Considerations for the Control of Background Fluorescence in Clinical Flow Cytometry

R (Ruud) Hulspas, MRG O'Gorman, BL Wood, Jan willem Gratama, DR Sutherland

Research output: Contribution to journalArticleAcademicpeer-review

150 Citations (Scopus)


Accurate measurement of antigen-positive cells by flow cytometry can be hampered by background fluorescence of antigen-negative cells and other particles (e.g., debris). This article focuses on three major causes of background (autofluorescence, spectral overlap, and undesirable antibody binding) by reviewing individual aspects of flow cytometric measurements that contribute to these causes. The appropriate use of controls facilitates a thorough understanding of these contributing factors as well as the development of robust cell labeling protocols intended for routine flow cytometric analysis. We present a set of recommendations that enables the user to develop an optimized cell labeling protocol that minimizes background and maximizes the ability to reliably distinguish between a positive and a negative population of cells. These recommendations are also intended to augment existing guidelines designed to aid in the formulation of a consensus regarding the utility of flow cytometry for the analysis of clinical samples. (C) 2009 Clinical Cytometry Society
Original languageUndefined/Unknown
Pages (from-to)355-364
Number of pages10
JournalCytometry Part B-Clinical Cytometry
Issue number6
Publication statusPublished - 2009

Cite this