期刊
ANNUAL REVIEW OF GENETICS, VOL 50
卷 50, 期 -, 页码 235-266出版社
ANNUAL REVIEWS
DOI: 10.1146/annurev-genet-120215-035034
关键词
DMS-seq; genome-wide; in vivo RNA folding; RNA structurome; SHAPE; Structure-seq
资金
- Direct For Biological Sciences [1339282] Funding Source: National Science Foundation
Single-stranded RNA molecules fold into extraordinarily complicated secondary and tertiary structures as a result of intramolecular base pairing. In vivo, these RNA structures are not static. Instead, they are remodeled in response to changes in the prevailing physicochemical environment of the cell and as a result of intermolecular base pairing and interactions with RNA binding proteins. Remarkable technical advances now allow us to probe RNA secondary structure at single-nucleotide resolution and genome-wide, both in vitro and in vivo. These data sets provide new glimpses into the RNA universe. Analyses of RNA structuromes in HIV, yeast, Arabidopsis, and mammalian cells and tissues have revealed regulatory effects of RNA structure on messenger RNA (mRNA) polyadenylation, splicing, translation, and turnover. Application of new methods for genome-wide identification of mRNA modifications, particularly methylation and pseudouridylation, has shown that the RNA epitranscriptome both influences and is influenced by RNA structure. In this review, we describe newly developed genome-wide RNA structure-probing methods and synthesize the information emerging from their application.
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