A plant tethering system for the functional study of protein-RNA interactions in vivo

The sorting of RNA transcripts dictates their ultimate post-transcriptional fates, such as translation, decay or degradation by RNA interference (RNAi). This sorting of RNAs into distinct fates is mediated by their interaction with RNA-binding proteins. While hundreds of RNA binding proteins have been identified, which act to sort RNAs into different pathways is largely unknown. Particularly in plants, this is due to the lack of reliable protein-RNA artificial tethering tools necessary to determine the mechanism of protein action on an RNA in vivo. Here we generated a protein-RNA tethering system which functions on an endogenous Arabidopsis RNA that is tracked by the quantitative flowering time phenotype. Unlike other protein-RNA tethering systems that have been attempted in plants, our system circumvents the inadvertent triggering of RNAi. We successfully in vivo tethered a protein epitope, deadenylase protein and translation factor to the target RNA, which function to tag, decay and boost protein production, respectively. We demonstrated that our tethering system (1) is sufficient to engineer the downstream fate of an RNA, (2) enables the determination of any protein's function upon recruitment to an RNA, and (3) can be used to discover new interactions with RNA-binding proteins.

Automated summary

The sorting of RNA transcripts into different fates is mediated by their interaction with RNA-binding proteins, but the mechanism by which hundreds of RNA-binding proteins sort RNAs into distinct pathways is largely unknown. In this study, the researchers developed a protein-RNA tethering system that can be used in plants to engineer the fate of RNAs, determine the function of proteins when recruited to an RNA, and discover new interactions with RNA-binding proteins.