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通过长读转录组测序对恒河猴全长 Ig 和 TCR 库多样性进行系统分析。

Systematic Profiling of Full-Length Ig and TCR Repertoire Diversity in Rhesus Macaque through Long Read Transcriptome Sequencing.

机构信息

Department of Molecular Biomedical Sciences, North Carolina State University College of Veterinary Medicine, Raleigh, NC 27607.

Bioinformatics Graduate Program, North Carolina State University, Raleigh, NC 27695.

出版信息

J Immunol. 2020 Jun 15;204(12):3434-3444. doi: 10.4049/jimmunol.1901256. Epub 2020 May 6.

Abstract

The diversity of Ig and TCR repertoires is a focal point of immunological studies. Rhesus macaques () are key for modeling human immune responses, placing critical importance on the accurate annotation and quantification of their Ig and TCR repertoires. However, because of incomplete reference resources, the coverage and accuracy of the traditional targeted amplification strategies for profiling rhesus Ig and TCR repertoires are largely unknown. In this study, using long read sequencing, we sequenced four Indian-origin rhesus macaque tissues and obtained high-quality, full-length sequences for over 6000 unique Ig and TCR transcripts, without the need for sequence assembly. We constructed, to our knowledge, the first complete reference set for the constant regions of all known isotypes and chain types of rhesus Ig and TCR repertoires. We show that sequence diversity exists across the entire variable regions of rhesus Ig and TCR transcripts. Consequently, existing strategies using targeted amplification of rearranged variable regions comprised of V(D)J gene segments miss a significant fraction (27-53% and 42-49%) of rhesus Ig/TCR diversity. To overcome these limitations, we designed new rhesus-specific assays that remove the need for primers conventionally targeting variable regions and allow single cell level Ig and TCR repertoire analysis. Our improved approach will enable future studies to fully capture rhesus Ig and TCR repertoire diversity and is applicable for improving annotations in any model organism.

摘要

免疫球蛋白(Ig)和 T 细胞受体(TCR)的多样性是免疫研究的重点。恒河猴(Macaca mulatta)是模拟人类免疫反应的关键动物,因此准确注释和量化其 Ig 和 TCR 库对于研究至关重要。然而,由于参考资源不完整,传统靶向扩增策略在分析恒河猴 Ig 和 TCR 库中的覆盖度和准确性在很大程度上尚不清楚。在这项研究中,我们使用长读测序技术对来自印度的四只恒河猴组织进行了测序,获得了超过 6000 个独特的 Ig 和 TCR 转录本的全长高质量序列,而无需进行序列组装。我们构建了迄今为止第一个包含所有已知恒河猴 Ig 和 TCR 库的同种型和链型的恒定区的完整参考集。我们表明,恒河猴 Ig 和 TCR 转录本的整个可变区都存在序列多样性。因此,使用靶向扩增包含 V(D)J 基因片段的重排可变区的现有策略会错过很大一部分(27-53%和 42-49%)的恒河猴 Ig/TCR 多样性。为了克服这些限制,我们设计了新的恒河猴特异性检测方法,这些方法无需使用传统靶向可变区的引物,从而可以进行单细胞水平的 Ig 和 TCR 库分析。我们改进的方法将使未来的研究能够充分捕获恒河猴 Ig 和 TCR 库的多样性,并且适用于任何模式生物的注释改进。

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