CSIG Inhibits PTEN Translation in Replicative Senescence

Author:

Ma Liwei1,Chang Na1,Guo Shuzhen1,Li Qian1,Zhang Zongyu1,Wang Wengong1,Tong Tanjun1

Affiliation:

1. Research Center on Aging, Department of Biochemistry and Molecular Biology, Peking University Health Science Center, 38 Xueyuan Road, Beijing 100083, People's Republic of China

Abstract

ABSTRACT Using a suppressive subtractive hybridization system, we identified CSIG (cellular senescence-inhibited gene protein; RSL1D1) that was abundant in young human diploid fibroblast cells but declined upon replicative senescence. Overexpression or knockdown of CSIG did not influence p21 Cip1 and p16 INK4a expressions. Instead, CSIG negatively regulated PTEN and p27 Kip1 expressions, in turn promoting cell proliferation. In PTEN-silenced HEK 293 cells and PTEN-deficient human glioblastoma U87MG cells, the effect of CSIG on p27 Kip1 expression and cell division was abolished, suggesting that PTEN was required for the role of CSIG on p27 Kip1 regulation and cell cycle progression. Investigation into the underlying mechanism revealed that the regulation of PTEN by CSIG was achieved through a translational suppression mechanism. Further study showed that CSIG interacted with PTEN mRNA in the 5′ untranslated region (UTR) and that knockdown of CSIG led to increased luciferase activity of a PTEN 5′ UTR-luciferase reporter. Moreover, overexpression of CSIG significantly delayed the progression of replicative senescence, while knockdown of CSIG expression accelerated replicative senescence. Knockdown of PTEN diminished the effect of CSIG on cellular senescence. Our findings indicate that CSIG acts as a novel regulatory component of replicative senescence, which requires PTEN as a mediator and involves in a translational regulatory mechanism.

Publisher

American Society for Microbiology

Subject

Cell Biology,Molecular Biology

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