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贾第虫的变异特异性表面蛋白VSP4A1是一种糖基化和棕榈酰化蛋白。

The variant-specific surface protein of Giardia, VSP4A1, is a glycosylated and palmitoylated protein.

作者信息

Papanastasiou P, McConville M J, Ralton J, Köhler P

机构信息

Institute of Parasitology, University of Zürich, Switzerland.

出版信息

Biochem J. 1997 Feb 15;322 ( Pt 1)(Pt 1):49-56. doi: 10.1042/bj3220049.

Abstract

The variant-specific surface proteins (VSPs) of the ancient protist Giardia duodenalis (syn.: Giardia intestinalis, Giardia lamblia) are cysteine- and threonine-rich polypeptides that can vary considerably in sequence and size. In the present study, we have purified a VSP (VSP4A1, formerly called CR1SP-90) from a cloned Giardia isolate, derived from a sheep, by Triton X-114 phase partitioning and anion-exchange chromatography. Analysis of the purified VSP4A1 showed that this protein is posttranslationally modified with both glycans and lipid. The glycans of VSP4A1 were detected and partially characterized by (1) compositional analysis, which indicated the presence of GlcNAc and Glc (0.5 and 1.0 mol/mol of protein respectively), and (2) the specific labelling of VSP4A1 with galactosyltransferase/UDP-[3H]Gal. The glycans were released by beta-elimination, suggesting that they are O-linked to the protein. Bio-Gel P4 chromatography of the released galactosylated glycans and further compositional analysis suggested that the major glycan on the VSP is a trisaccharide with Glc at the reducing terminus. These and other results indicate the absence of any N-linked glycans on the VSP and suggest instead that it is elaborated with a novel type of short O-linked glycan. Compositional analysis and radiolabelling experiments also indicated that VSP4A1 is modified with covalently linked palmitate (1 mol/mol of protein). Hydroxylamine treatment at neutral pH of[3H]palmitate-labelled VSP4A1 indicated that the acyl chain may be attached by a thioester linkage. A likely location for the lipid modification appears to be in the region of the C-terminal domain where it may facilitate association of the protein with the plasma membrane.

摘要

古老原生生物十二指肠贾第虫(同义词:肠贾第虫、蓝氏贾第虫)的变异特异性表面蛋白(VSPs)是富含半胱氨酸和苏氨酸的多肽,其序列和大小差异很大。在本研究中,我们通过Triton X - 114相分配和阴离子交换色谱法,从一只绵羊的克隆贾第虫分离株中纯化出一种VSP(VSP4A1,以前称为CR1SP - 90)。对纯化的VSP4A1的分析表明,该蛋白在翻译后被聚糖和脂质修饰。VSP4A1的聚糖通过以下方法检测并部分表征:(1)组成分析,表明存在GlcNAc和Glc(分别为0.5和1.0摩尔/摩尔蛋白);(2)用半乳糖基转移酶/UDP - [³H]Gal对VSP4A1进行特异性标记。聚糖通过β-消除反应释放,表明它们与蛋白质是O-连接的。对释放的半乳糖基化聚糖进行Bio-Gel P4色谱分析和进一步的组成分析表明,VSP上的主要聚糖是一种还原端为Glc的三糖。这些结果以及其他结果表明VSP上不存在任何N-连接聚糖,而是表明它是由一种新型的短O-连接聚糖修饰的。组成分析和放射性标记实验还表明VSP4A1被共价连接的棕榈酸酯(1摩尔/摩尔蛋白)修饰。在中性pH下用羟胺处理[³H]棕榈酸酯标记的VSP4A1表明,酰基链可能通过硫酯键连接。脂质修饰的一个可能位置似乎在C末端结构域区域,在那里它可能促进蛋白质与质膜的结合。

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