[Histonet] Re: Timms stain in fresh frozen cryosections
Delatour Benoît
benoit.delatour <@t> ibaic.u-psud.fr
Wed Nov 1 08:19:13 CST 2006
Hi Anna,
You can simply incubate mounted slices in a 1.2% NaS.9H2O solution (in
buffer w/v : 0.6 g / 50 cc of PB 0.1M) for 30 min. and then, after
rinsings, proceed with TIMM staining.
It works well with the limit that cutting fresh unfixed brains and doing
repeated incubations and baths is risky (tissue goes away!). To minimize
this, cut thin (<10µm) and slowly. Let the sections dry.
Other alternatives
1) mice are alive : perfuse them with Na2S followed by fixative ; gives
excellent results.
2) brains have not yet been cut : the simplest method for lazy people is to
do "immersion autometallography" by incubating tissue in a solution of
Na2S, then fixation in formadehyde. Once slices are obtained, proceed to
TIMM staining.
Benoît
--------"If you think research is expensive, try disease"--------
B. Delatour
Laboratoire de Neurobiologie de l'Apprentissage,
de la Mémoire & de la Communication,
NAMC, CNRS UMR 8620, Bât 446
Université Paris-Sud
91405 Orsay Cedex, FRANCE
Tel:33 (0)1 69 15 49 88
Fax:33 (0)1 69 15 77 26
Mobile:0682991092
Email benoit.delatour <@t> ibaic.u-psud.fr
Web http://www.namc.u-psud.fr
More information about the Histonet
mailing list