Development of a DNA barcode tagging method for monitoring dynamic changes in gene expression by using an ultra high-throughput sequencer

Author:

Maeda Norihiro12,Nishiyori Hiromi2,Nakamura Mari2,Kawazu Chika2,Murata Mitsuyoshi2,Sano Hiromi2,Hayashida Kengo2,Fukuda Shiro2,Tagami Michihira2,Hasegawa Akira2,Murakami Kayoko2,Schroder Kate3,Irvine Katharine3,Hume David A.4,Hayashizaki Yoshihide12,Carninci Piero12,Suzuki Harukazu2

Affiliation:

1. Advanced Science Institute, RIKEN Wako Main Campus, Saitama

2. RIKEN Genomic Sciences Center, RIKEN Yokohama Institute, Kanagawa, Japan

3. Institute for Molecular Bioscience, The University of Queensland, Queensland, Australia

4. The Roslin Institute and Royal (Dick) School of Veterinary Studies, University of Edinburgh, Scotland, UK

Abstract

CAGE (cap analysis of gene expression) is a method for identifying transcription start sites by sequencing the first 20 or 21 nucleotides from the 5′ end of capped transcripts, allowing genome-wide promoter analyses to be performed. The potential of the CAGE as a form of expression profiling was limited previously by sequencing technology and the labor-intensive protocol. Here we describe an improved CAGE method for use with a next generation sequencer. This modified method allows the identification of the RNA source of each CAGE tag within a pooled library by introducing DNA tags (barcodes). The method not only drastically improves the sequencing capacity, but also contributes to savings in both time and budget. Additionally, this pooled CAGE tag method enables the dynamic changes in promoter usage and gene expression to be monitored.

Publisher

Future Science Ltd

Subject

General Biochemistry, Genetics and Molecular Biology,Biotechnology

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