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easyCLIP analysis of RNA-protein interactions incorporating absolute quantification

Douglas F. Porter, Weili Miao, Yang Xue, Grant A. Goda, Andrew L. Ji, Laura K. Donohue, Maria M. Aleman, Daniel Domínguez, Paul A. Khavari

2021Nature Communications55 citationsDOIOpen Access PDF

Abstract

Quantitative criteria to identify proteins as RNA-binding proteins (RBPs) are presently lacking, as are criteria to define RBP target RNAs. Here, we develop an ultraviolet (UV) cross-linking immunoprecipitation (CLIP)-sequencing method, easyCLIP. easyCLIP provides absolute cross-link rates, as well as increased simplicity, efficiency, and capacity to visualize RNA libraries during sequencing library preparation. Measurement of >200 independent cross-link experiments across >35 proteins identifies an RNA cross-link rate threshold that distinguishes RBPs from non-RBPs and defines target RNAs as those with a complex frequency unlikely for a random protein. We apply easyCLIP to the 33 most recurrent cancer mutations across 28 RBPs, finding increased RNA binding per RBP molecule for KHDRBS2 R168C, A1CF E34K and PCBP1 L100P/Q cancer mutations. Quantitating RBP-RNA interactions can thus nominate proteins as RBPs and define the impact of specific disease-associated RBP mutations on RNA association.

Topics & Concepts

Computational biologyRNABiologyGeneticsGeneRNA and protein synthesis mechanismsRNA Research and SplicingRNA modifications and cancer
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