Abstract
Long non-coding RNAs (lncRNAs) are components of epigenetic control mechanisms that ensure appropriate and timely gene expression. The functions of lncRNAs are often mediated through associated gene regulatory activities, but how lncRNAs are distinguished from other RNAs and recruit effector complexes is unclear. Here, we utilize the fission yeast Schizosaccharomyces pombe to investigate how lncRNAs engage silencing activities to regulate gene expression in cis. We find that invasion of lncRNA transcription into the downstream gene body incorporates a cryptic intron required for repression of that gene. Our analyses show that lncRNAs containing cryptic introns are targeted by the conserved Pir2ARS2 protein in association with splicing factors, which recruit RNA processing and chromatin-modifying activities involved in gene silencing. Pir2 and splicing machinery are broadly required for gene repression. Our finding that human ARS2 also interacts with splicing factors suggests a conserved mechanism mediates gene repression through cryptic introns within lncRNAs.
Highlights
Long non-coding RNAs are components of epigenetic control mechanisms that ensure appropriate and timely gene expression
We investigated if MTREC and its associated factors, including the Pir2ARS2 protein[6,25], are required for repression of pho[1] and byr[2] by Long non-coding RNAs (lncRNAs)
Our analyses reveal that a cryptic intron within the lncRNA is a crucial element for gene repression via a pathway involving Pir2ARS2 and splicing factors (Fig. 6)
Summary
Long non-coding RNAs (lncRNAs) are components of epigenetic control mechanisms that ensure appropriate and timely gene expression. Mmi[1] mediates recruitment of the cleavage and polyadenylation factor (CPF) complex, which acts together with Rrp[6] to trigger transcription termination and degradation of lncRNAs, preventing them from invading and repressing downstream genes[7,11,12,13,14]. Despite these studies, a major unanswered question is how lncRNAs mediate gene repression
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