RE: [Histonet] guidelines
The question I have is what do you do when you have to start moving
results times back and the clinicians are already breathing down your
neck for the DX. I like the idea that you take a piece of tissue and
process it ahead of the rest this solves the issue of getting a
diagnosis, or you could even do a frozen section (if possible). Has
anyone looked at microwave processing as the answer to this?? Has the
FDA approved breast studies on microwave processed tissue? I note the
the current quote that was given states, as long as it is in occordance
with the same result, that it is ok, does not cut it. What if you are a
lab that is sending out blocks to have this study done and you are not
fixing the specimen adequatley?? What if you do not do the studies but
do the image analysis on the HER2 block??
Jesus A. Ellin HT ASCP
Yuma Regional Medical Center
Histology Systems Technologist
Pathology Information Systems
928-336-7444 or 928-336-1144
Fax: 928-336-7319
-----Original Message-----
From: histonet-bounces@lists.utsouthwestern.edu
[mailto:histonet-bounces@lists.utsouthwestern.edu] On Behalf Of Douglas
D Deltour
Sent: Monday, January 15, 2007 10:56 AM
To: 'Patsy Ruegg'; 'Webb, Dorothy L'; Histonet@lists.utsouthwestern.edu
Subject: RE: [Histonet] guidelines
You can use an alternative fixative if you would like.
This is from APPENDIX E Tissue Handling Requirement and Control
Materials
"Any alteration of standard conditions, such as use of alternative
fixatives, microwave fixation, or alternative processing methods, must
be validated against standard methods of testing before a test routinely
using these conditions is offered in a laboratory. Validation must
consist of testing of the same samples with the alternative fixative
buffered formalin using the same HER2 testing method to demonstrate
concordance of the result."
http://arpa.allenpress.com/pdf/i1543-2165-131-1-18.pdf
Douglas D. Deltour HT(ASCP)
Histology Supervisor
Professional Pathology Services, PC
One Science Court
Suite 200
Columbia, SC 29203
(803)252-1913
Fax (803)254-3262
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-----Original Message-----
From: histonet-bounces@lists.utsouthwestern.edu
[mailto:histonet-bounces@lists.utsouthwestern.edu] On Behalf Of Patsy
Ruegg
Sent: Monday, January 15, 2007 12:00 PM
To: 'Webb, Dorothy L'; Histonet@lists.utsouthwestern.edu
Subject: RE: [Histonet] guidelines
Dorothy et al,
One reason for the new Her2 guidelines from CAP is that there has been a
discrepancy in results when samples are not adequately fixed in formalin
and/or alcohol fixed. If the sample is not adequately cross linked by
formalin fixation before it is processed, alcohols can damage or destroy
the
Her2 protein making it unavailable for detection. Your best bet is to
fix
the sample for 24 hrs. in formalin, then it will be protected from
processing and can be retrieved but at least it is still there. I know,
who
has time to fix for 24hrs., well an approach to that could be that you
take
a piece of the sample and process it quickly for the H&E, while leaving
another piece to fix for 24hrs., by the time the H&E is read and Her2
ordered your sample will be properly fixed, will withstand paraffin
processing, then you do the IHC on the fixed piece. Requiring a minimum
of
6 hrs fixation in formalin is how CAP is starting to address this
problem.
I expect that I am opening up a can of worms here but I think this is
what
this is about. Studies have been done in labs using alcohol fixatives
and/or inadequate formalin fixation that show a drop in up to 30% of
positive Her2 cases. That should be telling.
Patsy
-----Original Message-----
From: histonet-bounces@lists.utsouthwestern.edu
[mailto:histonet-bounces@lists.utsouthwestern.edu] On Behalf Of Webb,
Dorothy L
Sent: Monday, January 15, 2007 9:00 AM
To: Histonet@lists.utsouthwestern.edu
Subject: [Histonet] guidelines
With the new Her2 guidelines from CAP, how is everyone planning on
handling not using alcoholic fixation of fatty breast tissue? We have
been using Davidson's on mastectomy and lumpectomy specimens (not needle
bx.s) and I have a dedicated processor with the first two stations of an
alcoholic formalin fixative. My pathologists want these breast
specimens to not be placed in these type of fixatives in lieu of the new
regs and I am already seeing underprocessed fatty breast tissue. Does
anyone have a longer processing time for their breast (fatty) specimens
they would be willing to share with me?
Also, does anyone have a dedicated pneumatic tube system for your OR
directly to histology for small specimens? Our facility is looking into
this and I would appreciate any feedback!!
Thanks ahead of time for any help in this area..I love this valuable
access to my fellow histology lab workers!!
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