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致病变形鞭毛虫福氏耐格里阿米巴的一种膜相关成孔蛋白的生化与功能特性

Biochemical and functional characterization of a membrane-associated pore-forming protein from the pathogenic ameboflagellate Naegleria fowleri.

作者信息

Young J D, Lowrey D M

机构信息

Laboratory of Cellular Physiology and Immunology, Rockefeller University, New York, New York 10021.

出版信息

J Biol Chem. 1989 Jan 15;264(2):1077-83.

PMID:2463245
Abstract

A membrane-bound cytolytic pore-forming protein (N-PFP) produced by the pathogenic ameboflagellate Naegleria fowleri was characterized. N-PFP was solubilized from ameba membranes by detergent and enriched 300-fold by gel filtration chromatography. When analyzed by gel electrophoresis, N-PFP migrates with a molecular mass of 66 kDa and 50-54 kDa, under reducing and non-reducing conditions, respectively. In addition to lysing erythrocytes, N-PFP is cytotoxic to several tumor cell lines tested. Its hemolytic activity is not dependent on the presence of divalent cations. N-PFP rapidly depolarizes the membrane potential of microelectrode-impaled chicken embryo myocytes, suggesting that functional channel formation may represent the mode of membrane damage. In planar bilayers, N-PFP forms ion channels with heterogeneous unit conductances ranging between 150 and 400 picosiemens in 0.1 M NaCl and that are relatively resistant to closing by high voltages. Upon heat treatment (75 degrees C, 30 min), N-PFP forms channels with unit conductances that are on average larger than those formed by untreated N-PFP. N-PFP channels are slightly more permeable to cations than to anions. Using a liposome swelling-shrinkage assay, the functional diameter of N-PFP channels is estimated to range between 3.6 and 5.2 nm. N-PFP is immunologically distinct from the PFP/perforin produced by lymphocytes, the terminal components of complement and a PFP from the ameba Entamoeba histolytica, all of which produce pores on target membranes. This protein may have a direct lytic role during target cell killing mediated by N. fowleri.

摘要

对致病性变形鞭毛虫福氏耐格里阿米巴产生的一种膜结合溶细胞成孔蛋白(N - PFP)进行了特性鉴定。N - PFP通过去污剂从阿米巴细胞膜中溶解出来,并通过凝胶过滤色谱法富集了300倍。在凝胶电泳分析时,N - PFP在还原条件下的分子量为66 kDa,在非还原条件下为50 - 54 kDa。除了裂解红细胞外,N - PFP对所测试的几种肿瘤细胞系也具有细胞毒性。其溶血活性不依赖于二价阳离子的存在。N - PFP能迅速使微电极刺入的鸡胚心肌细胞的膜电位去极化,这表明功能性通道的形成可能是膜损伤的方式。在平面双分子层中,N - PFP在0.1 M NaCl中形成具有异质单位电导的离子通道,其范围在150至400皮西门子之间,并且相对抗高压关闭。经过热处理(75摄氏度,30分钟)后,N - PFP形成的通道单位电导平均比未处理的N - PFP形成的通道大。N - PFP通道对阳离子的通透性略高于对阴离子的通透性。使用脂质体肿胀 - 收缩试验,估计N - PFP通道的功能直径在3.6至5.2纳米之间。N - PFP在免疫上与淋巴细胞产生的PFP/穿孔素、补体的终末成分以及溶组织内阿米巴的一种PFP不同,所有这些在靶膜上都会形成孔。这种蛋白在福氏耐格里阿米巴介导的靶细胞杀伤过程中可能具有直接的裂解作用。

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