Non-coding RNA profiling by high throughput sequencing Expression profiling by high throughput sequencing
Summary
Many microRNAs (miRNAs) exist alongside abundant miRNA isoforms (isomiRs), most of which arise from post-maturation sequence modifications, such as 3’ uridylation. However, the ways in which these sequence modifications affect miRNA function remain poorly understood. Here, using human miR-27a in cell lines as a model, we have discovered that a nonfunctional target site unable to base pair extensively with the miRNA seed sequence can regain function when an upstream adenosine is able to base-pair with a post-transcriptionally added uridine in the miR-27a tail. This Tail-U-Mediated Repression (TUMR) is abolished in cells lacking the uridylation enzymes TUT4 and TUT7, indicating that uridylation alters miRNA function by modulating target recognition. We identified a set of non-canonical targets in human cells that are specifically regulated by uridylated miR-27a. We provide evidence that TUMR expands the targets of other endogenous miRNAs. Our study reveals a function for uridylated isomiRs in regulating non-canonical miRNA targets.
Overall design
HEK293T cells and TUT4/7 Double Knockout (DKO) cells with or without ectopic expression of miR-27a or specific depletion of miR-148b were subjected to miRNA-Seq and isomiR profile analyses. In parallel, mRNA profiles were measured by RNA-seq to monitor miR-27a and miR-148b mediated repressions.