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Characterization of a caspase-3-substrate kinome using an N- and C-terminally tagged protein kinase library produced by a cell-free system

机译:使用无细胞系统产生的N和C末端标记的蛋白激酶文库表征caspase-3底物的激酶组

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摘要

Caspase-3 (CASP3) cleaves many proteins including protein kinases (PKs). Understanding the relationship(s) between CASP3 and its PK substrates is necessary to delineate the apoptosis signaling cascades that are controlled by CASP3 activity. We report herein the characterization of a CASP3-substrate kinome using a simple cell-free system to synthesize a library that contained 304 PKs tagged at their N- and C-termini (NCtagged PKs) and a luminescence assay to report CASP3 cleavage events. Forty-three PKs, including 30 newly identified PKs, were found to be CASP3 substrates, and 28 cleavage sites in 23 PKs were determined. Interestingly, 16 out of the 23 PKs have cleavage sites within 60 residues of their N- or C-termini. Furthermore, 29 of the PKs were cleaved in apoptotic cells, including five that were cleaved near their termini in vitro. In total, approximately 14% of the PKs tested were CASP3 substrates, suggesting that CASP3 cleavage of PKs may be a signature event in apoptotic-signaling cascades. This proteolytic assay method would identify other protease substrates.
机译:Caspase-3(CASP3)裂解包括蛋白质激酶(PKs)在内的许多蛋白质。了解CASP3及其PK底物之间的关系对于描述受CASP3活性控制的凋亡信号级联反应是必不可少的。我们在这里报告使用简单的无细胞系统合成一个文库,该文库包含在其N和C末端标记的304个PK(NCtagged PKs)和一个发光测定法来报告CASP3裂解事件,从而表征CASP3底物的基因组。发现43个PK(包括30个新发现的PK)是CASP3底物,并确定了23个PK中的28个切割位点。有趣的是,在23个PK中,有16个在其N或C末端的60个残基内具有切割位点。此外,在凋亡细胞中裂解了29种PK,其中5种在体外在其末端附近裂解。总共,大约14%的PKs是CASP3底物,这表明PKs的CASP3裂解可能是凋亡信号级联反应中的一个标志性事件。这种蛋白水解测定方法将鉴定其他蛋白酶底物。

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