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Clinical and Diagnostic Laboratory Immunology, May 1995, 337-342, Vol 2, No. 3
KR Tamul, JL Schmitz, K Kane and JD Folds
We compared flow cytometric immunophenotyping results obtained by using the
lysed whole blood method of sample preparation with those obtained by using
Ficoll-Hypaque-separated cells on 44 consecutive specimens from patients
with various hematologic malignancies. When the samples were analyzed as a
group, seven antigens (CD2, CD3, CD5, CD11c, CD20, CD22, and CD34)
demonstrated significantly different percentages of positively staining
cells. When the samples were grouped by disease, results for patients with
acute lymphocytic leukemia were discordant for CD22 and HLA-DR and results
for patients with hairy cell leukemia were discordant for CD34. Most of the
differences, however, were not with antigens critical to the evaluation of
the malignancy. Additionally, the most frequent reason for differences in
the percentage of positive cells was due to isotype control-based placement
of the quadrant markers and not an actual discrepancy in staining. However,
analysis of the CD34 antigen yielded eight instances in which staining of
Ficoll-Hypaque-separated cells was essentially negative, but a clearly
positive population was evident with the lysed preparation. This finding
has important implications because of the prognostic significance of this
antigen. Further studies are needed to determine the cause of this
phenomenon.
Copyright © 1995 by the American Society for Microbiology. All rights reserved.
Comparison of the effects of Ficoll-Hypaque separation and whole blood lysis on results of immunophenotypic analysis of blood and bone marrow samples from patients with hematologic malignancies
Clinical Immunology Laboratory, University of North Carolina Hospitals, Chapel Hill 27514, USA.
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