Optimized processing of fine-needle lymph node biopsies for automated immunostaining

Optimized processing of fine-needle lymph node biopsies for automated immunostaining

A straightforward, reliable technique for postcollection processing and evaluation of cytologic specimens for antigen detection using an automated immunostainer was developed. Visual assessment of cell suspension turbidity was used in parallel with light microscopic examination of concentrated cytos...

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Bibliographic Details
Published in:Journal of veterinary diagnostic investigation Vol. 22; no. 3; pp. 383 - 388
Main Authors: Aulbach, Adam D, Swenson, Cheryl L, Kiupel, Matti
Format: Journal Article
Language:English
Published: Los Angeles, CA SAGE Publications 01-05-2010
Subjects:
accuracy
animal diseases
Animals
automatic detection
Automation
B-lymphocytes
biopsy
Biopsy, Fine-Needle - methods
Biopsy, Fine-Needle - veterinary
CD3 Complex - analysis
CD79 Antigens - analysis
cell biology
cytospin
differential staining
disease diagnosis
dog diseases
Dog Diseases - immunology
Dog Diseases - pathology
Dogs
image analysis
immunocytochemistry
Immunohistochemistry - methods
Immunophenotyping
immunostaining
lymph nodes
Lymph Nodes - pathology
lymphoma
Lymphoma - immunology
Lymphoma - pathology
Lymphoma - veterinary
Lymphoma, B-Cell - immunology
Lymphoma, B-Cell - pathology
Lymphoma, B-Cell - veterinary
neoplasms
T-lymphocytes
validity
Automated immunostaining
CD79a
fine-needle biopsy processing
cluster of differentiation (CD)3e
lymphoma
dogs
immunocytochemistry
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Summary:A straightforward, reliable technique for postcollection processing and evaluation of cytologic specimens for antigen detection using an automated immunostainer was developed. Visual assessment of cell suspension turbidity was used in parallel with light microscopic examination of concentrated cytospin preparations to verify the diagnostic utility of samples for immunocytochemical staining. Fine-needle lymph node biopsies from 81 dogs with lymphadenomegally and a cytologic or histologic diagnosis of lymphoma were introduced into ethylenediamine tetra-acetic acid tubes containing standardized storage media. Cell suspension turbidity was assessed to estimate cell concentration and resultant volume required for cytospin preparations with optimal cellularity. Preliminary cytospin preparations (using estimated volumes based upon turbidity) were stained using modified Wright stain and examined microscopically for intact neoplastic cell concentration. Once an optimal volume for cytospin preparations was established, additional concentrated slides were prepared for immunophenotyping, using an automated immunostainer and antibodies specific for cluster of differentiation (CD)79a and CD3e. All cell suspension samples with adequate gross turbidity had ample intact neoplastic cell concentration for immunocytochemical staining. Based on CD79a and CD3e expression, 51 (63%) B cell, 19 (23%) T cell, 3 mixed T and B cells (4%), and 3 non-T- and non-B-cell lymphomas (4%), as well as 5 (6%) nondiagnostic samples were identified. Three out of 5 of the nondiagnostic samples were submitted early in the investigation prior to the establishment of gross specimen turbidity guidelines. Immunocytochemical staining results were in complete agreement with all 6 available immunohistochemical correlates. The ability to visually assess sample adequacy prior to sample submission may encourage more widespread use of immunocytochemical techniques.
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ISSN:1040-6387
1943-4936
DOI:10.1177/104063871002200306