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恶性疟原虫裂殖子表面蛋白2:保守N端结构域的表达、结构、动力学及纤维形成

Merozoite surface protein 2 of Plasmodium falciparum: expression, structure, dynamics, and fibril formation of the conserved N-terminal domain.

作者信息

Low Andrew, Chandrashekaran Indu R, Adda Christopher G, Yao Shenggen, Sabo Jennifer K, Zhang Xuecheng, Soetopo Alfreda, Anders Robin F, Norton Raymond S

机构信息

The Walter and Eliza Hall Institute of Medical Research, 1G Royal Parade, Parkville, VIC 3050, Australia.

出版信息

Biopolymers. 2007 Sep;87(1):12-22. doi: 10.1002/bip.20764.

DOI:10.1002/bip.20764
PMID:17516503
Abstract

Merozoite surface protein 2 (MSP2) is a GPI-anchored protein on the surface of the merozoite stage of the malaria parasite Plasmodium falciparum. It is largely disordered in solution, but has a propensity to form amyloid-like fibrils under physiological conditions. The N-terminal conserved region (MSP2(1-25)) is part of the protease-resistant core of these fibrils. To investigate the structure and dynamics of this region, its ability to form fibrils, and the role of individual residues in these properties, we have developed a bacterial expression system that yields > or =10 mg of unlabeled or (15)N-labeled peptide per litre of culture. Two recombinant versions of MSP2(1-25), wild-type and a Y7A/Y16A mutant, have been produced. Detailed conformational analysis of the wild-type peptide and backbone (15)N relaxation data indicated that it contains beta-turn and nascent helical structures in the central and C-terminal regions. Residues 6-21 represent the most ordered region of the structure, although there is some flexibility around residues 8 and 9. The 10-residue sequence (MSP2(7-16)) (with two Tyr residues) was predicted to have a higher propensity for beta-aggregation than the 8-mer sequence (MSP2(8-15)), but there was no significant difference in conformation between MSP2(1-25) and [Y7A,Y16A]MSP2(1-25) and the rate of fibril formation was only slightly slower in the mutant. The peptide expression system described here will facilitate further mutational analyses to define the roles of individual residues in transient structural elements and fibril formation, and thus contribute to the further development of MSP2 as a malaria vaccine candidate.

摘要

裂殖子表面蛋白2(MSP2)是恶性疟原虫裂殖子阶段表面的一种糖基磷脂酰肌醇(GPI)锚定蛋白。它在溶液中大多呈无序状态,但在生理条件下有形成淀粉样纤维的倾向。N端保守区域(MSP2(1 - 25))是这些纤维抗蛋白酶核心的一部分。为了研究该区域的结构和动力学、其形成纤维的能力以及单个残基在这些特性中的作用,我们开发了一种细菌表达系统,每升培养物可产生≥10 mg未标记或(15)N标记的肽。已制备了MSP2(1 - 25)的两种重组变体,即野生型和Y7A/Y16A突变体。对野生型肽和主链(15)N弛豫数据的详细构象分析表明,它在中央和C端区域含有β-转角和新生螺旋结构。残基6 - 21代表结构中最有序的区域,尽管残基8和9周围存在一些灵活性。10个残基的序列(MSP2(7 - 16))(有两个酪氨酸残基)预计比8聚体序列(MSP2(8 - 15))具有更高的β-聚集倾向,但MSP2(1 - 25)与[Y7A,Y16A]MSP2(1 - 25)之间的构象没有显著差异,并且突变体中纤维形成速率仅略慢。本文所述的肽表达系统将有助于进一步的突变分析,以确定单个残基在瞬时结构元件和纤维形成中的作用,从而有助于将MSP2进一步开发为疟疾疫苗候选物。

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