Nine-color flow cytometry for accurate measurement of T cell subsets and cytokine responses. Part II: Panel performance across different instrument platforms. Academic Article uri icon

Overview

abstract

  • Cellular immune responses elicited by vaccination are complex and require polychromatic analysis to accurately characterize the phenotype and function of rare, responding cells. Technical challenges and a lack of instrument standardization between research sites have limited the application of polychromatic cytometry in multicenter clinical trials. Two previously developed six-color T cell subset immunophenotyping reagent panels deliberately designed to accommodate three additional low frequency functional measurements were compared for their reproducibility of staining across three different flow cytometers. We repeatedly measured similar T cell subset frequencies between the two reagent panels and across the three different cytometers. Spectral overlap reduced sensitivity in two of the three open measurement channels (PE [IL-2] and APC [IFN gamma]) for one reagent combination, particularly in subsets with low cytokine expression. There was no significant interassay variation for measurements across instrument platforms. Careful panel design will identify reagent combinations that minimize spectral spillover into channels reserved for cytokine measurement and comparable results can be achieved using different cytometers, however, it is important to establish standardized quality control procedures for each instrument to minimize variation between cytometers.

publication date

  • May 1, 2008

Research

keywords

  • Cytokines
  • Flow Cytometry
  • Immunophenotyping
  • T-Lymphocyte Subsets

Identity

PubMed Central ID

  • PMC9191636

Scopus Document Identifier

  • 42949176079

Digital Object Identifier (DOI)

  • 10.1002/cyto.a.20555

PubMed ID

  • 18383309

Additional Document Info

volume

  • 73

issue

  • 5