RE: [Histonet] Washing out formalin fixation (Lengthy)

From:"Marshall Terry Dr, Consultant Histopathologist"



 "These studies these show that fixation of peptide spots (essentially
zero thickness) attached to glass slides take over 6 hours to "fix" at
room temperature. In this case they defined "fixed" as the point at
which an antibody  would no longer detect it's target epitope, or the
reaction was severely diminished. They also showed that HIER reverses
the "fixation"

So far so good, and supports what I have been saying in this forum for
years about the (long) time it takes to formalin fix tissue, and the
misbelief that wetting them for a few hours is fixing.
But then......

"This calls into question any method that relies on less than six hours
formalin fixation at room temperature (ie, biopsies, just because they
are small) and also the effect of exposing those short-fixed tissues to
long exposure to 70% alcohol, or other aqueous solution, before clearing
and embedding."

I know not what this all means/is getting at.

Terry

-----Original Message-----
From: histonet-bounces@lists.utsouthwestern.edu
[mailto:histonet-bounces@lists.utsouthwestern.edu] On Behalf Of Morken,
Tim
Sent: 04 March 2008 17:17
To: histonet@lists.utsouthwestern.edu
Subject: RE: [Histonet] Washing out formalin fixation (Lengthy)


Thanks for the synopsis Bryan.

I'd like to point out that the 2004 paper by Sompuram,and a followup in
2006 are very interesting. These studies these show that fixation of
peptide spots (essentially zero thickness) attached to glass slides take
over 6 hours to "fix" at room temperature. In this case they defined
"fixed" as the point at which an antibody  would no longer detect it's
target epitope, or the reaction was severly diminished. They also showed
that HIER reverses the "fixation."


The 2006 paper also investigates why some epitopes are affected by
formalin and others are not.

Sompuram SR, Vani K, Messana E and Bogen SA. A molecular mechanism of
formalin fixation and antigen retrieval. Am J Clin Pathol (2004);121:
190-199

Sompuram, et. al, A molecular model of antigen retrieval using a peptide
array, Am J Clin Path 2006;125:91-98


Tim Morken
Technical Support Manager
Lab Vision Products
Anatomical Pathology
ThermoFisher Scientific

-----Original Message-----
From: histonet-bounces@lists.utsouthwestern.edu
[mailto:histonet-bounces@lists.utsouthwestern.edu] On Behalf Of Bryan
Hewlett
Sent: Tuesday, March 04, 2008 7:56 AM
To: Johnson, Teri; histonet@lists.utsouthwestern.edu
Subject: Re: [Histonet] Washing out formalin fixation (Lengthy)

Hi Teri and everyone else on this thread,

Washing out many of the effects of formaldehyde fixation on tissues with
running water has been known for years (much longer than this old boy
has been around).
In modern terms, it is the essential underlying mechanism for so-called
antigen retrieval (HIER).

Formaldehyde fixes proteins by addition, with the formation of
hydroxymethyl adducts on the reactive side chains of proteins.
Once enough of these hydroxymethyl adducts are formed, and IF they are
in close approximation to each other, they may slowly cross-link by the
formation of methylene bridges.
However, these adducts and initial cross-links are unstable and readily
reversed by water and alcohol (see Kiernan (1999).
It takes 24 hours at room temperature for all the hydroxymethyl adducts
to form, i.e. maximal binding threshold (see Fox et al, 1985).
If the tissue is then exposed to running water before all the adducts
have formed (i.e. less than 24 hours), the reversal is very rapid.
The shorter the time in formaldehyde, the more rapid the reversal.
Even after the essential 24 hours fixation and also after a more lengthy
6 days fixation, running water will still remove the adducts and
hydrolyse the methylene bridges.
There is at least one publication (Helander, 1994) that provides data
regarding this effect.
After 24 hours fixation, 50% reversal occurred in less than 24 hours,
90% reversal was obtained after 6 days washing and for 6 days fixation
90% reversal after 4 weeks washing.
It should be noted that these reversal times were obtained at ambient
temperatures and the times may be considerably reduced by elevated
temperatures.

This reversal effect is also obtained on tissue sections that have been
processed to wax.
However, because of the additional shrinkage and hydrophobicity of the
processed proteins, the reversal is slowed somewhat until the proteins
re-hydrate.
The reversal effect can also be aided by the presence of other ions in
the water (the purpose of HIER buffers).
Back in the sixties, in order to successfully demonstrate Ig's by IF, we
were reversing the fixation effects on paraffin sections by placing them
in hypotonic buffers for 2 days at 37C.
Today, since we are all in a great rush for results, we obviously drive
the reversal at higher temperatures to speed things up!!

References:

Baker JR (1958), Principles of Biological Microtechnique, Methuen & Co.
Ltd.
Hopwood D. Fixatives and fixation: A review. Histochemical journal
(1969); 1, p19-55 Burnett MG. The mechanism of the formaldehyde clock
reaction: Methylene glycol dehydration. J Chem. educ. (1982); 59, 160
Fox CH et al. Formaldehyde fixation. J Histochem Cytochem (1985); 33,
845-853
Helander KG. Kinetic studies of formaldehyde binding in tissue.
Biotechnique and Histochemistry. (1994); 69, 177-179 Kiernan J.A.,
Histological and Histochemical Methods: Theory and Practice, 3rd
Edition, (1999). Oxford: Butterworth-Heinemann. ISBN # 0-7506-3106-6.
Shi SR, Gu J. and Taylor CR. Antigen Retrieval Techniques:
Immunohistochemistry and Molecular Morphology. (2000) Eaton Publishing.
ISBN 1-881299-43-0.
Sompuram SR, Vani K, Messana E and Bogen SA. A molecular mechanism of
formalin fixation and antigen retrieval. Am J Clin Pathol (2004);121:
190-199


Best regards,

Bryan

----- Original Message -----
From: "Johnson, Teri" 
To: 
Sent: Monday, March 03, 2008 2:33 PM
Subject: [Histonet] Washing out formalin fixation


Last week, a researcher here asked me what the chemical mechanism was of

washing out the effects of formalin fixation on the tissues with running

water. In other words, how does it work? Anybody here know?

Teri Johnson, HT(ASCP)QIHC
Managing Director Histology Facility
Stowers Institute for Medical Research
1000 E. 50th St.
Kansas City, MO 64110


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