Massively parallel dissection of RNA in RNA–protein interactions in vivo

Author:

Lee Yu Hsuan1ORCID,Hass Evan P2,Campodonico Will2,Lee Yong Kyu1,Lasda Erika2,Shah Jaynish S2,Rinn John L2,Hwang Taeyoung134ORCID

Affiliation:

1. Lieber Institute for Brain Development, Johns Hopkins Medical Campus , Baltimore , MD 21205 , USA

2. Department of Biochemistry and BioFrontiers Institute, University of Colorado , Boulder , CO 80309 , USA

3. Department of Neurology, Johns Hopkins University School of Medicine , Baltimore , MD 21205 , USA

4. Solomon H. Snyder Department of Neuroscience, Johns Hopkins University School of Medicine , Baltimore , MD 21205 , USA

Abstract

Abstract Many of the biological functions performed by RNA are mediated by RNA-binding proteins (RBPs), and understanding the molecular basis of these interactions is fundamental to biology. Here, we present massively parallel RNA assay combined with immunoprecipitation (MPRNA-IP) for in vivo high-throughput dissection of RNA–protein interactions and describe statistical models for identifying RNA domains and parsing the structural contributions of RNA. By using custom pools of tens of thousands of RNA sequences containing systematically designed truncations and mutations, MPRNA-IP is able to identify RNA domains, sequences, and secondary structures necessary and sufficient for protein binding in a single experiment. We show that this approach is successful for multiple RNAs of interest, including the long noncoding RNA NORAD, bacteriophage MS2 RNA, and human telomerase RNA, and we use it to interrogate the hitherto unknown sequence or structural RNA-binding preferences of the DNA-looping factor CTCF. By integrating systematic mutation analysis with crosslinking immunoprecipitation, MPRNA-IP provides a novel high-throughput way to elucidate RNA-based mechanisms behind RNA–protein interactions in vivo.

Funder

NIH

NIGMS

Publisher

Oxford University Press (OUP)

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