CtIP-mediated alternative mRNA splicing fine-tunes the DNA damage response

被引:5
作者
Prados-Carvajal, Rosario [1 ,2 ,3 ,4 ]
Rodriguez-Real, Guillermo [1 ,2 ]
Gutierrez-Pozo, Gabriel [1 ]
Huertas, Pablo [1 ,2 ]
机构
[1] Univ Seville, Dept Genet, Seville 41080, Spain
[2] Univ Pablo de Olavide, Univ Sevilla, CSIC, Ctr Andaluz Biol Mol & Med Regenerat CABIMER, Seville 41092, Spain
[3] AstraZeneca, DDR Biol, Biosci, Cambridge, England
[4] AstraZeneca, Oncol R&D, Cambridge, England
关键词
CtIP; SF3B complex; PIF1; DNA damage response; mRNA splicing;
D O I
10.1261/rna.078519.120
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
In order to survive to the exposure of DNA damaging agents, cells activate a complex response that coordinates the cellular metabolism, cell cycle progression, and DNA repair. Among many other events, recent evidence has described global changes in mRNA splicing in cells treated with genotoxic agents. Here, we explore further this DNA damage-dependent alternative splicing. Indeed, we show that both the splicing factor SF3B2 and the repair protein CtIP contribute to the global pattern of splicing both in cells treated or not to DNA damaging agents. Additionally, we focus on a specific DNA damage- and CtIP-dependent alternative splicing event of the helicase PIF1 and explore its relevance for the survival of cells upon exposure to ionizing radiation. Indeed, we describe how the nuclear, active form of PIF1 is substituted by a splicing variant, named vPIF1, in a fashion that requires both the presence of DNA damage and CtIP. Interestingly, timely expression of vPIF1 is required for optimal survival to exposure to DNA damaging agents, but early expression of this isoform delays early events of the DNA damage response. On the contrary, expression of the full length PIF1 facilitates those early events but increases the sensitivity to DNA damaging agents if the expression is maintained long-term.
引用
收藏
页码:303 / 323
页数:21
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