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Photoactivatable ribonucleosides mark base-specific RNA-binding sites

Cited 9 time in Web of Science Cited 9 time in Scopus
Authors

Bae, Jong Woo; Kim, Sangtae; Kim, V. Narry; Kim, Jong-Seo

Issue Date
2021-12
Publisher
Nature Publishing Group
Citation
Nature Communications, Vol.12 No.1, p. 6026
Abstract
RNA-protein interactions play critical roles in post-transcriptional gene regulation. Here the authors demonstrate pRBS-ID, an updated MS/MS-based method that combines the benefits of photoactivatable ribonucleosides and the chemical cleavage of RNA. RNA-protein interaction can be captured by crosslinking and enrichment followed by tandem mass spectrometry, but it remains challenging to pinpoint RNA-binding sites (RBSs) or provide direct evidence for RNA-binding. To overcome these limitations, we here developed pRBS-ID, by incorporating the benefits of UVA-based photoactivatable ribonucleoside (PAR; 4-thiouridine and 6-thioguanosine) crosslinking and chemical RNA cleavage. pRBS-ID robustly detects peptides crosslinked to PAR adducts, offering direct RNA-binding evidence and identifying RBSs at single amino acid-resolution with base-specificity (U or G). Using pRBS-ID, we could profile uridine-contacting RBSs globally and discover guanosine-contacting RBSs, which allowed us to characterize the base-specific interactions. We also applied the search pipeline to analyze the datasets from UVC-based RBS-ID experiments, altogether offering a comprehensive list of human RBSs with high coverage (3,077 RBSs in 532 proteins in total). pRBS-ID is a widely applicable platform to investigate the molecular basis of posttranscriptional regulation.
ISSN
2041-1723
URI
https://hdl.handle.net/10371/178029
DOI
https://doi.org/10.1038/s41467-021-26317-5
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Research Area Molecular Biology & Genetics

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