[Histonet] Golgi Cox staining
histo <@t> ambree.com
histo <@t> ambree.com
Fri Aug 27 08:55:14 CDT 2004
I try to establish a Golgi Cox staining for mouse brain tissue. After the
first trials, I have two major problems:
1) The slices (between 20 and 80µm) cut from paraffin blocks using a
sliding microtome are rather fragile.
2) There are so many neurones stained, that I do not know, how to
distinguish between them and how to quantify the data.
Does anybody have an idea to solve these problems?
Thank you, and kind regards
Oliver Ambrée
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Oliver Ambrée
Institute of Neuropathology
University Hospital Münster
Domagkstr. 19
D - 48149 Münster
phone: +49 251/ 83-52359
fax: +49 251/ 83-56971
ambree <@t> uni-muenster.de
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