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普氏立克次氏体ATP/ADP转位酶的增溶与复性

Solubilization and reconstitution of the Rickettsia prowazekii ATP/ADP translocase.

作者信息

Plano G V, Winkler H H

机构信息

Department of Microbiology and Immunology, University of South Alabama College of Medicine, Mobile 36688.

出版信息

J Membr Biol. 1989 Sep;110(3):227-33. doi: 10.1007/BF01869153.

Abstract

The ATP/ADP translocase protein of Rickettsia prowazekii, an obligate intracellular parasite that had been grown in the chick yolk sac, was solubilized and reconstituted into liposomes composed of Escherichia coli phospholipid by an octylglucoside dilution procedure. Proteoliposomes prepared from membranes of Renografin-purified R. prowazekii translocated ATP by an obligate exchange mechanism. Influx of extravesicular ATP required intravesicular transportable nucleotide and efflux of intravesicular ATP required transportable extravesicular nucleotide in the medium. The transport activity was insensitive to carboxyatractyloside and bongkrekic acid, inhibitors of mitochondrial ADP/ATP translocation. Proteoliposomes prepared from membranes of standard (non-Renografin-purified) R. prowazekii exhibited both an inhibitor-sensitive mitochondrial translocase activity and an inhibitor-resistant rickettsial translocase activity. Proteoliposomes prepared from uninoculated yolk sac membranes exhibited only the inhibitor-sensitive mitochondrial translocase activity. The substrate specificity of each reconstituted translocase was determined and shown to correspond with that reported for intact mitochondria or rickettsiae. Following influx of ATP the steady-state value for intravesicular labeled ATP was dependent on the concentration of intravesicular nucleotide available for exchange.

摘要

普氏立克次体是一种专性细胞内寄生虫,曾在鸡卵黄囊中培养,其ATP/ADP转位酶蛋白通过辛基葡糖苷稀释法溶解,并重新组装到由大肠杆菌磷脂组成的脂质体中。用泛影葡胺纯化的普氏立克次体膜制备的蛋白脂质体通过专一性交换机制转运ATP。囊泡外ATP的流入需要囊泡内可转运的核苷酸,而囊泡内ATP的流出需要培养基中可转运的囊泡外核苷酸。该转运活性对线粒体ADP/ATP转位的抑制剂羧基苍术苷和邦克雷酸不敏感。用标准(未用泛影葡胺纯化)的普氏立克次体膜制备的蛋白脂质体表现出对抑制剂敏感的线粒体转位酶活性和对抑制剂有抗性的立克次体转位酶活性。用未接种的卵黄囊膜制备的蛋白脂质体仅表现出对抑制剂敏感的线粒体转位酶活性。测定了每种重组转位酶的底物特异性,结果表明与完整线粒体或立克次体报道的底物特异性一致。ATP流入后,囊泡内标记ATP的稳态值取决于可用于交换的囊泡内核苷酸的浓度。

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