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嗜盐古菌沃氏嗜盐栖热菌ATP合酶的特性、亚基结构及ATP合酶基因的组织

Characterization and subunit structure of the ATP synthase of the halophilic archaeon Haloferax volcanii and organization of the ATP synthase genes.

作者信息

Steinert K, Wagner V, Kroth-Pancic P G, Bickel-Sandkötter S

机构信息

Institut für Biochemie der Pflanzen, Heinrich-Heine-Universität Düsseldorf, Universitätsstrasse 1, D-40225 Düsseldorf, Federal Republic of Germany.

出版信息

J Biol Chem. 1997 Mar 7;272(10):6261-9. doi: 10.1074/jbc.272.10.6261.

DOI:10.1074/jbc.272.10.6261
PMID:9045643
Abstract

The archaeal ATPase of the halophile Haloferax volcanii synthesizes ATP at the expense of a proton gradient, as shown by sensitivity to the uncoupler carboxyl cyanide p-trifluoromethoxyphenylhydrazone, to the ionophore nigericin, and to the proton channel-modifying reagent N,N'-dicyclohexylcarbodiimide. The conditions for an optimally active ATP synthase have been determined. We were able to purify the enzyme complex and to identify the larger subunits with antisera raised against synthetic peptides. To identify additional subunits of this enzyme complex, we cloned and sequenced a gene cluster encoding five hydrophilic subunits of the A1 part of the proton-translocating archaeal ATP synthase. Initiation, termination, and ribosome-binding sequences as well as the result of a single transcript suggest that the ATPase genes are organized in an operon. The calculated molecular masses of the deduced gene products are 22. 0 kDa (subunit D), 38.7 kDa (subunit C), 11.6 kDa (subunit E), 52.0 kDa (subunit B), and 64.5 kDa (subunit A). The described operon contains genes in the order D, C, E, B, and A; it contains no gene for the hydrophobic, so-called proteolipid (subunit c, the proton-conducting subunit of the A0 part). This subunit has been isolated and purified; its molecular mass as deduced by SDS-polyacrylamide gel electrophoresis is 9.7 kDa.

摘要

嗜盐菌沃氏嗜盐碱杆菌的古菌ATP酶利用质子梯度合成ATP,这可通过其对解偶联剂羰基氰对三氟甲氧基苯腙、离子载体尼日利亚菌素和质子通道修饰试剂N,N'-二环己基碳二亚胺的敏感性得以证明。已确定了使ATP合酶活性最佳的条件。我们成功纯化了该酶复合物,并用针对合成肽产生的抗血清鉴定了较大的亚基。为了鉴定该酶复合物的其他亚基,我们克隆并测序了一个基因簇,该基因簇编码质子转运古菌ATP合酶A1部分的五个亲水性亚基。起始、终止和核糖体结合序列以及单一转录本的结果表明,ATP酶基因以操纵子形式组织。推导的基因产物的计算分子量分别为22.0 kDa(亚基D)、38.7 kDa(亚基C)、11.6 kDa(亚基E)、52.0 kDa(亚基B)和64.5 kDa(亚基A)。所述操纵子包含按D、C、E、B和A顺序排列的基因;它不包含编码疏水性所谓的蛋白脂质(亚基c,A0部分的质子传导亚基)的基因。该亚基已被分离和纯化;通过SDS-聚丙烯酰胺凝胶电泳推导其分子量为9.7 kDa。

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