Transcriptome-Wide Profiling of RNA Stability

Nina Fasching, Jan Petržílek, Niko Popitsch, Veronika A Herzog, Stefan L Ameres

Publications: Contribution to bookChapter

Abstract

Gene expression is controlled at multiple levels, including RNA transcription and turnover. But determining the relative contributions of RNA biogenesis and decay to the steady-state abundance of cellular transcripts remains challenging because conventional transcriptomics approaches do not provide the temporal resolution to derive the kinetic parameters underlying steady-state gene expression.Here, we describe a protocol that combines metabolic RNA labeling by 4-thiouridine with chemical nucleoside conversion and whole-transcriptome sequencing followed by bioinformatics analysis to determine RNA stability in cultured cells at a genomic scale. Time-resolved transcriptomics by thiol (SH)-linked alkylation for the metabolic sequencing of RNA (SLAMseq) provides accurate information on transcript half-lives across annotated features in the genome, including by-products of transcription, such as introns. We provide a step-by-step instruction for time-resolved transcriptomics, which enhances traditional RNA sequencing protocols to acquire the temporal resolution required to directly measure the cellular kinetics of RNA turnover under physiological conditions.

Original languageEnglish
Title of host publicationPost-Transcriptional Gene Regulation
Place of PublicationNew York
Pages311-330
Number of pages20
Volume2404
Edition3
ISBN (Electronic)978-1-0716-1851-6
DOIs
Publication statusPublished - 2022

Publication series

SeriesMethods in Molecular Biology
ISSN1064-3745

Austrian Fields of Science 2012

  • 106023 Molecular biology

Keywords

  • Gene Expression Profiling
  • RNA/genetics
  • RNA Stability
  • Sequence Analysis, RNA
  • Thiouridine
  • Transcriptome
  • 4-Thiouridine
  • RNA stability
  • SLAMseq
  • Gene regulation
  • Metabolic RNA sequencing

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