easyCLIP analysis of RNA-protein interactions incorporating absolute quantification

结合绝对定量的 RNA-蛋白质相互作用 easyCLIP 分析

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作者:Douglas F Porter, Weili Miao, Xue Yang, Grant A Goda, Andrew L Ji, Laura K H Donohue, Maria M Aleman, Daniel Dominguez, Paul A Khavari
期刊:Nature Communications影响因子:14.700
时间:2021起止号:2021 Mar 10;12(1):1569.
doi:10.1038/s41467-021-21623-4方法学: IP、WB
靶点: Fibrillarin研究方向: 信号转导

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.

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