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用于下一代测序的单细胞RNA测序文库制备

Preparation of Single-Cell RNA-Seq Libraries for Next Generation Sequencing.

作者信息

Trombetta John J, Gennert David, Lu Diana, Satija Rahul, Shalek Alex K, Regev Aviv

机构信息

Broad Institute of MIT and Harvard, Cambridge, Massachusetts.

Department of Chemistry and Chemical Biology and Department of Physics, Harvard University, Cambridge, Massachusetts.

出版信息

Curr Protoc Mol Biol. 2014 Jul 1;107:4.22.1-4.22.17. doi: 10.1002/0471142727.mb0422s107.

Abstract

For the past several decades, due to technical limitations, the field of transcriptomics has focused on population-level measurements that can mask significant differences between individual cells. With the advent of single-cell RNA-Seq, it is now possible to profile the responses of individual cells at unprecedented depth and thereby uncover, transcriptome-wide, the heterogeneity that exists within these populations. This unit describes a method that merges several important technologies to produce, in high-throughput, single-cell RNA-Seq libraries. Complementary DNA (cDNA) is made from full-length mRNA transcripts using a reverse transcriptase that has terminal transferase activity. This, when combined with a second "template-switch" primer, allows for cDNAs to be constructed that have two universal priming sequences. Following preamplification from these common sequences, Nextera XT is used to prepare a pool of 96 uniquely indexed samples ready for Illumina sequencing.

摘要

在过去几十年里,由于技术限制,转录组学领域一直专注于群体水平的测量,而这些测量可能会掩盖单个细胞之间的显著差异。随着单细胞RNA测序技术的出现,现在能够以前所未有的深度分析单个细胞的反应,从而在转录组范围内揭示这些细胞群体中存在的异质性。本单元介绍了一种融合多种重要技术的方法,可高通量生成单细胞RNA测序文库。使用具有末端转移酶活性的逆转录酶,从全长mRNA转录本合成互补DNA(cDNA)。这与第二种“模板转换”引物相结合,使得构建出的cDNA具有两个通用引物序列。从这些共同序列进行预扩增后,使用Nextera XT制备一组96个具有唯一索引的样本,准备用于Illumina测序。

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