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Analyzing T cell repertoire diversity by high-throughput sequencing

机译:通过高通量测序分析T CelectoIre多样性

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Diversity on a large scale is one of the most striking and powerful features utilized by the mammalian immune system to fight off a vast universe of pathogens. The T-cell driven immune response is characterized by a multitude of distinct receptors capable of antigen recognition with high specificity. Using high-throughput sequencing we are able to investigate the T cell receptor (TCR) repertoire as the collection of its individual receptors, aiming to profile the global properties of the complementarily determining region 3 (CDR3) of the TCR in human immunity. However, analysis of the data is highly sensitive to single nucleotide polymoprhisms, read length and error rate, accuracy in mapping to a genomic reference, and our ability to translate the sequence, in silico, in the appropriate reading frame. We have developed a computational pipeline that performs error correction on overlapping paired-end long (250 nt) reads, and maps the reads unambiguously to V and J cassettes corresponding to TCR-α and -β chains. Our methods were applied to functional T cell receptors from healthy blood tissue and to several patients with low grade glioma (LGG) and glioblastoma multiforme (GBM). We used Shannon entropy to measure levels of diversity in the productive T cell repertoire and observed that greater than 50% of the TCR diversity can be explained by V, J cassette usage.
机译:大规模的多样性是哺乳动物免疫系统利用的最引人注目和强大的特征之一,以消除巨大的病原体宇宙。 T细胞驱动免疫应答的特征在于能够具有高特异性抗原识别的多种不同的受体。使用高通量测序我们能够研究T细胞受体(TCR)曲目作为其个体受体的收集,旨在简要互补决定区域3(CDR3)的全局性质在人类免疫中。然而,对数据的分析对单核苷酸多孔,读取长度和误差率,映射到基因组参考的准确性,以及我们在适当的阅读框架中在硅中转换序列的能力。我们开发了一种计算流水线,其对重叠成对结束长(250nt)读取执行纠错,并明确地将读取的读取到与TCR-α和-β链相对应的V和J盒。我们的方法应用于来自健康血液组织的功能性T细胞受体和几种低级胶质瘤(LGG)和胶质母细胞瘤的患者(GBM)。我们使用Shannon熵来测量生产性T细胞曲目中的多样性水平,并且观察到大于50%的TCR多样性可以通过V,J盒式使用来解释。

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