Evaluation of In Vivo Breast Fine Needle Aspirates by Flow Cytometry: An Efficacy Study

doi:10.1093/jnci/84.16.1272

JNCI Journal of the National Cancer Institute 1992 84(16):1272-1276; doi:10.1093/jnci/84.16.1272
© 1992 by Oxford University Press

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Journal of the National Cancer Institute, Vol. 84, No. 16, 1272-1276, August 19, 1992
© 1992 Oxford University Press

Evaluation of In Vivo Breast Fine Needle Aspirates by Flow Cytometry: An Efficacy Study

Joseph E. Fuhr^*^,, Anthony A. Kattine, H. Sperry Nelson, Jr.

Section of Experimental Pathology, University of Tennesse Medical Center Knoxville
Department of Surgery, University of Tennesse Medical Center Knoxville

^*Correspondence to: Joseph E. Fuhr, ph.D., Section of Experimental Pathology, University of Tennessee Medical Center, 1924 Alcoa Highway, Knoxville, TN 37920.

Background: Malignancy of the breast is frequently diagnosedthrough fine needle aspiration. in the hands of a skilled aspiratorand Cytopathologist, this can be a highly accurate procedure.Purpose: This study was undertaken to evalate whether sufficientresedual cells in the bore of the needle could be harvestedand analyzed efficiently by flow cytopmetry analysis. The goalwas then to determine the value of routine flow cytometry asan adjuctive technology in the interpretation of breast fineneedle aspirations. Methods: Cells were rinsed from tthe neddlesof 83 consecutive diagnostic fine needle aspirates after preliminaryinspection had confirmed adquate material was obntained forcytopathology. Cells were washed, and nuclei prepared by detergenttreatment. Afger ribonuclease treatment, DNA was stained withthe fluorescent marler propodoium iodide. DNA content per cellwas determined by flow cytometry by measurement of right anglefluorescence. Results. Less then 4% of the sample were rejctedfor inadequate cell numbers. Flow cytometry criteria for evidenceof malignancy included the presence of a DNA aneuploid populationor an elevated rate of proliferation(13% or higher) of a diploidpopulation. Accuracy of flow cytometry was based on cytopathologicinterpretation in all cases except tow whcih were based on resultsof excisional biopsy. The sensitivity of the flow cytometryanalysis was 76% the specificity was 100, with results fromflow cytometry pivotal in the correct diagnoses for two patientswhose cytopathologic results were equivocal. Analyusis of histogramsindicateded acceptable coefficients of variation for all populations.Gating analysis indicated the suitability of the material forthis type of study, with an average of 85% of the events selected,or " gated in. " Low recoveries were associated with the presenceof necrotic debris in the sample. Conclusion: Flow cytometrycan be a valuable adjunctive technology, Capable of providingthe cytopathologist with additional information regarding thecharacter of cells an; yzed. [ J Natl Cancer Inst 84: 1272–1276,1992]

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