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用于检测抗原特异性细胞介导细胞毒性的FATT-CTL检测法。

FATT-CTL assay for detection of antigen-specific cell-mediated cytotoxicity.

作者信息

van Baalen Carel A, Gruters Rob A, Berkhoff Eufemia G M, Osterhaus Albert D M E, Rimmelzwaan Guus F

机构信息

Department of Virology, Erasmus MC University Medical Center and Postgraduate School of Molecular Medicine, Rotterdam, The Netherlands.

出版信息

Cytometry A. 2008 Nov;73(11):1058-65. doi: 10.1002/cyto.a.20613.

DOI:10.1002/cyto.a.20613
PMID:18636472
Abstract

Here we describe a flowcytometric assay that measures the defining function of virus-specific cytotoxic T lymphocytes (CTL), i.e., killing viral protein expressing cells. The fluorescent antigen-transfected target cell (FATT)-CTL assay requires no viruses, recombinant viral vectors, or radioactive isotopes to generate CTL target cells that present naturally processed epitopes. It facilitates developing standardized applications in clinical trial settings. Plasmid vectors encoding antigen-green fluorescent protein (GFP) fusion proteins were used directly to nucleofect immortalized B cells or peripheral blood mononuclear cells (PBMCs). Elimination of antigen-GFP expressing cells by cloned CTL, in vitro sensitized PBMC, or ex vivo PBMC was quantified following a 4-18-h coculture period by flowcytometry. This technology successfully detected cell-mediated cytotoxicity in studies involving human PBMC and various viral antigens, including structural proteins of influenza A virus, and structural and nonstructural HIV proteins. Standardized protocols are currently being developed in the framework of a clinical immunotherapy trial in HIV-infected individuals. The FATT-CTL assay principles facilitate standardized flowcytometric detection of antigenic protein-specific cell-mediated cytotoxicity in many different basic research and clinical trial settings. By measuring their defining function, the FATT-CTL assay contributes to a more complete assessment of antigen-specific CTL responses to infection and vaccination.

摘要

在此,我们描述了一种流式细胞术检测方法,该方法可测量病毒特异性细胞毒性T淋巴细胞(CTL)的关键功能,即杀伤表达病毒蛋白的细胞。荧光抗原转染靶细胞(FATT)-CTL检测方法无需病毒、重组病毒载体或放射性同位素即可产生呈现天然加工表位的CTL靶细胞。它有助于在临床试验环境中开发标准化应用。编码抗原-绿色荧光蛋白(GFP)融合蛋白的质粒载体直接用于核转染永生化B细胞或外周血单核细胞(PBMC)。在4至18小时的共培养期后,通过流式细胞术对克隆的CTL、体外致敏的PBMC或离体PBMC消除表达抗原-GFP细胞的情况进行定量。该技术在涉及人PBMC和各种病毒抗原(包括甲型流感病毒的结构蛋白以及HIV的结构和非结构蛋白)的研究中成功检测到细胞介导的细胞毒性。目前正在针对HIV感染者的临床免疫治疗试验框架内制定标准化方案。FATT-CTL检测原理有助于在许多不同的基础研究和临床试验环境中对流式细胞术检测抗原蛋白特异性细胞介导的细胞毒性进行标准化。通过测量其关键功能,FATT-CTL检测有助于更全面地评估抗原特异性CTL对感染和疫苗接种的反应。

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