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自噬及细胞质到液泡靶向途径中Aut7p的膜募集需要Aut1p、Aut2p和自噬缀合复合体。

Membrane recruitment of Aut7p in the autophagy and cytoplasm to vacuole targeting pathways requires Aut1p, Aut2p, and the autophagy conjugation complex.

作者信息

Kim J, Huang W P, Klionsky D J

机构信息

Department of Biology, University of Michigan, Ann Arbor, Michigan 48109, USA.

出版信息

J Cell Biol. 2001 Jan 8;152(1):51-64. doi: 10.1083/jcb.152.1.51.

DOI:10.1083/jcb.152.1.51
PMID:11149920
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2193654/
Abstract

Autophagy is a degradative pathway by which cells sequester nonessential, bulk cytosol into double-membrane vesicles (autophagosomes) and deliver them to the vacuole for recycling. Using this strategy, eukaryotic cells survive periods of nutritional starvation. Under nutrient-rich conditions, autophagy machinery is required for the delivery of a resident vacuolar hydrolase, aminopeptidase I, by the cytoplasm to vacuole targeting (Cvt) pathway. In both pathways, the vesicle formation process requires the function of the starvation-induced Aut7 protein, which is recruited from the cytosol to the forming Cvt vesicles and autophagosomes. The membrane binding of Aut7p represents an early step in vesicle formation. In this study, we identify several requirements for Aut7p membrane association. After synthesis in the cytosol, Aut7p is proteolytically cleaved in an Aut2p-dependent manner. While this novel processing event is essential for Aut7p membrane binding, Aut7p must undergo additional physical interactions with Aut1p and the autophagy (Apg) conjugation complex before recruitment to the membrane. Lack of these interactions results in a cytosolic distribution of Aut7p rather than localization to forming Cvt vesicles and autophagosomes. This study assigns a functional role for the Apg conjugation system as a mediator of Aut7p membrane recruitment. Further, we demonstrate that Aut1p, which physically interacts with components of the Apg conjugation complex and Aut7p, constitutes an additional factor required for Aut7p membrane recruitment. These findings define a series of steps that results in the modification of Aut7p and its subsequent binding to the sequestering transport vesicles of the autophagy and cytoplasm to vacuole targeting pathways.

摘要

自噬是一种降解途径,通过该途径细胞将非必需的大量细胞质隔离到双膜囊泡(自噬体)中,并将它们输送到液泡进行循环利用。利用这种策略,真核细胞能够在营养饥饿时期存活下来。在营养丰富的条件下,细胞质到液泡靶向(Cvt)途径需要自噬机制来输送驻留液泡水解酶氨基肽酶I。在这两种途径中,囊泡形成过程都需要饥饿诱导的Aut7蛋白发挥作用,该蛋白从细胞质中被募集到正在形成的Cvt囊泡和自噬体上。Aut7蛋白与膜的结合是囊泡形成的早期步骤。在本研究中,我们确定了Aut7蛋白与膜结合的几个必要条件。在细胞质中合成后,Aut7蛋白以依赖于Aut2蛋白的方式被蛋白水解切割。虽然这种新的加工事件对于Aut7蛋白与膜的结合至关重要,但Aut7蛋白在被募集到膜上之前必须与Aut1蛋白和自噬(Apg)缀合复合物进行额外的物理相互作用。缺乏这些相互作用会导致Aut7蛋白在细胞质中分布,而不是定位于正在形成的Cvt囊泡和自噬体。本研究赋予Apg缀合系统作为Aut7蛋白膜募集介质的功能作用。此外,我们证明与Apg缀合复合物和Aut7蛋白的组分发生物理相互作用的Aut1蛋白是Aut7蛋白膜募集所需的另一个因素。这些发现定义了一系列步骤,这些步骤导致Aut7蛋白的修饰及其随后与自噬和细胞质到液泡靶向途径的隔离运输囊泡的结合。

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3
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自噬调节剂对子囊菌植物真菌致病性的抑制作用。
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