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利什曼原虫中异常的自噬相关蛋白8(ATG8)样蛋白家族和自噬相关蛋白12(ATG12)的特征分析

Characterization of unusual families of ATG8-like proteins and ATG12 in the protozoan parasite Leishmania major.

作者信息

Williams Roderick A M, Woods Kerry L, Juliano Luiz, Mottram Jeremy C, Coombs Graham H

机构信息

Strathclyde Institute of Pharmacy and Biomedical Sciences, University of Strathclyde, Glasgow, Scotland, UK.

出版信息

Autophagy. 2009 Feb;5(2):159-72. doi: 10.4161/auto.5.2.7328. Epub 2009 Feb 4.

DOI:10.4161/auto.5.2.7328
PMID:19066473
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2642932/
Abstract

Leishmania major possesses, apparently uniquely, four families of ATG8-like genes, designated ATG8, ATG8A, ATG8B and ATG8C, and 25 genes in total. L. major ATG8 and examples from the ATG8A, ATG8B and ATG8C families are able to complement a Saccharomyces cerevisiae ATG8-deficient strain, indicating functional conservation. Whereas ATG8 has been shown to form putative autophagosomes during differentiation and starvation of L. major, ATG8A primarily form puncta in response to starvation-suggesting a role for ATG8A in starvation-induced autophagy. Recombinant ATG8A was processed at the scissile glycine by recombinant ATG4.2 but not ATG4.1 cysteine peptidases of L. major and, consistent with this, ATG4.2-deficient L. major mutants were unable to process ATG8A and were less able to withstand starvation than wild-type cells. GFP-ATG8-containing puncta were less abundant in ATG4.2 overexpression lines, in which unlipidated ATG8 predominated, which is consistent with ATG4.2 being an ATG8-deconjugating enzyme as well as an ATG8A-processing enzyme. In contrast, recombinant ATG8, ATG8B and ATG8C were all processed by ATG4.1, but not by ATG4.2. ATG8B and ATG8C both have a distinct subcellular location close to the flagellar pocket, but the occurrence of the GFP-labeled puncta suggest that they do not have a role in autophagy. L. major genes encoding possible ATG5, ATG10 and ATG12 homologues were found to complement their respective S. cerevisiae mutants, and ATG12 localized in part to ATG8-containing puncta, suggestive of a functional ATG5-ATG12 conjugation pathway in the parasite. L. major ATG12 is unusual as it requires C-terminal processing by an as yet unidentified peptidase.

摘要

硕大利什曼原虫显然独特地拥有四个类似ATG8的基因家族,分别命名为ATG8、ATG8A、ATG8B和ATG8C,总共25个基因。硕大利什曼原虫的ATG8以及ATG8A、ATG8B和ATG8C家族的示例能够互补酿酒酵母ATG8缺陷型菌株,表明功能保守。虽然已证明ATG8在硕大利什曼原虫的分化和饥饿期间形成假定的自噬体,但ATG8A主要在饥饿时形成斑点,这表明ATG8A在饥饿诱导的自噬中起作用。重组ATG8A由重组ATG4.2在可裂解甘氨酸处进行加工,但不由硕大利什曼原虫的ATG4.1半胱氨酸肽酶加工,与此一致的是,ATG4.2缺陷型硕大利什曼原虫突变体无法加工ATG8A,并且比野生型细胞更难以耐受饥饿。在ATG4.2过表达系中,含GFP-ATG8的斑点较少,其中未脂化的ATG8占主导,这与ATG4.2是一种ATG8去偶联酶以及一种ATG8A加工酶一致。相反,重组ATG8、ATG8B和ATG8C均由ATG4.1加工,但不由ATG4.2加工。ATG8B和ATG8C都有一个靠近鞭毛囊的独特亚细胞定位,但GFP标记斑点的出现表明它们在自噬中不起作用。发现编码可能的ATG5、ATG10和ATG12同源物的硕大利什曼原虫基因能够互补各自的酿酒酵母突变体,并且ATG12部分定位于含ATG8的斑点,提示该寄生虫中存在功能性的ATG5-ATG12偶联途径。硕大利什曼原虫的ATG12不同寻常,因为它需要一种尚未鉴定的肽酶进行C末端加工。