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Characterization of a membrane pore-forming protein from Entamoeba histolytica

机译:溶组织变形杆菌的膜孔形成蛋白的表征

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摘要

We describe the partial purification and characterization of a pore- forming material (PEM) from Entamoeba histolytica. The formation of ion channels by PFM was examined in three systems. (a) PFM depolarizes J774 macrophages and mouse spleen lymphocytes as measured by [3H]TPP+ uptake. (b) PFM induces rapid monovalent cation flux across the membrane of phosphatidylcholine-cholesterol vesicles. (c) PFM confers a voltage-dependent conductance to artificial planar bilayers, which is resolved as a summation of opening of individually conducting steps of 67 pS in 0.1 M KCl. Monomers of PFM are functional; however, a preferential aggregation occurs in the planar bilayer. Activity is pronase, trypsin, and heat sensitive and is stable between pH 5-8. PFM is not secreted by unstimulated amoebae but after exposure to the calcium ionophore A23187, concanavalin A, and E. coli lipopolysaccharide, 5-10% of the total cell content of PFM is released into the medium within 5-10 min. High-performance gel filtration results in an approximately 1,000-fold purification of PFM and gives an Mr of 30,000. This protein may play a role in the cytotoxicity mediated by E. histolytica.
机译:我们描述了从组织变形虫(Entamoeba histolytica)的成孔材料(PEM)的部分纯化和表征。在三个系统中检查了由PFM形成的离子通道。 (a)PFM使J774巨噬细胞和小鼠脾淋巴细胞去极化,这是通过[3H] TPP +摄取测量的。 (b)PFM诱导穿过磷脂酰胆碱-胆固醇囊泡膜的快速单价阳离子通量。 (c)PFM将电压依赖的电导赋予人造平面双层,其解析为在0.1 M KCl中打开67 pS的单个导电步骤的总和。 PFM的单体具有功能。然而,在平面双层中发生优先聚集。酶对蛋白酶,胰蛋白酶和热敏感,在pH 5-8范围内稳定。 PFM不是由不受刺激的变形虫分泌的,而是在暴露于钙离子载体A23187,伴刀豆球蛋白A和大肠杆菌脂多糖后,在5-10分钟内PFM总细胞含量的5-10%被释放到培养基中。高性能的凝胶过滤可将PFM纯化约1,000倍,Mr为30,000。该蛋白可能在溶组织大肠杆菌介导的细胞毒性中起作用。

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