AI Article Synopsis
- HITS-CLIP libraries contain RNA fragments bound by RNA binding proteins (RBPs), and these can form chimeric CLIP tags that reveal base pairing details between small RNAs and their targets.
- A recent study on the Drosophila Piwi protein revealed a new mechanism for mRNA entrapment in germ cell granules through chimeric reads.
- The novel method called chimeric CLIP (cCLIP) can help researchers identify chimeric reads and analyze the functions of various RNA-binding proteins, potentially extending to those affecting RNA secondary structures.
Article Abstract
HITS-CLIP (High-Throughput Sequencing after in vivo Crosslinking and Immunoprecipitation, CLIP-Seq) libraries contain fragments of the RNA sequences bound in vivo by an RNA binding protein (RBP). Such fragments, especially if they represent RNA duplexes bound in vivo by the RBP, can occasionally be ligated together to form chimeric CLIP tags. Chimeric CLIP tags from Argonaute CLIP libraries can provide the exact base pairing profiles of small RNAs with their target RNA sequences, thus solving a critical problem in the field of post-transcriptional regulation. We recently reported an analysis of chimeric reads from the Drosophila Piwi protein Aubergine, which revealed a novel mechanism for mRNA entrapment within germ RNP granules. We term this novel approach chimeric CLIP (cCLIP) and present here the main steps that a researcher can take after the acquisition of the deep sequencing data, for the identification of candidate chimeric reads in Piwi CLIP libraries. Extending the scope beyond small-RNA binding proteins, we believe that cCLIP can be utilized to elucidate the in vivo functions of RNA-binding proteins in general, and especially those that modulate RNA secondary structures. We, therefore, also describe aspects of the generalized chimeric read identification problem, which can find use in the analysis of the CLIP libraries of any RNA-binding protein.
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