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首页> 外文期刊>Molecular cell >Dynamics of PARKIN-Dependent Mitochondrial Ubiquitylation in Induced Neurons and Model Systems Revealed by Digital Snapshot Proteomics
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Dynamics of PARKIN-Dependent Mitochondrial Ubiquitylation in Induced Neurons and Model Systems Revealed by Digital Snapshot Proteomics

机译:诱导神经元诱导神经元和模型系统中Parkin依赖性线粒体的动态和数字快照蛋白质组学

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摘要

Flux through kinase and ubiquitin-driven signaling systems depends on the modification kinetics, stoichiometry, primary site specificity, and target abundance within the pathway, yet we rarely understand these parameters and their spatial organization within cells. Here we develop temporal digital snapshots of ubiquitin signaling on the mitochondrial outer membrane in embryonic stem cell-derived neurons, and we model HeLa cell systems upon activation of the PINK1 kinase and PARKIN ubiquitin ligase by proteomic counting of ubiquitylation and phosphorylation events. We define the kinetics and site specificity of PARKIN-dependent target ubiquitylation, and we demonstrate the power of this approach to quantify pathway modulators and to mechanistically define the role of PARKIN UBL phosphorylation in pathway activation in induced neurons. Finally, through modulation of pS65-Ub on mitochondria, we demonstrate that Ub hyper-phosphorylation is?inhibitory to mitophagy receptor recruitment, indicating that pS65-Ub stoichiometryin?vivois optimized to coordinate PARKIN recruitment via pS65-Ub and mitophagy receptors via unphosphorylated chains.
机译:通过激酶和泛素驱动的信号传导系统的通量取决于途径内的改性动力学,化学计量,原始位点特异性和目标丰度,但我们很少了解细胞内的这些参数及其空间组织。在这里,我们在胚胎干细胞衍生的神经元的线粒体外膜上开发泛素信号传导的时间数字快照,并在通过蛋白质组计数和磷酸化事件的蛋白质组计数激活Pink1激酶和Parkin泛素连接酶时,我们模拟Hela细胞系统。我们定义了Parkin依赖性目标泛力的动力学和场地特异性,我们证明了这种方法的功率来量化途径调节剂,并机械地定义Parkin Ubl磷酸化在诱导神经元中途径激活中的作用。最后,通过调节线粒体上的PS65-UB,我们证明了UB超磷酸化是α抑制对MICOCHAGY受体募集的,表明PS65-UB的化学计量素ααα,vivois通过不磷酸化的链通过PS65-UB和MITOCHAGY受体进行了优化。

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