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Digital gene expression analysis with sample multiplexing and PCR duplicate detection: A straightforward protocol

Authors :
Andrey Rozenberg
Florian Leese
Linda C. Weiss
Ralph Tollrian
Source :
BioTechniques, Vol 61, Iss 1, Pp 26-32 (2016)
Publication Year :
2016
Publisher :
Taylor & Francis Group, 2016.

Abstract

Tag-Seq is a high-throughput approach used for discovering SNPs and characterizing gene expression. In comparison to RNA-Seq, Tag-Seq eases data processing and allows detection of rare mRNA species using only one tag per transcript molecule. However, reduced library complexity raises the issue of PCR duplicates, which distort gene expression levels. Here we present a novel Tag-Seq protocol that uses the least biased methods for RNA library preparation combined with a novel approach for joint PCR template and sample labeling. In our protocol, input RNA is fragmented by hydrolysis, and poly(A)-bearing RNAs are selected and directly ligated to mixed DNA—RNA P5 adapters. The P5 adapters contain i5 barcodes composed of sample-specific (moderately) degenerate base regions (mDBRs), which later allow detection of PCR duplicates. The P7 adapter is attached via reverse transcription with individual i7 barcodes added during the amplification step. The resulting libraries can be sequenced on an Illumina sequencer. After sample demultiplexing and PCR duplicate removal with a free software tool we designed, the data are ready for downstream analysis. Our protocol was tested on RNA samples from predator-induced and control Daphnia microcrustaceans.

Details

Language :
English
ISSN :
19409818 and 07366205
Volume :
61
Issue :
1
Database :
Directory of Open Access Journals
Journal :
BioTechniques
Publication Type :
Academic Journal
Accession number :
edsdoj.7a53c012ac03459096a8f1b2f080c138
Document Type :
article
Full Text :
https://doi.org/10.2144/000114434