首页> 美国卫生研究院文献>Molecular Neurodegeneration >Evidence against roles for phorbol binding protein Munc13-1 ADAM adaptor Eve-1 or vesicle trafficking phosphoproteins Munc18 or NSF as phospho-state-sensitive modulators of phorbol/PKC-activated Alzheimer APP ectodomain shedding
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Evidence against roles for phorbol binding protein Munc13-1 ADAM adaptor Eve-1 or vesicle trafficking phosphoproteins Munc18 or NSF as phospho-state-sensitive modulators of phorbol/PKC-activated Alzheimer APP ectodomain shedding

机译:反对佛波结合蛋白Munc13-1ADAM接头Eve-1或囊泡运输磷蛋白Munc18或NSF作为佛波/ PKC激活的阿尔茨海默病APP胞外域脱落的磷酸化状态敏感调节剂的作用的证据

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摘要

BackgroundShedding of the Alzheimer amyloid precursor protein (APP) ectodomain can be accelerated by phorbol esters, compounds that act via protein kinase C (PKC) or through unconventional phorbol-binding proteins such as Munc13-1. We have previously demonstrated that application of phorbol esters or purified PKC potentiates budding of APP-bearing secretory vesicles at the trans-Golgi network (TGN) and toward the plasma membrane where APP becomes a substrate for enzymes responsible for shedding, known collectively as α-secretase(s). However, molecular identification of the presumptive "phospho-state-sensitive modulators of ectodomain shedding" (PMES) responsible for regulated shedding has been challenging. Here, we examined the effects on APP ectodomain shedding of four phorbol-sensitive proteins involved in regulation of vesicular membrane trafficking of APP: Munc13-1, Munc18, NSF, and Eve-1.
机译:背景佛波酯可通过蛋白激酶C(PKC)或非常规的佛波结合蛋白(例如Munc13-1)起作用,从而加速阿尔茨海默氏淀粉样蛋白前体蛋白(APP)胞外域的脱落。之前我们已经证明,使用佛波酯或纯化的PKC可以增强带有APP的分泌小泡在反面高尔基网络(TGN)处和质膜的萌芽状态,在此质膜上APP成为负责脱落酶的底物,统称为α-分泌酶。但是,负责调节脱落的推测性“胞外域脱落的磷酸状态敏感调节剂”(PMES)的分子鉴定一直具有挑战性。在这里,我们检查了参与调控APP囊泡运输的四种佛波醇敏感蛋白对APP胞外域脱落的影响:Munc13-1,Munc18,NSF和Eve-1。

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