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在小鼠单细胞水平对 TCRα 和 TCRβ 链进行配对分析。

Paired analysis of TCRα and TCRβ chains at the single-cell level in mice.

机构信息

St Jude Children’s Research Hospital, Memphis, Tennessee 38105-3678, USA.

出版信息

J Clin Invest. 2011 Jan;121(1):288-95. doi: 10.1172/JCI44752. Epub 2010 Dec 6.

DOI:10.1172/JCI44752
PMID:21135507
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3007160/
Abstract

Characterizing the TCRα and TCRβ chains expressed by T cells responding to a given pathogen or underlying autoimmunity helps in the development of vaccines and immunotherapies, respectively. However, our understanding of complementary TCRα and TCRβ chain utilization is very limited for pathogen- and autoantigen-induced immunity. To address this problem, we have developed a multiplex nested RT-PCR method for the simultaneous amplification of transcripts encoding the TCRα and TCRβ chains from single cells. This multiplex method circumvented the lack of antibodies specific for variable regions of mouse TCRα chains and the need for prior knowledge of variable region usage in the TCRβ chain, resulting in a comprehensive, unbiased TCR repertoire analysis with paired coexpression of TCRα and TCRβ chains with single-cell resolution. Using CD8+ CTLs specific for an influenza epitope recovered directly from the pneumonic lungs of mice, this technique determined that 25% of such effectors expressed a dominant, nonproductively rearranged Tcra transcript. T cells with these out-of-frame Tcra mRNAs also expressed an alternate, in-frame Tcra, whereas approximately 10% of T cells had 2 productive Tcra transcripts. The proportion of cells with biallelic transcription increased over the course of a response, a finding that has implications for immune memory and autoimmunity. This technique may have broad applications in mouse models of human disease.

摘要

鉴定针对特定病原体或潜在自身免疫的 T 细胞表达的 TCRα 和 TCRβ 链,分别有助于疫苗和免疫疗法的开发。然而,我们对病原体和自身抗原诱导的免疫中互补 TCRα 和 TCRβ 链利用的理解非常有限。为了解决这个问题,我们开发了一种多重嵌套 RT-PCR 方法,用于从单个细胞同时扩增编码 TCRα 和 TCRβ 链的转录本。这种多重方法避免了缺乏针对小鼠 TCRα 链可变区的特异性抗体的问题,也不需要事先了解 TCRβ 链中可变区的使用情况,从而实现了全面、无偏倚的 TCR 库分析,并具有单细胞分辨率的 TCRα 和 TCRβ 链的配对共表达。使用直接从患有肺炎的小鼠肺部回收的针对流感表位的 CD8+ CTL,该技术确定 25%的此类效应器表达主要的、非生产性重排的 Tcra 转录本。具有这些无框 Tcra mRNA 的 T 细胞也表达另一种框架内的 Tcra,而大约 10%的 T 细胞具有 2 个有功能的 Tcra 转录本。具有双等位基因转录的细胞比例随着反应的进行而增加,这一发现对免疫记忆和自身免疫具有重要意义。该技术可能在人类疾病的小鼠模型中有广泛的应用。

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本文引用的文献

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