Abstract

BackgroundRNA editing is a co/posttranscriptional modification mechanism that increases the diversity of transcripts, with potential functional consequences. The advent of next-generation sequencing technologies has enabled the identification of RNA edits at unprecedented throughput and resolution. However, our knowledge of RNA editing in swine is still limited.ResultsHere, we utilized RES-Scanner to identify RNA editing sites in the brain, subcutaneous fat, heart, liver, muscle, lung and ovary in three 180-day-old Large White gilts based on matched strand-specific RNA sequencing and whole-genome resequencing datasets. In total, we identified 74863 editing sites, and 92.1% of these sites caused adenosine-to-guanosine (A-to-G) conversion. Most A-to-G sites were located in noncoding regions and generally had low editing levels. In total, 151 A-to-G sites were detected in coding regions (CDS), including 94 sites that could lead to nonsynonymous amino acid changes. We provide further evidence supporting a previous observation that pig transcriptomes are highly editable at PRE-1 elements. The number of A-to-G editing sites ranged from 4155 (muscle) to 25001 (brain) across the seven tissues. The expression levels of the ADAR enzymes could explain some but not all of this variation across tissues. The functional analysis of the genes with tissue-specific editing sites in each tissue revealed that RNA editing might play important roles in tissue function. Specifically, more pathways showed significant enrichment in the fat and liver than in other tissues, while no pathway was enriched in the muscle.ConclusionsThis study identified a total of 74863 nonredundant RNA editing sites in seven tissues and revealed the potential importance of RNA editing in tissue function. Our findings largely extend the porcine editome and enhance our understanding of RNA editing in swine.

Highlights

  • RNA editing is a co/posttranscriptional modification mechanism that increases the diversity of transcripts, with potential functional consequences

  • Our study largely extends the list of RNA editing sites in swine and provides deeper insight into the characteristics of the pig editome

  • To fully utilize our sequencing data, the possible RNA editing events were detected with RES-Scanner, which requires matched RNA sequencing (RNA-seq) and DNA-seq data to rule out genomic single nucleotide variants and automatically separates the plus-strand alignments from the minus-strand alignments for the strand-specific RNA-seq libraries to identify the correct genomic loci of origin

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Summary

Introduction

RNA editing is a co/posttranscriptional modification mechanism that increases the diversity of transcripts, with potential functional consequences. The advent of next-generation sequencing technologies has enabled the identification of RNA edits at unprecedented throughput and resolution. The identification of RNA editing sites heavily depends on sequencing technologies. The advent of next-generation sequencing (NGS) technologies has enabled the identification of transcriptome-wide RNA editing events across individuals and tissues at unprecedented throughput and resolution. RNA editing studies involving pigs can promote an understanding of the molecular basis of human diseases. To the best of our knowledge, only one research study, which identified 5294 nonredundant A-to-G sites across three tissues from one pig, has provided information about RNA editing at a transcriptome-wide level in pigs [22]. Our knowledge of RNA editing in pigs is very limited compared to that in humans and other model species

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