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β-D-呋喃半乳糖在硕大利什曼原虫巨噬细胞侵袭中的作用。

Role of beta-D-galactofuranose in Leishmania major macrophage invasion.

作者信息

Suzuki Erika, Tanaka Ameria K, Toledo Marcos S, Takahashi Helio K, Straus Anita H

机构信息

Department of Biochemistry, Universidade Federal de São Paulo/Escola Paulista de Medicina, Brazil.

出版信息

Infect Immun. 2002 Dec;70(12):6592-6. doi: 10.1128/IAI.70.12.6592-6596.2002.

Abstract

The role of glycosylinositol phospholipid 1 (GIPL-1) of Leishmania (Leishmania) major in the interaction of promastigotes and amastigotes with macrophages was analyzed. Monoclonal antibody MEST-1, which recognizes glycolipids containing terminal galactofuranose (Galf) residues (E. Suzuki, M. S. Toledo, H. K. Takahashi, and A. H. Straus, Glycobiology 7:463-468, 1997), was used to detect GIPL-1 in Leishmania by indirect immunofluorescence and to analyze its role in macrophage infectivity. L. major promastigotes showed intense fluorescence with MEST-1, and GIPL-1 was detected in both amastigote and promastigote forms by high-performance thin-layer chromatography immunostaining by using MEST-1. Delipidation of L. major promastigotes with isopropanol-hexane-water eliminated the MEST-1 reactivity, confirming that only GIPL-1 is recognized in either amastigotes or promastigotes of this species. The biological role of GIPL-1 in the ability of L. major to invade macrophages was studied by using either Fab fragments of MEST-1 or methylglycosides. Preincubation of parasites with Fab fragments reduced macrophage infectivity in about 80% of the promastigotes and 30% of the amastigotes. Preincubation of peritoneal macrophages with p-nitrophenyl-beta-galactofuranoside (10 mM) led to significant ( approximately 80%) inhibition of promastigote infectivity. These data suggest that a putative new receptor recognizing beta-D-Galf is associated with L. major macrophage infectivity and that GIPL-1 containing a terminal Galf residue is involved in the L. major-macrophage interaction.

摘要

分析了硕大利什曼原虫(利什曼原虫属)的糖基肌醇磷脂1(GIPL-1)在前鞭毛体和无鞭毛体与巨噬细胞相互作用中的作用。单克隆抗体MEST-1可识别含有末端半乳呋喃糖(Galf)残基的糖脂(E. Suzuki、M. S. Toledo、H. K. Takahashi和A. H. Straus,《糖生物学》7:463 - 468,1997),通过间接免疫荧光法用于检测利什曼原虫中的GIPL-1,并分析其在巨噬细胞感染性中的作用。硕大利什曼原虫前鞭毛体与MEST-1呈现强烈荧光,通过使用MEST-1的高效薄层色谱免疫染色在无鞭毛体和前鞭毛体形式中均检测到GIPL-1。用异丙醇 - 己烷 - 水对硕大利什曼原虫前鞭毛体进行脱脂处理消除了MEST-1反应性,证实该物种的无鞭毛体或前鞭毛体中仅识别GIPL-1。通过使用MEST-1的Fab片段或甲基糖苷研究了GIPL-1在硕大利什曼原虫侵袭巨噬细胞能力中的生物学作用。用Fab片段对寄生虫进行预孵育可使约80%的前鞭毛体和30%的无鞭毛体的巨噬细胞感染性降低。用对硝基苯基 - β - 半乳呋喃糖苷(10 mM)对腹腔巨噬细胞进行预孵育可导致前鞭毛体感染性显著(约80%)抑制。这些数据表明,一种假定的识别β - D - Galf的新受体与硕大利什曼原虫巨噬细胞感染性相关,并且含有末端Galf残基的GIPL-1参与了硕大利什曼原虫 - 巨噬细胞相互作用。

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