Revised iCLIP-seq Protocol for Profiling RNA-protein Interaction Sites at Individual Nucleotide Resolution in Living Cells

被引:2
作者
Nabeel-Shah, Syed [1 ,2 ]
Greenblatt, Jack F. [1 ,2 ]
机构
[1] Univ Toronto, Dept Mol Genet, Toronto M5S IA8, ON, Canada
[2] Univ Toronto, Donnelly Ctr, Toronto M5S 3E1, ON, Canada
基金
加拿大健康研究院;
关键词
iCLIP; eCLIP; Posttranscriptional regulation; RNA-binding proteins; UV crosslinking; NETWORKS; REVEALS; CLIP;
D O I
10.21769/BioProtoc.4688
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Individual nucleotide resolution UV cross-linking and immunoprecipitation followed by high-throughput sequencing (iCLIP-seq) is a powerful technique that is used to identify RNA-binding proteins' (RBP) binding sites on target RNAs and to characterize the molecular basis of posttranscriptional regulatory pathways. Several variants of CLIP have been developed to improve its efficiency and simplify the protocol [e.g., iCLIP2 and enhanced CLIP (eCLIP)]. We have recently reported that transcription factor SP1 functions in the regulation of alternative cleavage and polyadenylation through direct RNA binding. We utilized a modified iCLIP method to identify RNA-binding sites for SP1 and several of the cleavage and polyadenylation complex subunits, including CFIm25, CPSF7, CPSF100, CPSF2, and Fip1. Our revised protocol takes advantage of several features of the eCLIP procedure and also improves on certain steps of the original iCLIP method, including optimization of circularization of cDNA. Herein, we describe a step-by-step procedure for our revised iCLIP-seq protocol, that we designate as iCLIP-1.5, and provide alternative approaches for certain difficult-to-CLIP proteins.
引用
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页数:21
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