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在新的囊泡形成之前,多种自噬和细胞质到液泡靶向成分汇聚到液泡周围膜区室。

Convergence of multiple autophagy and cytoplasm to vacuole targeting components to a perivacuolar membrane compartment prior to de novo vesicle formation.

作者信息

Kim John, Huang Wei-Pang, Stromhaug Per E, Klionsky Daniel J

机构信息

Department of Molecular, Cellular, and Developmental Biology, University of Michigan, Ann Arbor, Michigan 48109, USA.

出版信息

J Biol Chem. 2002 Jan 4;277(1):763-73. doi: 10.1074/jbc.M109134200. Epub 2001 Oct 23.

DOI:10.1074/jbc.M109134200
PMID:11675395
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2754695/
Abstract

Under starvation conditions, the majority of intracellular degradation occurs at the lysosome or vacuole by the autophagy pathway. The cytoplasmic substrates destined for degradation are packaged inside unique double-membrane transport vesicles called autophagosomes and are targeted to the lysosome/vacuole for subsequent breakdown and recycling. Genetic analyses of yeast autophagy mutants, apg and aut, have begun to identify the molecular machinery as well as indicate a substantial overlap with the biosynthetic cytoplasm to vacuole targeting (Cvt) pathway. Transport vesicle formation is a key regulatory step of both pathways. In this study, we characterize the putative compartment from which both autophagosomes and the analogous Cvt vesicles may originate. Microscopy analyses identified a perivacuolar membrane as the resident compartment for both the Apg1-Cvt9 signaling complex, which mediates the switching between autophagic and Cvt transport, and the autophagy/Cvt-specific phosphatidylinositol 3-kinase complex. Furthermore, the perivacuolar compartment designates the initial site of membrane binding by the Apg/Cvt vesicle component Aut7, the Cvt cargo receptor Cvt19, and the Apg conjugation machinery, which functions in the de novo formation of vesicles. Biochemical isolation of the vesicle component Aut7 and density gradient analyses recapitulate the microscopy findings although also supporting the paradigm that components required for vesicle formation and packaging concentrate at subdomains within the donor membrane compartment.

摘要

在饥饿条件下,细胞内的大部分降解过程通过自噬途径在溶酶体或液泡中发生。注定要被降解的细胞质底物被包裹在称为自噬体的独特双膜运输小泡中,并被靶向运输到溶酶体/液泡进行后续的分解和再循环。对酵母自噬突变体apg和aut的遗传分析,已经开始鉴定其分子机制,同时也表明与生物合成的细胞质到液泡的靶向运输(Cvt)途径有大量重叠。运输小泡的形成是这两条途径的关键调控步骤。在本研究中,我们对自噬体和类似的Cvt小泡可能共同起源的假定区室进行了表征。显微镜分析确定了液泡周围膜是Apg1-Cvt9信号复合体和自噬/Cvt特异性磷脂酰肌醇3激酶复合体的驻留区室,其中Apg1-Cvt9信号复合体介导自噬运输和Cvt运输之间的转换。此外,液泡周围区室指定了Apg/Cvt小泡组分Aut7、Cvt货物受体Cvt19和Apg缀合机制的膜结合起始位点,该缀合机制在小泡的从头形成中起作用。尽管也支持小泡形成和包装所需的组分集中在供体膜区室的亚结构域中的范式,但对小泡组分Aut7的生化分离和密度梯度分析重现了显微镜观察结果。

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