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凋亡小体形成与凋亡执行的系统生物学分析支持别构半胱天冬酶-9激活。

A systems biology analysis of apoptosome formation and apoptosis execution supports allosteric procaspase-9 activation.

作者信息

Würstle Maximilian L, Rehm Markus

机构信息

Department of Physiology and Medical Physics, Royal College of Surgeons in Ireland, Dublin 2, Ireland; Centre for Systems Medicine, Royal College of Surgeons in Ireland, Dublin 2, Ireland.

Department of Physiology and Medical Physics, Royal College of Surgeons in Ireland, Dublin 2, Ireland; Centre for Systems Medicine, Royal College of Surgeons in Ireland, Dublin 2, Ireland.

出版信息

J Biol Chem. 2014 Sep 19;289(38):26277-26289. doi: 10.1074/jbc.M114.590034. Epub 2014 Aug 8.

Abstract

The protease caspase-9 is activated on the apoptosome, a multiprotein signal transduction platform that assembles in response to mitochondria-dependent apoptosis initiation. Despite extensive molecular research, the assembly of the holo-apoptosome and the process of caspase-9 activation remain incompletely understood. Here, we therefore integrated quantitative data on the molecular interactions and proteolytic processes during apoptosome formation and apoptosis execution and conducted mathematical simulations to investigate the resulting biochemical signaling, quantitatively and kinetically. Interestingly, when implementing the homodimerization of procaspase-9 as a prerequisite for activation, the calculated kinetics of apoptosis execution and the efficacy of caspase-3 activation failed to replicate experimental data. In contrast, assuming a scenario in which procaspase-9 is activated allosterically upon binding to the apoptosome backbone, the mathematical simulations quantitatively and kinetically reproduced all experimental data. These data included a XIAP threshold concentration at which apoptosis execution is suppressed in HeLa cervical cancer cells, half-times of procaspase-9 processing, as well as the molecular timer function of the apoptosome. Our study therefore provides novel mechanistic insight into apoptosome-dependent apoptosis execution and suggests that caspase-9 is activated allosterically by binding to the apoptosome backbone. Our findings challenge the currently prevailing dogma that all initiator procaspases require homodimerization for activation.

摘要

蛋白酶caspase-9在凋亡小体上被激活,凋亡小体是一种多蛋白信号转导平台,它在响应线粒体依赖性凋亡启动时组装而成。尽管进行了广泛的分子研究,但全凋亡小体的组装和caspase-9的激活过程仍未完全了解。因此,在这里我们整合了凋亡小体形成和凋亡执行过程中分子相互作用和蛋白水解过程的定量数据,并进行了数学模拟,以从定量和动力学角度研究由此产生的生化信号。有趣的是,当将procaspase-9的同二聚化作为激活的先决条件时,计算出的凋亡执行动力学和caspase-3激活的效率无法复制实验数据。相反,假设procaspase-9在与凋亡小体骨架结合后被变构激活的情况,数学模拟在定量和动力学上重现了所有实验数据。这些数据包括在HeLa宫颈癌细胞中抑制凋亡执行的XIAP阈值浓度、procaspase-9加工的半衰期以及凋亡小体的分子定时器功能。因此,我们的研究为凋亡小体依赖性凋亡执行提供了新的机制见解,并表明caspase-9通过与凋亡小体骨架结合而被变构激活。我们的发现挑战了目前流行的教条,即所有起始procaspase都需要同二聚化才能激活。

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