[Histonet] slides for frozens
Rene J Buesa
rjbuesa <@t> yahoo.com
Thu Feb 2 14:08:02 CST 2012
That could be the solution. The problem is that you changed 2 things: the protocol and the slides and now you do not know which is "the culprit". Returning to the old protocols is a first step to trying to solve the present situation and, as you can imagine, if the old protocol does not solve the problem, the slides may be the cause.
René J.
--- On Thu, 2/2/12, Sherwood, Margaret <MSHERWOOD <@t> PARTNERS.ORG> wrote:
From: Sherwood, Margaret <MSHERWOOD <@t> PARTNERS.ORG>
Subject: RE: [Histonet] slides for frozens
To: "Rene J Buesa" <rjbuesa <@t> yahoo.com>, "histonet" <histonet <@t> lists.utsouthwestern.edu>
Date: Thursday, February 2, 2012, 3:03 PM
That may be true, but I don't recall having this problem with our previous
protocol (which was longer and included a fix in alcoholic formalin). I think
we will try the "old" method and see what happens.
Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (EDR 214)
Massachusetts General Hospital
50 Blossom Street
Boston, MA 02114-2696
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-1206 (fax)
msherwood <@t> partners.org
________________________________
From: Rene J Buesa [mailto:rjbuesa <@t> yahoo.com]
Sent: Thursday, February 02, 2012 2:57 PM
To: histonet; Sherwood, Margaret
Subject: Re: [Histonet] slides for frozens
There is a known saying that goes: "You get what you pay for".
René J.
--- On Thu, 2/2/12, Sherwood, Margaret <MSHERWOOD <@t> PARTNERS.ORG> wrote:
From: Sherwood, Margaret <MSHERWOOD <@t> PARTNERS.ORG>
Subject: Re: [Histonet] slides for frozens
To: "histonet" <histonet <@t> lists.utsouthwestern.edu>
Date: Thursday, February 2, 2012, 2:46 PM
To all:
We have been using the same slides for paraffins and frozens. We have
no
trouble with paraffin-embedded tissue adhering to the slides through the
whole
staining procedure. But our frozens (even 5um sections)have been
falling off
during manual staining. The slides are (+) charged. We used to use
slides from
Fisher, but they are so expensive, we changed to an independent vendor
(half the
price).
Our procedure for frozen H&Es has recently changed:
1. Fix in 95% ETOH 1 min.
2. Hematoxylin 5 min.
3. Acetic acid H2O 2 quick dips
4. Wash-running H2O 10 seconds (10 dips)
5. Bluing reagent 10 dips
6. Wash-running H2O 10 seconds (or 10 dips)
7. Eosin 5 seconds
8. Dehydrate-95% ETOH 10 dips each
9. Dehydrate-100%ETOH 10 dips each
10.CitriSolv 10 dips each
11.Coverslip
The tissue seems to fall off in the bluing reagent (we order from
Mossberg).
Can anyone help us? Suggest anything--what slides you are using? We
have had
the same problem with special stains (i.e. Oil Red O for fat on
frozens).
Thanks!
Peggy
P.S. I use the same slides for my 1um plastic embedding which I dip in
water
rinses and have no problem with the tissue falling off.
Peggy Sherwood
Lab Associate, Photopathology
Wellman Center for Photomedicine (EDR 214)
Massachusetts General Hospital
50 Blossom Street
Boston, MA 02114-2696
617-724-4839 (voice mail)
617-726-6983 (lab)
617-726-1206 (fax)
msherwood <@t> partners.org
<http://us.mc1621.mail.yahoo.com/mc/compose?to=msherwood@partners.org>
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