从单细胞RNA测序文库中去除核糖体RNA序列

Depletion of Ribosomal RNA Sequences from Single-Cell RNA-Sequencing Library.

作者信息

Fang Nan, Akinci-Tolun Rumeysa

机构信息

QIAGEN GmbH, Hilden, Germany.

出版信息

Curr Protoc Mol Biol. 2016 Jul 1;115:7.27.1-7.27.20. doi: 10.1002/cpmb.11.

Abstract

Recent advances in single-cell RNA sequencing technologies have revealed high heterogeneity of gene expression profiles in individual cells. However, most current single-cell RNA-seq methods use oligo-dT priming in the reverse transcription steps and detect only polyA-positive for more accuracy, since there are also polyA-positive non-coding RNAs transcripts, not other important RNA species, such as polyA-negative noncoding RNA. Reverse transcription using random oligos enables detection of not only the noncoding RNA species without polyA tails, but also ribosomal RNA (rRNA). rRNA comprises more than 90% of the total RNA and should be depleted from the RNA-seq library to ensure efficient usage of the sequencing capacity. Commonly used hybridization-based rRNA depletion methods can preserve noncoding RNA in the standard RNA-seq library. However, such rRNA depletion methods require high input amounts of total RNA and do not work at the single-cell level or with limited input DNA. This unit describes a novel procedure for RNA-seq library construction from single cells or a minimal amount of RNA. A thermostable duplex-specific nuclease is used in this method to effectively remove ribosomal RNA sequences following whole-transcriptome amplification and sequencing library construction. © 2016 by John Wiley & Sons, Inc.

摘要

单细胞RNA测序技术的最新进展揭示了单个细胞中基因表达谱的高度异质性。然而,目前大多数单细胞RNA测序方法在逆转录步骤中使用oligo-dT引物,并且仅检测polyA阳性以提高准确性,因为也存在polyA阳性非编码RNA转录本,而不是其他重要的RNA种类,例如polyA阴性非编码RNA。使用随机寡核苷酸进行逆转录不仅能够检测没有polyA尾巴的非编码RNA种类,还能检测核糖体RNA(rRNA)。rRNA占总RNA的90%以上,应从RNA测序文库中去除,以确保测序能力的有效利用。常用的基于杂交的rRNA去除方法可以在标准RNA测序文库中保留非编码RNA。然而,这种rRNA去除方法需要大量的总RNA输入,并且在单细胞水平或有限的输入DNA情况下不起作用。本单元描述了一种从单细胞或少量RNA构建RNA测序文库的新方法。该方法使用一种热稳定的双链特异性核酸酶,在全转录组扩增和测序文库构建后有效地去除核糖体RNA序列。©2016约翰威立父子公司。

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