings to all,

Richard

_______________________________
Richard Beanland
Analytical Services
Bookham Technology plc
Caswell,
Towcester,
Northamptonshire NN12 8EQ
UK
Tel: +44 (0) 1327 356362
Fax: +44 (0) 1327 356775
http://www.bookham.com

=======================================================================
This e-mail is intended for the person it is addressed to only. The
information contained in it may be confidential and/or protected by
law. If you are not the intended recipient of this message, you must
not make any use of this information, or copy or show it to any
person. Please contact us immediately to tell us that you have
received this e-mail, and return the original to us. Any use,
forwarding, printing or copying of this message is strictly prohibited.
No part of this message can be considered a request for goods or
services.
=======================================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 23 18:18:59 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (jfb-at-yadtel.net) from http://www.microscopy.com/MicroscopyListserver/MLFormMail.html on Thursday, December 23, 2004 at 15:29:38
---------------------------------------------------------------------------

Email: jfb-at-yadtel.net
Name: John

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: I have a Zeiss Tessovar lens turret that has what appears to be either optical adhesive or some previous cleaning solution that is slightly clouding the back surface (very edges) of a small .25 and .5 lens. Is there a method of releasing the glue on the front lens(of two sandwich with space between)in order that one could access the middle surfaces to clean, and then replace? Any comments would be appreicated.

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 25 00:45:41 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Scott Walck wrote:
============================================================================
=
} snip {

General Claim: The type of carbon that you have is going to play a role in
"contamination" effects and the effectiveness in carbon removal with plasma
cleaners.

} snip {
============================================================================
=
Since SPI Supplies also manufactures a plasma cleaner under license from
Argonne National Laboratory, see URL
http://www.2spi.com/catalog/instruments/plasma-cleaner.shtml

I would like to make the following comments:

a) The efficacy of the cleaning depends on the power being used for the
cleaning, with 100 watts being much more effective than 10 watts. The
higher power units would also be much more aggressive in terms of etching
away a carbon filmed grid whereas 10 watts, so far as I can determine, would
not etch away a carbon filmed grid. Units described as plasma cleaners
generally operate at 10 watts or less, plasma etchers at 100 watts or more.
One can clean with an etcher in some circumstances, with oxygen, where there
are no carbon inclusions or other carbonaceous domains in the sample. One
would not want to clean with Ar at 100 watts since those conditions would
argon etch the rod and holder if not also the sample itself.

b) One could use a SiO2 filmed grid in many of the instances one would be
using a carbon filmed grid. One of the main reasons why one would prefer to
use an SiO2 filmed grid is that the grid can be "cleaned" with pure oxygen
without any fear of the substrate being etched away. The SiO2 filmed grids
will generally withstand a more aggressive cleaning at higher power levels.
Exposure to the higher power level generally results in a longer
contamination-free observation time.

c) We have never seen instances where some carbonaceous contamination
formed in a TEM on a TEM foiled sample can be removed this way and other
contamination could not (because it was a DLC).

Disclaimer: SPI Supplies manufactures the Plasma Prep Plasma Cleaner
instrument and we are also producers of both carbon and SiO2 filmed grids.

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 25 10:45:17 2004

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Microscopy Listserver Colleagues...

During the Xmas holidays as some of you know , I am deploying a new database and restructuring the
system. In order to make sure everyone stays on-line, there will be some
overlap of the databases. This means that a limited number of you may receive duplicate copies of Email
postings if your address is listed twice (once in each database). This should occur only if your
address is subscribed twice in two different forms something like this.

Someone-at-address1.organization.com
Someone-at-address2.organization.com

This usually occurs when individuals setup aliases and forwarding accounts.

If both databases have the same (i.e. identical) Email addresses then duplicate
should NOT occur, this case should apply to the MAJORITY of subscribers.

Purging these pseudo-duplicates (remember the software doesn't apriori know
these are the same individual) is time consuming and tedious. I'm asking that
if you are one of these individuals who gets duplicates please bear with them
until the ~ first week of Jan, when they should stop. I expect the volume
of such duplicated Email over the Xmas holiday to be pretty minimal as
traffic dies down alot over the holiday.

If you find this problem annoying, just unsubscribe the address which you
no longer use by the online form (http://www.microscopy.com/MicroscopyListserver).

Remember you can only post messages from an address which
is recorded in the subscription list, so if you make a change, insure that your EMail
client is also using the correct "FROM" address in its settings file.

Thanks in advance... & have a good holiday

Nestor
Your Friendly Neighborhood SysOp

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 25 16:04:52 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

At 01:45 AM 12/25/2004, Garber, Charles A. wrote:

} {...snip...}
}
} c) We have never seen instances where some carbonaceous contamination
} formed in a TEM on a TEM foiled sample can be removed this way and other
} contamination could not (because it was a DLC).
}

Hi Chuck,

I'm unclear about what you are saying in point (c). Are you saying that
e-beam generated contamination is DLC or that the other material is
DLC? Can DLC be removed by plasma cleaning? Do you have any references on
the form of carbon created by the e-beam? Presumably, SEM raster squares
are the same material as TEM contamination, yet they do eventually clean up
with plasma cleaning.

SiO2 filmed grids sound like a good solution when you need to plasma
clean. Are there any issues with the support film conductivity? I'd hate
to have the film blow apart like uncoated formvar! Also, has anyone used
the SiO2 support films for holding FIB liftout samples?

Cheers,
Henk

Hendrik O. Colijn colijn.1-at-osu.edu
OSU Campus Electron Optics Facility www.ceof.ohio-state.edu
040 Fontana Labs, 116 W. 19th Ave

From MicroscopyL-request-at-ns.microscopy.com Sat Dec 25 22:18:59 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Hendrik O. Colijn wrote:
=========================================================
Hi Chuck,

I'm unclear about what you are saying in point (c). Are you saying that e-
beam generated contamination is DLC or that the other material is DLC? Can
DLC be removed by plasma cleaning? Do you have any references on the form
of carbon created by the e-beam? Presumably, SEM raster squares are the
same material as TEM contamination, yet they do eventually clean up with
plasma cleaning.

SiO2 filmed grids sound like a good solution when you need to plasma clean.
Are there any issues with the support film conductivity? I'd hate to have
the film blow apart like uncoated formvar! Also, has anyone used the SiO2
support films for holding FIB liftout samples?
==========================================================
Sorry about the ambiguity; I guess that is my punishment for submitting a
posting over the holidays.

I was only trying to say that when it comes to contamination formed in a
column as a result of interaction with the electron beam, be it an SEM or
TEM, it has always been able to be removed with plasma cleaning. I have
never encountered what one might call a DLC formed under those conditions.
Physics is physics and irrespective of the brand and model of the plasma
cleaner being used, or the price paid, the contamination can be removed.
The higher the power the faster will be removed the contamination spot but
again, that is true for anyone's plasma cleaner.

With regard to SiO2 filmed grids, I have never heard of any conductivity
issues, but for FIB liftout samples (ex-situ techniques), take a look at URL
http://www.2spi.com/catalog/instruments/perforated-membrane-window-grids.
shtml
This type of grid might be a more stable alternative to the more traditional
holey support films be they carbon or SiO2. And of course, silicon nitride
should stand up quite nicely under conditions of plasma cleaning, even a
more aggressive cleaning with higher power if the FIB sample could stand it.

Disclaimer: SPI Supplies manufactures the Plasma Prep Plasma Cleaner so we
have a vested interest in seeing more people thinking about the plasma
cleaning of their samples prior to observation. See URL
http://www.2spi.com/catalog/instruments/plasma-cleaner.shtml

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 27 12:18:34 2004

Contents Retrieved from Microscopy Listserver Archives
http://www.microscopylistserver.com/MicroscopyListserver/MicroscopyArchives.html

On Dec 25, 2004, at 8:18 PM, Garber, Charles A. wrote:

} With regard to SiO2 filmed grids, I have never heard of any
} conductivity
} issues,

Dear Chuck,
Has anyone investigated SiO2 or SiO conductivities at either LN2 or
LHe temps?
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Mon Dec 27 20:09:46 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (rporter1-at-sbcglobal.net) from http://www.msa.microscopy.com/Ask-A-Microscopist/Ask-A-Microscopist.html on Monday, December 27, 2004 at 19:40:24
---------------------------------------------------------------------------

Email: rporter1-at-sbcglobal.net
Name: Randall Porter

Organization: UCSC

Education: 9-12th Grade High School

Location: Santa Cruz, CA, USA

Question: Hi,
Can you recommend manufacturers of reasonably priced microscopes for high school biology? I understand that Motic manufactures good, inexpensive scopes. I would rather not pay the overhead of the big four brands such as Olympus. Can you confirm that we should always purchase achromatic lenses and objectives?

Thanks for your help.
Randall

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 28 07:46:33 2004

Contents Retrieved from Microscopy Listserver Archives
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=======================================
Second Notice of Microscopy Listserver DataBase Update:
=======================================
Dec. 28, 2004

Colleagues, if you have subscribed/resubscribed since Dec. 21st
You may ignore the remainder of this message:

=======================================
First Notice of Microscopy Listserver DataBase Update:
=======================================
Dec. 21, 2004

Colleagues....

After nearly a dozen years of operation, the master database of the
Microscopy Listserver needs a serious reworking and purging. I have done
the hard work of restructuring the software model but now the
database needs to be "repopulated" with updated/new user information.

The easiest way for me to accomplish this is to simply purge the entire database,
and have each of you resubscribe as if you are a new user.

As a result, I'm asking EACH and EVERY ONE of you to visit the following WWW site
and fill out the new subscription form. Here is the URL:

http://www.microscopy.com/MicroscopyListserver/SubscribeMicroscopy.html

You can do this beginning immediately, the changes will be stored and
I will implement the new system on or about the second week of Jan. 2005.
If all goes well, resubscribing should only take a few minutes of your time,
so please do it as soon as possible.

For the balance of 2004 the old database will remain in use, but
if you have not resubscribed by ~ the first week of Jan 2005,
you will no longer receive Listserver Email as I will cease using the
old database and only forward Listserver Email to those individuals who have
subscribed and are recorded in the new system.

I'll post this message every Monday through Jan 3, as a reminder and shortly thereafter will
transition away from the old database to the new one.

Thanks in advance for your patience and cooperation.

Nestor
Your Friendly Neighborhood SysOp.

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 28 12:11:33 2004

Contents Retrieved from Microscopy Listserver Archives
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On Dec 27, 2004, at 6:12 PM, by way of Ask-A-Microscopist wrote:

} Email: rporter1-at-sbcglobal.net
} Name: Randall Porter
}
} Organization: UCSC
}
} Education: 9-12th Grade High School
}
} Location: Santa Cruz, CA, USA
}
} Question: Hi,
} Can you recommend manufacturers of reasonably priced microscopes for
} high school biology? I understand that Motic manufactures good,
} inexpensive scopes. I would rather not pay the overhead of the big
} four brands such as Olympus. Can you confirm that we should always
} purchase achromatic lenses and objectives?
}
} Thanks for your help.
}
Dear Randall,
Caroline Schooley is an expert on this; her contact info and the web
site for Project MICRO are:

Caroline Schooley
Project MICRO Coordinator
Microscopy Society of America
Box 117, 45301 Caspar Point Road
Caspar, CA 95420
Phone/FAX (707)964-9460
Project MICRO: http://www.msa.microscopy.com/ProjectMicro/
Intertidal invertebrates:
http://www.fortbragg.k12.ca.us/AG/marinelab.html

Project MICRO's purpose is to enhance pre-college education, as stated
on the web page.
Yours,
Bill Tivol, PhD
EM Scientist and Manager
Cryo-Electron Microscopy Facility
Broad Center, Mail Code 114-96
California Institute of Technology
Pasadena CA 91125
(626) 395-8833
tivol-at-caltech.edu

From MicroscopyL-request-at-ns.microscopy.com Tue Dec 28 20:53:58 2004

Contents Retrieved from Microscopy Listserver Archives
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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (tttan-at-simtech.a-star.edu.sg) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Tuesday, December 28, 2004 at 18:47:07
---------------------------------------------------------------------------

Email: tttan-at-simtech.a-star.edu.sg
Name: T T Tan

Organization: Singapore Institute of Manufacturing Technology

Title-Subject: [Microscopy] [Filtered] SEM - Wobbler Adjustment:

Question: Hello,

I am trying to understand the principle of and also to learn about focus wobbler adjustment for SEM. Can anyone please help me?
I found the earlier thread in the MSA achieve but couldnít find the article by Le Poole and related articles.
Ran searches on Google, Sciencedirect etc. but yielded nothing.

I understand that focus wobbler IN SEM is meant for aperture alignment. How can I tell which alignment (the ěxî or the ěyî) to adjust?

Also earlier on, I was operating the JEOL JSM 6340F. The image couldnít be focused even at 15,000X. When I over focuses, the image smudge in the x-y direction, along bottom left to top right of the screen. How can I adjust this?

Regards
T T Tan

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 29 06:55:26 2004

Contents Retrieved from Microscopy Listserver Archives
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T T Tan writes ...

} I am trying to understand the principle of and also to learn
} about focus wobbler adjustment for SEM. Can anyone please help me?
} I found the earlier thread in the MSA achieve but couldnít find
} the article by Le Poole and related articles.
} Ran searches on Google, Sciencedirect etc. but yielded nothing.

If (1) the final aperture is misaligned, or if (2) the beam is astimagtic,
it becomes evident as you focus above and below exact focus ... and this is
what the "wobbler" is supposed to help you with ... that is, to continuously
focus above/below, while you make the proper adjustments. Some SEM
operators, maybe most, have learned not to use it. Depending on the sample,
or the degree of the problem, it may be easiest to simply make the
adjustments until best focus is achieved.

While the wobbler is enabled, if the image shifts during focus
(left-right, up-down, diagonally, ... NOTE twisting is normal), then the
problem is the final aperture. Beginning with either aperture adjustment
(x,y), I usually adjust the wrong way first to make the problem worse, and
then I adjust thru and past the problem, to make it oppositely worse, and
then I come back ... and back again ... until I minimize the problem. Do the
same with the other aperture adjuster.

If the image does not move, but out-of-focus has directionality (as you
describe below), the the problem is astigmatism. The "stigmator" is a bit
more difficult to descibe its use. Additionally, there are 2 different
types of stigmators used by different manufacturers. I believe the JEOL
6xxx uses "x-y" adjusters and you would approch correcting the problem
similar to above. However, if the stigmator is the "rotation-amplitude"
type, I find the best approach is to make the problem worse with 'amplitude'
.. then minimize the problem with 'rotation' and then minimize the problem
with 'rotation'. Reitteration may be required, and keep in mind that your
problem may be a combination of (1) and (2).

HTH & Seasons' Greetings from "the rock"
cheerios ... shAf :o)
Avalon Peninsula, Newfoundland
www.micro-investigations.com (in progress)

} I understand that focus wobbler IN SEM is meant for aperture
} alignment. How can I tell which alignment (the ěxî or the ěyî) to adjust?
}
} Also earlier on, I was operating the JEOL JSM 6340F. The image
} couldnít be focused even at 15,000X. When I over focuses, the
} image smudge in the x-y direction, along bottom left to top right
} of the screen. How can I adjust this?
}
}
}
} Regards
} T T Tan
}
} ------------------------------------------------------------------
} ---------
}
}

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 29 09:50:05 2004

Contents Retrieved from Microscopy Listserver Archives
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It's true that correcting astigmatism is difficult to describe without
actually having someone observe it. The approach I take, with pretty
decent success, is as follows:

Find an area with lots of non-directional detail (i.e., straight edges
are bad while "sandy" looking areas are good). Throw the image out of
focus until a "smearing" effect is noticed, then go through the focus
point and observe that the "smearing" is now shifted 90 degrees from its
first orientation. This is definitely asigmatism when this is observed.
Still using the focus knob, adjust the image until you are in between
the "smearing" parts of the focus range. In other words, the image
should now be free of directional distortion, but will probably be
somewhat out of focus and if you turn the focus knob significantly in
either direction, the smearing will return.

Now use one of the stigmator controls, either x or y, and turn slowly,
using it as a "fine focus control". The image should appear to get
blurrier or sharper---make it as sharp as you can. Then do the same
with the other stigmator control. Repeat the process a couple times,
then go back to the focus knob and adjust it back and forth through the
focus point. If astigmatism has been corrected, the image will get
blurry on both sides of focus, but should not show any directional
"smearing".

"Smearing" = the effect you get by putting cooking oil on your hand and
wiping it in one direction on your kitchen window. The view of your
yard is now blurred and distorted in the direction of your application
of the oil. (Make note to clean window before your significant other
sees it---explaining this as an education tool is non-effective.)

Happy New Smear!

Randy

Randy Tindall
EM Specialist
Electron Microscopy Core Facility---We Do Small Well!
W122 Veterinary Medicine
University of Missouri
Columbia, MO 65211
Tel: (573) 882-8304
Fax: (573) 884-5414
Email: tindallr-at-missouri.edu
Web: http://www.emc.missouri.edu

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 29 16:17:29 2004

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Below is the result of your feedback form (NJZFM-ultra-55). It was submitted by (cdh1-at-cdc.gov) from http://microscopy.com/MicroscopyListserver/MLFormMail.html on Wednesday, December 29, 2004 at 12:07:22
---------------------------------------------------------------------------

Email: cdh1-at-cdc.gov
Name: Charles Humphrey

Organization: CDC, Atlanta GA

Title-Subject: [Microscopy] [Filtered] MListserver:

Question: Listserver:

I was wondering if anyone can assist me in obtaining replacement parts for an LKB 2188 Ultrotome NOVA.

Specific parts include the following.
90 01 3235 Oscillator PC board
90 01 5294 Transformer for diffuse light T1,T2
90 01 3195 Bushing for microscope stand
95 82 1005 Halogen lamp

Also, does anyone know the voltage and wattage for the above designated halogen lamp?

Thanks in advance
Charles Humphrey, CDC
I may be reached by telephone at 404-639-3307 January 4th 2005 and later

---------------------------------------------------------------------------

From MicroscopyL-request-at-ns.microscopy.com Wed Dec 29 17:52:16 2004

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Thanks, Randy and shAf, for your contributions re stigmator and aperture adjustment.

I've never been able to make much sense of the JEOL (840) instructions for condenser
lens alignment. It seems they take me into a loop from which there is no escape other
than giving up (yet again) in frustration.

Do you guys, or does anyone, have either a lucid step-by-step procedure for this, or an
explanation of what is aiming to be achieved that I can translate into specifics for the
840?

I use the thing only as a microprobe, so the spot tightness isn't a real issue, but it would
be nice to be able to do the sort of imaging that I know the 840 is capable of, and I
suspect that beam current stability is improved by good alignment.

Happy New Year

rtch

--
Ritchie Sims Ph D Phone : 64 9 3737599 ext 87713
Microanalyst Fax : 64 9 3737435
Department of Geology email : r.sims-at-auckland.ac.nz
The University of Auckland
Private Bag 92019
Auckland
New Zealand

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 30 01:30:43 2004

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Dear friends,
this e-mail is to inform you that you can find

Microscopy Research and Technique, Volume 63 Issue 1 - 1 January 2004
(1 - 86)
Special Issue: Two-Photon Microscopy - Part II

as free sample copy on the
http://www3.interscience.wiley.com/cgi-bin/jtoc/38527/
webpage.

Please, let me also wish again a bright and peaceful 2005.
Alby

------------------------------------------------------------------------
---------------------------
Alberto Diaspro, Department of Physics, University of Genoa
Via Dodecaneso 33, 16146 Genova, Italy
facsimile +39-010314218 - voice +39-0103536426/480/309
URL: http://www.lambs.it
http://www.wiley.com/WileyCDA/WileyTitle/productCd-0471409200.html
------------------------------------------------------------------------
--------------------------

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 30 10:47:41 2004

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We have tried SiO2 films in our lab for FIB liftout for just the reason
that Chuck mentioned, i.e., that we should be able to then plasma clean
without losing the sample. We have tried both bulk and lacy SiO2 films.
What we found was that the membrane is sufficiently non-conducting that the
liftout membranes charged up, then flew off the grid. Very distressing!!

We tried to cure this by using lacy carbon grids and Cr coating them, but
the stress of sputtered Cr broke the membrane. Carbon coating is not an
option since plasma cleaning will remove the C.

We have stayed with Formvar membranes and adjusted our plasma cleaning to
allow us to minimize contamination without destroying the formvar support
film. This was originally driven by the need to plasma clean polymer based
low-k dielectrics for chip fabrication; as a side benefit, we found that we
preserved the Formvar support film. Using a reduced O2 content in Ar, and
reduced power settings, we can do multiple iterations of plasma cleaning.
Typically, we find that 20 seconds is sufficient to allow EELS analysis
without causing measurable C contamination. I have been able to do three
such cleanings on a typical grid without losing the specimen.

Phil

Philip L. Flaitz
IBM Microelectronics, Hopewell Junction, NY
Ph.......(845) 892-3094, FAX -6256
pager - 800-352-4732, PIN# 1121
flaitz-at-us.ibm.com

"Garber, Charles
A." To: MICROSCOPY BB {Microscopy-at-MSA.Microscopy.com}
{cgarber-at-2spi.com cc:
} Subject: [Microscopy] Plasma cleaning of TEM + SEM samples

12/25/2004 11:18
PM

------------------------------------------------------------------------------

The Microscopy ListServer -- Sponsor: The Microscopy Society of America

-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Hendrik O. Colijn wrote:
=========================================================
Hi Chuck,

I'm unclear about what you are saying in point (c). Are you saying that
e-
beam generated contamination is DLC or that the other material is DLC?
Can
DLC be removed by plasma cleaning? Do you have any references on the form
of carbon created by the e-beam? Presumably, SEM raster squares are the
same material as TEM contamination, yet they do eventually clean up with
plasma cleaning.

SiO2 filmed grids sound like a good solution when you need to plasma
clean.
Are there any issues with the support film conductivity? I'd hate to
have
the film blow apart like uncoated formvar! Also, has anyone used the SiO2
support films for holding FIB liftout samples?
==========================================================
Sorry about the ambiguity; I guess that is my punishment for submitting a
posting over the holidays.

I was only trying to say that when it comes to contamination formed in a
column as a result of interaction with the electron beam, be it an SEM or
TEM, it has always been able to be removed with plasma cleaning. I have
never encountered what one might call a DLC formed under those conditions.

Physics is physics and irrespective of the brand and model of the plasma
cleaner being used, or the price paid, the contamination can be removed.
The higher the power the faster will be removed the contamination spot but
again, that is true for anyone's plasma cleaner.

With regard to SiO2 filmed grids, I have never heard of any conductivity
issues, but for FIB liftout samples (ex-situ techniques), take a look at
URL
http://www.2spi.com/catalog/instruments/perforated-membrane-window-grids.
shtml
This type of grid might be a more stable alternative to the more
traditional
holey support films be they carbon or SiO2. And of course, silicon nitride
should stand up quite nicely under conditions of plasma cleaning, even a
more aggressive cleaning with higher power if the FIB sample could stand
it.

Disclaimer: SPI Supplies manufactures the Plasma Prep Plasma Cleaner so we
have a vested interest in seeing more people thinking about the plasma
cleaning of their samples prior to observation. See URL
http://www.2spi.com/catalog/instruments/plasma-cleaner.shtml

Chuck

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
==================================================

From MicroscopyL-request-at-ns.microscopy.com Thu Dec 30 13:17:26 2004

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microscopy-at-microscopy.com

X-Mailer: CommuniGate Pro WebUser Interface v.4.2.6

--
Mei Lie Wong
412 Carl Street
San Francisco, CA 94117-3602

--_===2280893====msg.ucsf.edu===_--

From MicroscopyL-request-at-ns.microscopy.com Fri Dec 31 14:59:38 2004

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-- [ From: Garber, Charles A. * EMC.Ver #3.1 ] --

Philip Flaitz wrote:
=============================================================
We have tried SiO2 films in our lab for FIB liftout for just the reason that
Chuck mentioned, i.e., that we should be able to then plasma clean without
losing the sample. We have tried both bulk and lacy SiO2 films. What we
found was that the membrane is sufficiently non-conducting that the liftout
membranes charged up, then flew off the grid. Very distressing!!

We tried to cure this by using lacy carbon grids and Cr coating them, but
the stress of sputtered Cr broke the membrane. Carbon coating is not an
option since plasma cleaning will remove the C.

We have stayed with Formvar membranes and adjusted our plasma cleaning to
allow us to minimize contamination without destroying the formvar support
film. This was originally driven by the need to plasma clean polymer based
low-k dielectrics for chip fabrication; as a side benefit, we found that we
preserved the Formvar support film. Using a reduced O2 content in Ar, and
reduced power settings, we can do multiple iterations of plasma cleaning.
Typically, we find that 20 seconds is sufficient to allow EELS analysis
without causing measurable C contamination. I have been able to do three
such cleanings on a typical grid without losing the specimen.
================================================================
Could you tell us more about the conditions of the plasma cleaning in which
you reported that "Carbon coating is not an option since plasma cleaning
will remove the C." We have been able to plasma clean carbon support films
at 10watts power using oxygen without breaking the carbon films. This is
accomplished using the SPI Plasma Cleaner as shown on URL
http://www.2spi.com/catalog/instruments/plasma-cleaner.shtml

The application of chromium is still a sputtering process but one can apply
a 1 nm (sometimes less) coating of osmium metal in the OPC Osmium Coaters,
see URL
http://www.2spi.com/catalog/osmi-coat.html
I know that the use of the high Z element goes against conventional wisdom
but 1 nm is very very thin, so thin in fact that as one can see in URL
http://www.2spi.com/catalog/osmium-plasma-coater-demonstration.html
its presence at this thin of a layer does not interfere with BSE imaging at
all. So if the concept of applying a conductive layer is valid, and
chromium did not work, there is a good chance that osmium would work,
especially since the heat output with PVD is much less than if by sputtering
(or so I have been led to believe). If EELS imaging is being contemplated,
and since one is looking through the holes anyhow, the presence of the
osmium (or chromium) metal should not matter. We have not actually done
these experiments so in that sense this is speculation on my part.

With regard to FIB liftout samples, the perforated Si3N4 membranes might be
a solution. I have not heard that charging is a problem but if it was, then
a 1 nm layer of osmium on the membrane might solve that problem as well. Or
since a perforated Si3N4 membrane film is so much more robust than a lacy
carbon film, even chromium might not be a problem if indeed there was a
charging problem that had to be solved (this way).

Chuck

Disclaimer: SPI Supplies offers plasma cleaners, osmium coaters and
perforated silicon nitride membrane window grids so we would have a vested
interest in seeing more people using these products.

===================================================
Charles A. Garber, Ph. D. Ph: 1-(610)-436-5400
President 1-(800)-2424-SPI
SPI SUPPLIES FAX: 1-(610)-436-5755
PO BOX 656 e-mail: cgarber-at-2spi.com
West Chester, PA 19381-0656 USA Cust. Service: spi2spi-at-2spi.com

Look for us!
############################
WWW: http://www.2spi.com
############################
===================================================

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