| Literature DB >> 31477927 |
Shigeki Hirabayashi1,2,3, Shruti Bhagat3,4, Yu Matsuki3,5, Yujiro Takegami3,5, Takuya Uehata6,7, Ai Kanemaru5, Masayoshi Itoh8, Kotaro Shirakawa2, Akifumi Takaori-Kondo2, Osamu Takeuchi6,7, Piero Carninci3, Shintaro Katayama4, Yoshihide Hayashizaki8, Juha Kere4,9,10,11, Hideya Kawaji12,13,14, Yasuhiro Murakawa15,16,17,18.
Abstract
Promoters and enhancers are key cis-regulatory elements, but how they operate to generate cell type-specific transcriptomes is not fully understood. We developed a simple and robust method, native elongating transcript-cap analysis of gene expression (NET-CAGE), to sensitively detect 5' ends of nascent RNAs in diverse cells and tissues, including unstable transcripts such as enhancer-derived RNAs. We studied RNA synthesis and degradation at the transcription start site level, characterizing the impact of differential promoter usage on transcript stability. We quantified transcription from cis-regulatory elements without the influence of RNA turnover, and show that enhancer-promoter pairs are generally activated simultaneously on stimulation. By integrating NET-CAGE data with chromatin interaction maps, we show that cis-regulatory elements are topologically connected according to their cell type specificity. We identified new enhancers with high sensitivity, and delineated primary locations of transcription within super-enhancers. Our NET-CAGE dataset derived from human and mouse cells expands the FANTOM5 atlas of transcribed enhancers, with broad applicability to biomedical research.Entities:
Mesh:
Substances:
Year: 2019 PMID: 31477927 DOI: 10.1038/s41588-019-0485-9
Source DB: PubMed Journal: Nat Genet ISSN: 1061-4036 Impact factor: 38.330