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麸质的翻译后修饰塑造了乳糜泻中TCR的使用情况。

Posttranslational modification of gluten shapes TCR usage in celiac disease.

机构信息

Department of Immunology, Centre for Immune Regulation, University of Oslo, 0027 Oslo, Norway.

出版信息

J Immunol. 2011 Sep 15;187(6):3064-71. doi: 10.4049/jimmunol.1101526. Epub 2011 Aug 17.

DOI:10.4049/jimmunol.1101526
PMID:21849672
Abstract

Posttranslational modification of Ag is implicated in several autoimmune diseases. In celiac disease, a cereal gluten-induced enteropathy with several autoimmune features, T cell recognition of the gluten Ag is heavily dependent on the posttranslational conversion of Gln to Glu residues. Evidence suggests that the enhanced recognition of deamidated gluten peptides results from improved peptide binding to the MHC and TCR interaction with the peptide-MHC complex. In this study, we report that there is a biased usage of TCR Vβ6.7 chain among TCRs reactive to the immunodominant DQ2-α-II gliadin epitope. We isolated Vβ6.7 and DQ2-αII tetramer-positive CD4(+) T cells from peripheral blood of gluten-challenged celiac patients and sequenced the TCRs of a large number of single T cells. TCR sequence analysis revealed in vivo clonal expansion, convergent recombination, semipublic response, and the notable conservation of a non-germline-encoded Arg residue in the CDR3β loop. Functional testing of a prototype DQ2-α-II-reactive TCR by analysis of TCR transfectants and soluble single-chain TCRs indicate that the deamidated residue in the DQ2-α-II peptide poses constraints on the TCR structure in which the conserved Arg residue is a critical element. The findings have implications for understanding T cell responses to posttranslationally modified Ags.

摘要

抗原的翻译后修饰与多种自身免疫性疾病有关。在乳糜泻(一种具有多种自身免疫特征的谷物麸质诱导的肠病)中,麸质抗原的T细胞识别严重依赖于谷氨酰胺(Gln)残基向谷氨酸(Glu)残基的翻译后转化。有证据表明,对脱酰胺化麸质肽的增强识别源于肽与主要组织相容性复合体(MHC)结合的改善以及T细胞受体(TCR)与肽-MHC复合体的相互作用。在本研究中,我们报告在对免疫显性的DQ2-α-II麦醇溶蛋白表位有反应的TCR中,TCR Vβ6.7链存在偏向性使用。我们从接受麸质激发的乳糜泻患者外周血中分离出Vβ6.7和DQ2-αII四聚体阳性的CD4(+) T细胞,并对大量单个T细胞的TCR进行测序。TCR序列分析揭示了体内克隆扩增、趋同重组、半公共反应以及CDR3β环中非种系编码的精氨酸(Arg)残基的显著保守性。通过分析TCR转染子和可溶性单链TCR对原型DQ2-α-II反应性TCR进行功能测试表明,DQ2-α-II肽中的脱酰胺化残基对TCR结构构成限制,其中保守的Arg残基是关键元件。这些发现对于理解T细胞对翻译后修饰抗原的反应具有重要意义。

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