The cells are definitely in the blocks.  And we are filtering the formalin bath 
also.  Thanks all!
Brandi



(prev response I received included here just for everyone's info)
I would be more suspicious of the formalin "bath" that the tissues are
sitting in while they await being placed on the processor.  Those
containers of formalin are often very cruddy by the end of the day -
bits of tissue that may be on the ends of gloves, etc often end up in
the container.  Strain out the bits of tissue one night and see what
kind of debris is floating amongst your blocks!  It is very important to
begin each day with a new container for formalin.  

Tissue can migrate too - we have seen very messy endometrial biopsies
that "share" with the blocks adjacent to them in the rack.  It can
happen.  

Sheila 







-----Original Message-----
From: kim.dona...@bhcpns.org
To: tigger...@aol.com
Cc: histonet@lists.utsouthwestern.edu; histonet-boun...@lists.utsouthwestern.edu
Sent: Wed, Mar 24, 2010 1:00 pm
Subject: Re: [Histonet] Contamination..processor?



You are definite that the cells are in the block? If so I would change all the 
paraffins out as well, even the paraffin on your embedding center. 




Kim Donadio 
Pathology Supervisor
Baptist Hospital
1000 W Moreno St.
Pensacola FL 32501
Phone (850) 469-7718
Fax (850) 434-4996 




tigger...@aol.com 
Sent by: histonet-boun...@lists.utsouthwestern.edu 
03/24/2010 11:40 AM 



To

histonet@lists.utsouthwestern.edu 


cc



Subject

[Histonet] Contamination..processor?















Hello everyone.

    Today we have a problem with contamination.  The pathologist notes cells 
from tonsil specimens here and there on our GI biopsy slides.  The cells are in 
the block.  I'm trying to ascertain the source of the contamination.  
    The grossing pathologist grossed the tonsils AFTER all GI specimens 
yesterday (not source of contaminant).  We (the techs) embedded all GI 
specimens first, trimmed, cut, floated and stained ALL GI specimens BEFORE the 
tonsils (not source of contaminant).  The only other source of the 
contamination I can think of is from the tissue processor.  We have a Tissue 
Tek VIP closed processor.  Has anyone ever experienced any problems like this?  
We had a similar issue a few weeks ago.  I thought the contaminant cells may be 
from a bladder tumor, which had multiple sections submitted.  In this instance 
the cells showed up days work of the bladder tumor, and in the following days 
work also (though the pathologists could not say for sure the cells were from 
the bladder case).  We changed our formalin solutions in the processor and the 
problem did not present the next day.  We also started putting all bladder 
tumor specimens in the microcassettes, to prevent tissue from escaping.  Has 
anyone had any problem like this, or does anyone have any ideas on how to 
prevent this in the future?  We had not seen this problem until these past two 
incidences, and this tonsil problem is particularly strange to me because we 
process tonsils and GI specimens in the same workload on a regular basis and 
have never had this issue before.  Any help is appreciated!  

Thanks!
Brandi


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