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Intracellular cytokine staining for the characterization and quantitation of antigen-specific T lymphocyte responses.

机译:细胞内细胞因子染色,用于表征和定量抗原特异性T淋巴细胞反应。

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摘要

Standard proliferation assays used for analysis of T cell function have significant shortcomings, including limited sensitivity, lack of quantitative readouts, and considerable variability. Recently, flow cytometric methods have been developed to allow multiparametric detection of cell surface antigens and intracellular cytokine expression in response to polyclonal stimuli and antigen. We have optimized an intracellular cytokine staining assay in the non-human primate model of AIDS, which allows us to identify antigen-specific T lymphocytes at the single cell level with high sensitivity, while reducing background staining to a minimum. Central to our optimized protocol is the addition of cross-linked costimulatory anti-CD28 and anti-CD49d Mabs, a modification that results in up to 3-fold enhancement of the frequency of cytokine-secreting CD4(+) T cells following superantigen or antigen-specific stimulation. Optimization of the antigen concentration and duration of antigenic stimulation resulted in a convenient and highly reproducible assay, which permits delineation of antigen-specific cells at the single cell level, thereby providing new insights into pathogen-specific immune responses and allowing detailed phenotypic analysis of extremely low frequency events.
机译:用于T细胞功能分析的标准增殖测定法存在重大缺陷,包括灵敏度有限,缺乏定量读数以及较大的可变性。近来,已经开发了流式细胞术方法以响应于多克隆刺激和抗原而对细胞表面抗原和细胞内细胞因子表达进行多参数检测。我们在AIDS的非人类灵长类动物模型中优化了细胞内细胞因子染色测定法,这使我们能够以高灵敏度在单个细胞水平上鉴定抗原特异性T淋巴细胞,同时将背景染色降至最低。优化方案的核心是添加了交联的共刺激性抗CD28和抗CD49d单抗,这种修饰可使超抗原或抗原后分泌细胞因子的CD4(+)T细胞的频率提高多达3倍。特异性刺激。抗原浓度和抗原刺激持续时间的优化产生了一种方便且高度可重复的测定方法,该方法可以在单个细胞水平上鉴定抗原特异性细胞,从而提供了对病原体特异性免疫反应的新见解,并可以对极端低频事件。

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