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The flow cytometric PKH-26 assay for the determination of T-cell mediated cytotoxic activity.

机译:用于确定T细胞介导的细胞毒活性的流式细胞术PKH-26分析。

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We present a rapid flow cytometric and non-radioactive functional assay developed for the determination of the cytotoxic activity of T lymphocytes, natural killer cells, and lymphokine-activated killer cells. In contrast to indirect evaluation of cytotoxicity using radioactive assays, this assay is based on the quantitative and qualitative flow cytometric analysis of cell damage on a single cell level. Target cells are stained with PKH-26, a lipophilic dye that stably integrates into the cell membrane, without disturbing its surface marker expression. It, thus, permits the distinction between target and effector cells. After short term in vitro incubation (1.5-3h), AnnexinV-FITC (ann-FITC) staining allows to discriminate between apoptotic and non-apoptotic target cells. Data analysis is performed first by gating on PKH-26 positive target cells, followed by the analysis of the ann-FITC positive subpopulation. The percentage of cytotoxicity in the PKH-26 gated cell population is calculated by subtractingunspecific ann-FITC positive target cells, measured in appropriate controls without effector cells. Using in vitro generated antigen-specific cytotoxic T lymphocytes, we demonstrate that this flow cytometric assay is sensitive, correlates well with the standard 51Cr release assay, and is easy to handle.
机译:我们提出了一种快速流式细胞仪和非放射性功能测定法,用于测定T淋巴细胞,天然杀伤细胞和淋巴因子激活的杀伤细胞的细胞毒活性。与使用放射性测定法间接评估细胞毒性相反,该测定法基于单个细胞水平上细胞损伤的定量和定性流式细胞仪分析。靶细胞用PKH-26染色,PKH-26是一种亲脂性染料,可稳定整合到细胞膜中,而不会干扰其表面标志物的表达。因此,它可以区分靶细胞和效应细胞。短期体外孵育(1.5-3h)后,AnnexinV-FITC(ann-FITC)染色可区分凋亡和非凋亡靶细胞。首先通过对PKH-26阳性靶细胞进行门控来进行数据分析,然后分析ann-FITC阳性亚群。 PKH-26门控细胞群中细胞毒性的百分比是通过减去未特异性的an-FITC阳性靶细胞(在没有效应细胞的适当对照中测得)来计算的。使用体外产生的抗原特异性细胞毒性T淋巴细胞,我们证明了这种流式细胞术测定法灵敏,与标准51Cr释放测定法很好地相关,并且易于操作。

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