Caspase-2 is required for DNA damage-induced expression of the CDK inhibitor p21WAF1/CIP1

被引:0
作者
D Sohn
W Budach
R U Jänicke
机构
[1] Laboratory of Molecular Radiooncology,
[2] Clinic and Policlinic for Radiation Therapy and Radiooncology,undefined
[3] University of Düsseldorf,undefined
[4] Universitätsstrasse 1,undefined
来源
Cell Death & Differentiation | 2011年 / 18卷
关键词
apoptosis; cell cycle; translational control; 3′-UTR; p53; RAIDD;
D O I
暂无
中图分类号
学科分类号
摘要
Although caspase-2 represents the most conserved caspase across species and was the second caspase identified, its precise function remains enigmatic. In several cell types we show that knockdown of caspase-2 specifically impaired DNA damage-induced p21 expression, whereas overexpression of a caspase-2 mutant increased p21 levels. Caspase-2 did not influence p21 mRNA transcription; moreover, various inhibitors targeting proteasomal or non-proteasomal proteases, including caspases, could not restore p21 protein levels following knockdown of caspase-2. As, however, silencing of caspase-2 impaired exogenous expression of p21 constructs containing 3′-UTR sequences, our results strongly indicate that caspase-2 regulates p21 expression at the translational level. Intriguingly, unlike depletion of caspase-2, which prevented p21 expression and thereby reverted the γ-IR-induced senescent phenotype of wild-type HCT116 colon carcinoma cells into apoptosis, knockdown of none of the caspase-2-interacting components RAIDD, RIP or DNA-PKcs was able to mimic these processes. Together, our data suggest that this novel role of caspase-2 as a translational regulator of p21 expression occurs not only independently of its enzymatic activity but also does not require known caspase-2-activating platforms.
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页码:1664 / 1674
页数:10
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