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Literature DB >> 23973811

Use of Bru-Seq and BruChase-Seq for genome-wide assessment of the synthesis and stability of RNA.

Michelle T Paulsen¹, Artur Veloso², Jayendra Prasad¹, Karan Bedi³, Emily A Ljungman¹, Brian Magnuson¹, Thomas E Wilson⁴, Mats Ljungman⁵.

Abstract

Gene expression studies commonly examine total cellular RNA, which only provides information about its steady-state pool of RNA. It remains unclear whether differences in the steady-state reflects variable rates of transcription or RNA degradation. To specifically monitor RNA synthesis and degradation genome-wide, we developed Bru-Seq and BruChase-Seq. These assays are based on metabolic pulse-chase labeling of RNA using bromouridine (Bru). In Bru-Seq, recently labeled RNAs are sequenced to reveal spans of nascent transcription in the genome. In BruChase-Seq, cells are chased in uridine for different periods of time following Bru-labeling, allowing for the isolation of RNA populations of specific ages. Here we describe these methodologies in detail and highlight their usefulness in assessing RNA synthesis and stability as well as splicing kinetics with examples of specific genes from different human cell lines.

Entities: CellLine Chemical Disease Gene Mutation Species

Keywords: RNA splicing; RNA stability; Transcription

Mesh：

Substances：

Year: 2013 PMID： 23973811 PMCID： PMC4009065 DOI： 10.1016/j.ymeth.2013.08.015

Source DB: PubMed Journal: Methods ISSN： 1046-2023 Impact factor: 3.608

28 in total

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