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In-depth determination and analysis of the human paired heavy- and light-chain antibody repertoire

机译:人配对重链和轻链抗体库的深入测定和分析

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High-throughput immune repertoire sequencing has emerged as a critical step in the understanding of adaptive responses following infection or vaccination or in autoimmunity. However, determination of native antibody variable heavy-light pairs (VH-VL pairs) remains a major challenge, and no technologies exist to adequately interrogate the >1 x 10(6) B cells in typical specimens. We developed a low-cost, single-cell, emulsion-based technology for sequencing antibody VH-VL repertoires from >2 x 10(6) B cells per experiment with demonstrated pairing precision >97%. A simple flow-focusing apparatus was used to sequester single B cells into emulsion droplets containing lysis buffer and magnetic beads for mRNA capture; subsequent emulsion RT-PCR generated VH-VL amplicons for next-generation sequencing. Massive VH-VL repertoire analyses of three human donors provided new immunological insights including (i) the identity, frequency and pairing propensity of shared, or 'public', VL genes, (ii) the detection of allelic inclusion (an implicated autoimmune mechanism) in healthy individuals and (iii) the occurrence of antibodies with features, in terms of gene usage and CDR3 length, associated with broadly neutralizing antibodies to rapidly evolving viruses such as HIV-1 and influenza.
机译:高通量免疫库测序已成为理解感染或疫苗接种或自身免疫后适应性反应的关键步骤。然而,确定天然抗体可变重链对(VH-VL对)仍然是一项重大挑战,并且还没有技术可以对典型标本中的> 1 x 10(6)B细胞进行充分讯问。我们开发了一种低成本,单细胞,基于乳液的技术,每个实验可从> 2 x 10(6)个B细胞中对抗体VH-VL组成成分进行测序,并证明配对精度> 97%。使用简单的流聚焦设备将单个B细胞隔离到含有裂解缓冲液和磁珠的mRNA乳液乳液液滴中;随后的乳液RT-PCR生成了VH-VL扩增子,用于下一代测序。对三位人类供体的大规模VH-VL血库分析提供了新的免疫学见解,包括(i)共享或“公共” VL基因的身份,频率和配对倾向,(ii)等位基因包涵体的检测(涉及的自身免疫机制) (iii)在基因使用和CDR3长度方面具有特征的抗体的出现,这些特征与针对迅速发展的病毒(如HIV-1和流感)的广泛中和抗体有关。

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