哺乳动物新生RNA的长读测序制备

Q2 Biochemistry, Genetics and Molecular Biology

Current Protocols in Molecular Biology Pub Date : 2020-10-21 DOI:10.1002/cpmb.128

Kirsten A. Reimer, Karla M. Neugebauer

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引用次数: 3

摘要

长读测序技术现在允许对数百到数千个核苷酸长的rna(或它们的cdna)进行高质量的测序。新生RNA的长读序列提供了共转录RNA加工事件的单核苷酸分辨率信息。拼接、折叠和碱基修饰。在这里，我们描述了如何通过染色质相关RNA的亚细胞分离从哺乳动物细胞中分离新生RNA，以及如何耗尽poly(A)+ RNA和rRNA，最后，如何生成全长cDNA文库用于长读测序平台。这种方法通过揭示剪接模式或其他传统短读RNA测序无法获得的RNA加工事件，可以了解跨多内含子转录本的协调剪接状态。©2020 Wiley期刊有限公司基本协议1:亚细胞分离基本协议2:新生RNA分离和适配器连接基本协议3:cDNA扩增子制备

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Preparation of Mammalian Nascent RNA for Long Read Sequencing

Long read sequencing technologies now allow high-quality sequencing of RNAs (or their cDNAs) that are hundreds to thousands of nucleotides long. Long read sequences of nascent RNA provide single-nucleotide-resolution information about co-transcriptional RNA processing events—e.g., splicing, folding, and base modifications. Here, we describe how to isolate nascent RNA from mammalian cells through subcellular fractionation of chromatin-associated RNA, as well as how to deplete poly(A)⁺ RNA and rRNA, and, finally, how to generate a full-length cDNA library for use on long read sequencing platforms. This approach allows for an understanding of coordinated splicing status across multi-intron transcripts by revealing patterns of splicing or other RNA processing events that cannot be gained from traditional short read RNA sequencing. © 2020 Wiley Periodicals LLC.

Basic Protocol 1: Subcellular fractionation

Basic Protocol 2: Nascent RNA isolation and adapter ligation

Basic Protocol 3: cDNA amplicon preparation

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来源期刊

Current Protocols in Molecular Biology Biochemistry, Genetics and Molecular Biology-Molecular Biology

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