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Long noncoding RNA pncRNA-D reduces cyclin D1 gene expression and arrests cell cycle through RNA m 6 A modification

Journal of Biological Chemistry, ISSN: 0021-9258, Vol: 295, Issue: 17, Page: 5626-5639
2020
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Article Description

pncRNA-D is an irradiation-induced 602-nt long noncoding RNA transcribed from the promoter region of the cyclin D1 ( CCND1 ) gene. CCND1 expression is predicted to be inhibited through an interplay between pncRNA-D and RNA-binding protein TLS/FUS. Because the pncRNA-D –TLS interaction is essential for pncRNA-D –stimulated CCND1 inhibition, here we studied the possible role of RNA modification in this interaction in HeLa cells. We found that osmotic stress induces pncRNA-D by recruiting RNA polymerase II to its promoter. pncRNA-D was highly m 6 A-methylated in control cells, but osmotic stress reduced the methylation and also arginine methylation of TLS in the nucleus. Knockdown of the m 6 A modification enzyme methyltransferase-like 3 (METTL3) prolonged the half-life of pncRNA-D, and among the known m 6 A recognition proteins, YTH domain-containing 1 (YTHDC1) was responsible for binding m 6 A of pncRNA-D. Knockdown of METTL3 or YTHDC1 also enhanced the interaction of pncRNA-D with TLS, and results from RNA pulldown assays implicated YTHDC1 in the inhibitory effect on the TLS– pncRNA-D interaction. CRISPR/Cas9-mediated deletion of candidate m 6 A site decreased the m 6 A level in pncRNA-D and altered its interaction with the RNA-binding proteins. Of note, a reduction in the m 6 A modification arrested the cell cycle at the G 0 /G 1 phase, and pncRNA-D knockdown partially reversed this arrest. Moreover, pncRNA-D induction in HeLa cells significantly suppressed cell growth. Collectively, these findings suggest that m 6 A modification of the long noncoding RNA pncRNA-D plays a role in the regulation of CCND1 gene expression and cell cycle progression.

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