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首页> 外文期刊>Journal of Immunological Methods >An optimized multi-parameter flow cytometry protocol for human T regulatory cell analysis on fresh and viably frozen cells, correlation with epigenetic analysis, and comparison of cord and adult blood
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An optimized multi-parameter flow cytometry protocol for human T regulatory cell analysis on fresh and viably frozen cells, correlation with epigenetic analysis, and comparison of cord and adult blood

机译:一种优化的多参数流式细胞术方案,用于对新鲜和有活力的冷冻细胞进行人T调节细胞分析,与表观遗传学分析的相关性以及脐带血和成人血的比较

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摘要

Multi-parameter flow cytometry analysis of T regulatory (Treg) cells is a widely used approach in basic and translational research studies. This approach has been complicated by a lack of specific markers for Treg cells and lack of uniformity in the quantification of Treg cells. Given the central role of Treg cells in the inception and perpetuation of diverse immune responses as well as its target as a therapeutic, it is imperative to have established methodologies for Treg cell analysis that are robust and usable for studies with multiple subjects as well as multicenter studies. In this study, we describe an optimized multi-parameter flow cytometry protocol for the quantification of human Treg cells from freshly obtained and viably frozen samples and correlations with epigenetic Treg cell analysis (TSDR demethylation). We apply these two methodologies to characterize Treg cell differences between cord blood and adult peripheral blood. In summary, the optimized protocol appears to be robust for Treg cell quantification from freshly isolated or viably frozen cells and the multi-parameter flow cytometry findings are strongly positively correlated with TSDR demethylation thus providing several options for the characterization of Treg cell frequency and function in large translational or clinical studies.
机译:T调节(Treg)细胞的多参数流式细胞术分析是基础研究和转化研究中广泛使用的方法。由于缺乏Treg细胞的特异性标记物以及Treg细胞定量的均一性,这种方法变得很复杂。鉴于Treg细胞在多种免疫反应的发生和持续过程中起着核心作用,以及其作为治疗靶点,迫切需要为Treg细胞分析建立可靠且可用于多个受试者和多中心研究的方法学。学习。在这项研究中,我们描述了一种优化的多参数流式细胞术方案,用于量化来自新鲜获得的和有活力的冷冻样品中人Treg细胞的定量以及与表观遗传Treg细胞分析(TSDR去甲基化)的相关性。我们应用这两种方法来表征脐带血和成人外周血之间的Treg细胞差异。总而言之,优化的方案对于从新鲜分离的或存活的冷冻细胞中进行Treg细胞定量分析似乎是可靠的,并且多参数流式细胞术的发现与TSDR去甲基化密切相关,因此为表征Treg细胞的频率和功能提供了多种选择大型翻译或临床研究。

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