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多杀性巴氏杆菌双功能γ-谷氨酰胺半胱氨酸连接酶/谷胱甘肽合成酶(GshF)的特性分析

Characterization of the bifunctional gamma-glutamate-cysteine ligase/glutathione synthetase (GshF) of Pasteurella multocida.

作者信息

Vergauwen Bjorn, De Vos Dirk, Van Beeumen Jozef J

机构信息

Laboratory of Protein Biochemistry and Protein Engineering, Ghent University, Belgium.

出版信息

J Biol Chem. 2006 Feb 17;281(7):4380-94. doi: 10.1074/jbc.M509517200. Epub 2005 Dec 8.

DOI:10.1074/jbc.M509517200
PMID:16339152
Abstract

Glutamate-cysteine ligase (gamma-ECL) and glutathione synthetase (GS) are the two unrelated ligases that constitute the glutathione biosynthesis pathway in most eukaryotes, purple bacteria, and cyanobacteria. gamma-ECL is a member of the glutamine synthetase family, whereas GS enzymes group together with highly diverse carboxyl-to-amine/thiol ligases, all characterized by the so-called two-domain ATP-grasp fold. This generalized scheme toward the formation of glutathione, however, is incomplete, as functional steady-state levels of intracellular glutathione may also accumulate solely by import, as has been reported for the Pasteurellaceae member Haemophilus influenzae, as well as for certain Gram-positive enterococci and streptococci, or by the action of a bifunctional fusion protein (termed GshF), as has been reported recently for the Gram-positive firmicutes Streptococcus agalactiae and Listeria monocytogenes. Here, we show that yet another member of the Pasteurellaceae family, Pasteurella multocida, acquires glutathione both by import and GshF-driven biosynthesis. Domain architecture analysis shows that this P. multocida GshF bifunctional ligase contains an N-terminal gamma-proteobacterial gamma-ECL-like domain followed by a typical ATP-grasp domain, which most closely resembles that of cyanophycin synthetases, although it has no significant homology with known GS ligases. Recombinant P. multocida GshF overexpresses as an approximately 85-kDa protein, which, on the basis of gel-sizing chromatography, forms dimers in solution. The gamma-ECL activity of GshF is regulated by an allosteric type of glutathione feedback inhibition (K(i) = 13.6 mM). Furthermore, steady-state kinetics, on the basis of which we present a novel variant of half-of-the-sites reactivity, indicate intimate domain-domain interactions, which may explain the bifunctionality of GshF proteins.

摘要

谷氨酸-半胱氨酸连接酶(γ-ECL)和谷胱甘肽合成酶(GS)是两种不相关的连接酶,它们在大多数真核生物、紫色细菌和蓝细菌中构成谷胱甘肽生物合成途径。γ-ECL是谷氨酰胺合成酶家族的成员,而GS酶则与高度多样化的羧基到胺/硫醇连接酶归为一类,所有这些连接酶都具有所谓的双结构域ATP抓握折叠特征。然而,这种形成谷胱甘肽的一般模式并不完整,因为细胞内谷胱甘肽的功能稳态水平也可能仅通过导入而积累,如巴斯德菌科成员流感嗜血杆菌以及某些革兰氏阳性肠球菌和链球菌的情况,或者通过双功能融合蛋白(称为GshF)的作用而积累,如最近报道的革兰氏阳性厚壁菌无乳链球菌和单核细胞增生李斯特菌的情况。在这里,我们表明巴斯德菌科家族的另一个成员多杀巴斯德菌通过导入和GshF驱动的生物合成获得谷胱甘肽。结构域结构分析表明,这种多杀巴斯德菌GshF双功能连接酶包含一个N端γ-变形菌γ-ECL样结构域,随后是一个典型的ATP抓握结构域,该结构域与藻青素合成酶的结构域最相似,尽管它与已知的GS连接酶没有明显的同源性。重组多杀巴斯德菌GshF以大约85 kDa的蛋白质形式过表达,根据凝胶过滤色谱法,它在溶液中形成二聚体。GshF的γ-ECL活性受变构类型的谷胱甘肽反馈抑制(K(i)=13.6 mM)调节。此外,基于稳态动力学我们提出了一种新的半位点反应性变体,这表明结构域间存在紧密的相互作用,这可能解释了GshF蛋白的双功能性。

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