Profiling of RNA editing events in plant organellar transcriptomes with high‐throughput sequencing

Abstract

SUMMARYRNA editing is a crucial post‐transcriptional modification process in plant organellar RNA metabolism. rRNA removal‐based total RNA‐seq is one of the most common methods to study this event. However, the lack of commercial kits to remove rRNAs limits the usage of this method, especially for non‐model plant species. DSN‐seq is a transcriptome sequencing method utilizing duplex‐specific nuclease (DSN) to degrade highly abundant cDNA species especially those from rRNAs while keeping the robustness of transcript levels of the majority of other mRNAs, and has not been applied to study RNA editing in plants before. In this study, we evaluated the capability of DSN‐seq to reduce rRNA content and profile organellar RNA editing events in plants, as well we used commercial Ribo‐off‐seq and standard mRNA‐seq as comparisons. Our results demonstrated that DSN‐seq efficiently reduced rRNA content and enriched organellar transcriptomes in rice. With high sensitivity to RNA editing events, DSN‐seq and Ribo‐off‐seq provided a more complete and accurate RNA editing profile of rice, which was further validated by Sanger sequencing. Furthermore, DSN‐seq also demonstrated efficient organellar transcriptome enrichment and high sensitivity for profiling RNA editing events in Arabidopsis thaliana. Our study highlights the capability of rRNA removal‐based total RNA‐seq for profiling RNA editing events in plant organellar transcriptomes and also suggests DSN‐seq as a widely accessible RNA editing profiling method for various plant species.