Enhanced Detection of Antigen-Specific CD4+ T Cells Using Altered Peptide Flanking Residue Peptide–MHC Class II Multimers

The Journal of Immunology Author Choice Pub Date : 2015-11-09 DOI:10.4049/jimmunol.1402787

C. Holland, G. Dolton, M. Scurr, K. Ladell, Andrea Schauenburg, K. Miners, Florian Madura, A. Sewell, D. Price, D. Cole, A. Godkin

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引用次数: 11

Abstract

Fluorochrome-conjugated peptide–MHC (pMHC) class I multimers are staple components of the immunologist’s toolbox, enabling reliable quantification and analysis of Ag-specific CD8+ T cells irrespective of functional outputs. In contrast, widespread use of the equivalent pMHC class II (pMHC-II) reagents has been hindered by intrinsically weaker TCR affinities for pMHC-II, a lack of cooperative binding between the TCR and CD4 coreceptor, and a low frequency of Ag-specific CD4+ T cell populations in the peripheral blood. In this study, we show that peptide flanking regions, extending beyond the central nonamer core of MHC-II–bound peptides, can enhance TCR–pMHC-II binding and T cell activation without loss of specificity. Consistent with these findings, pMHC-II multimers incorporating peptide flanking residue modifications proved superior for the ex vivo detection, characterization, and manipulation of Ag-specific CD4+ T cells, highlighting an unappreciated feature of TCR–pMHC-II interactions.

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利用改变的肽侧残基肽- mhc II类多聚体增强抗原特异性CD4+ T细胞的检测

荧光染料共轭肽- mhc (pMHC) I类多聚物是免疫学家工具箱的主要组成部分，无论功能输出如何，都可以对ag特异性CD8+ T细胞进行可靠的定量和分析。相比之下，等效pMHC II类(pMHC-II)试剂的广泛使用受到TCR对pMHC-II本质上较弱的亲和力、TCR与CD4辅助受体之间缺乏协同结合以及外周血中ag特异性CD4+ T细胞群的低频率的阻碍。在这项研究中，我们发现肽侧翼区域延伸到mhc - ii结合肽的中心高分子核心之外，可以增强TCR-pMHC-II结合和T细胞活化，而不会失去特异性。与这些发现一致，结合肽侧残基修饰的pMHC-II多聚体被证明在ag特异性CD4+ T细胞的体外检测、表征和操作方面具有优势，突出了TCR-pMHC-II相互作用的一个未被认识的特征。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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The Journal of Immunology Author Choice

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