A New Method for Stranded Whole Transcriptome RNA-seq

Miller, David F. B.; Yan, Pearlly S.; Buechlein, Aaron; Rodriguez, Benjamin A.; Yilmaz, Ayse S.; Goel, Shokhi; Lin, Hai; Collins-Burow, Bridgette; Rhodes, Lyndsay V.; Braun, Chris; Pradeep, Sunila; Rupaimoole, Rajesha; Dalkilic, Mehmet; Sood, Anil K.; Burow, Matthew E.; Tang, Haixu; Huang, Tim H.; Liu, Yunlong; Rusch, Douglas B.; Nephew, Kenneth P.

A New Method for Stranded Whole Transcriptome RNA-seq

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Miller2013New-AAM.pdf (1.75 MB)

Date

2013

Language

American English

Department

Cellular and Integrative Physiology, School of Medicine

Found At

Elsevier

Abstract

This report describes an improved protocol to generate stranded, barcoded RNA-seq libraries to capture the whole transcriptome. By optimizing the use of duplex specific nuclease (DSN) to remove ribosomal RNA reads from stranded barcoded libraries, we demonstrate improved efficiency of multiplexed next generation sequencing (NGS). This approach detects expression profiles of all RNA types, including miRNA (microRNA), piRNA (Piwi-interacting RNA), snoRNA (small nucleolar RNA), lincRNA (long non-coding RNA), mtRNA (mitochondrial RNA) and mRNA (messenger RNA) without the use of gel electrophoresis. The improved protocol generates high quality data that can be used to identify differential expression in known and novel coding and non-coding transcripts, splice variants, mitochondrial genes and SNPs (single nucleotide polymorphisms).

Keywords

Duplex-specific nuclease, Gene expression, Transcriptome, Duplex-specific nuclease, Fragmented LgRNA

Cite As

Miller DF, Yan PS, Buechlein A, et al. A new method for stranded whole transcriptome RNA-seq. Methods. 2013;63(2):126-134. doi:10.1016/j.ymeth.2013.03.023

Journal

Methods

Rights

Publisher Policy

Source

PMC

Type

Article

Permanent Link

https://hdl.handle.net/1805/47976

DOI

https://doi.org/10.1016/j.ymeth.2013.03.023

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Author's manuscript

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