3′ UTR lengthening as a novel mechanism in regulating cellular senescence

Author:

Chen Meng,Lyu Guoliang,Han Miao,Nie Hongbo,Shen Ting,Chen Wei,Niu Yichi,Song Yifan,Li Xueping,Li Huan,Chen Xinyu,Wang Ziyue,Xia Zheng,Li Wei,Tian Xiao-Li,Ding Chen,Gu Jun,Zheng Yufang,Liu Xinhua,Hu Jinfeng,Wei Gang,Tao Wei,Ni TingORCID

Abstract

Cellular senescence has been viewed as a tumor suppression mechanism and also as a contributor to individual aging. Widespread shortening of 3′ untranslated regions (3′ UTRs) in messenger RNAs (mRNAs) by alternative polyadenylation (APA) has recently been discovered in cancer cells. However, the role of APA in the process of cellular senescence remains elusive. Here, we found that hundreds of genes in senescent cells tended to use distal poly(A) (pA) sites, leading to a global lengthening of 3′ UTRs and reduced gene expression. Genes that harbor longer 3′ UTRs in senescent cells were enriched in senescence-related pathways. Rras2, a member of the Ras superfamily that participates in multiple signal transduction pathways, preferred longer 3′ UTR usage and exhibited decreased expression in senescent cells. Depletion of Rras2 promoted senescence, while rescue of Rras2 reversed senescence-associated phenotypes. Mechanistically, splicing factor TRA2B bound to a core “AGAA” motif located in the alternative 3′ UTR of Rras2, thereby reducing the RRAS2 protein level and causing senescence. Both proximal and distal poly(A) signals showed strong sequence conservation, highlighting the vital role of APA regulation during evolution. Our results revealed APA as a novel mechanism in regulating cellular senescence.

Funder

National Basic Research Program of China

National Natural Science Foundation of China

111 Project of China

Publisher

Cold Spring Harbor Laboratory

Subject

Genetics(clinical),Genetics

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