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玫瑰色硫囊菌BBS中NiFe氢化酶的电子传递亚基。

Electron-transfer subunits of the NiFe hydrogenases in Thiocapsa roseopersicina BBS.

作者信息

Palágyi-Mészáros Lívia S, Maróti Judit, Latinovics Dóra, Balogh Tímea, Klement Eva, Medzihradszky Katalin F, Rákhely Gábor, Kovács Kornél L

机构信息

Department of Biotechnology, University of Szeged, Hungary.

出版信息

FEBS J. 2009 Jan;276(1):164-74. doi: 10.1111/j.1742-4658.2008.06770.x. Epub 2008 Nov 19.

DOI:10.1111/j.1742-4658.2008.06770.x
PMID:19019079
Abstract

Thiocapsa roseopersicina BBS contains at least three different active NiFe hydrogenases: two membrane-bound enzymes and one apparently localized in the cytoplasm. In addition to the small and large structural subunits, additional proteins are usually associated with the NiFe hydrogenases, connecting their activity to other redox processes in the cells. The operon of the membrane-associated hydrogenase, HynSL, has an unusual gene arrangement: between the genes coding for the large and small subunits, there are two open reading frames, namely isp1 and isp2. Isp1 is a b-type haem-containing transmembrane protein, whereas Isp2 displays marked sequence similarity to the heterodisulfide reductases. The other membrane-bound (Hup) NiFe hydrogenase contains the hupC gene, which codes for a cytochrome b-type protein that probably plays a role in electron transport. The operon of the NAD(+)-reducing Hox hydrogenase contains a hoxE gene. In addition to the hydrogenase and diaphorase parts of the complex, the fifth HoxE subunit may serve as a third redox gate of this enzyme. The physiological functions of these putative electron-mediating subunits were studied by disruption of their genes. The deletion of some accessory proteins dramatically reduced the in vivo activities of the hydrogenases, although they were fully active in vitro. The absence of HupC resulted in a decrease in HupSL activity in the membrane, but removal of the Isp1 and Isp2 proteins did not have any significant effect on the location of HynSL activity. Through the use of a tagged HoxE protein, the whole Hox hydrogenase pentamer could be purified as an intact complex.

摘要

玫瑰红硫菌BBS至少包含三种不同的活性镍铁氢化酶:两种膜结合酶和一种明显定位于细胞质中的酶。除了大小结构亚基外,镍铁氢化酶通常还与其他蛋白质相关联,将其活性与细胞中的其他氧化还原过程联系起来。膜相关氢化酶HynSL的操纵子具有不寻常的基因排列:在编码大亚基和小亚基的基因之间,有两个开放阅读框,即isp1和isp2。Isp1是一种含b型血红素的跨膜蛋白,而Isp2与异二硫键还原酶具有显著的序列相似性。另一种膜结合(Hup)镍铁氢化酶含有hupC基因,该基因编码一种细胞色素b型蛋白,可能在电子传递中起作用。NAD(+)还原型Hox氢化酶的操纵子包含一个hoxE基因。除了复合物的氢化酶和黄递酶部分外,第五个HoxE亚基可能作为该酶的第三个氧化还原门。通过破坏这些假定的电子介导亚基的基因来研究它们的生理功能。一些辅助蛋白的缺失显著降低了氢化酶在体内的活性,尽管它们在体外完全有活性。HupC的缺失导致膜中HupSL活性降低,但去除Isp1和Isp2蛋白对HynSL活性的定位没有任何显著影响。通过使用标记的HoxE蛋白,可以将整个Hox氢化酶五聚体作为完整复合物纯化出来。

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