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结构和生化分析表明,一种细菌过硫化物双加氧酶-硫氰酸酶融合蛋白在硫同化过程中发挥作用。

Structural and biochemical analyses indicate that a bacterial persulfide dioxygenase-rhodanese fusion protein functions in sulfur assimilation.

作者信息

Motl Nicole, Skiba Meredith A, Kabil Omer, Smith Janet L, Banerjee Ruma

机构信息

From the Department of Biological Chemistry, University of Michigan Medical Center, Ann Arbor, Michigan 48109-0600.

From the Department of Biological Chemistry, University of Michigan Medical Center, Ann Arbor, Michigan 48109-0600; Life Sciences Institute, University of Michigan, Ann Arbor, Michigan 48109.

出版信息

J Biol Chem. 2017 Aug 25;292(34):14026-14038. doi: 10.1074/jbc.M117.790170. Epub 2017 Jul 6.

Abstract

Hydrogen sulfide (HS) is a signaling molecule that is toxic at elevated concentrations. In eukaryotes, it is cleared via a mitochondrial sulfide oxidation pathway, which comprises sulfide quinone oxidoreductase, persulfide dioxygenase (PDO), rhodanese, and sulfite oxidase and converts HS to thiosulfate and sulfate. Natural fusions between the non-heme iron containing PDO and rhodanese, a thiol sulfurtransferase, exist in some bacteria. However, little is known about the role of the PDO-rhodanese fusion (PRF) proteins in sulfur metabolism. Herein, we report the kinetic properties and the crystal structure of a PRF from the Gram-negative endophytic bacterium The crystal structures of wild-type PRF and a sulfurtransferase-inactivated C314S mutant with and without glutathione were determined at 1.8, 2.4, and 2.7 Å resolution, respectively. We found that the two active sites are distant and do not show evidence of direct communication. The PRF exhibited robust PDO activity and preferentially catalyzed sulfur transfer in the direction of thiosulfate to sulfite and glutathione persulfide; sulfur transfer in the reverse direction was detectable only under limited turnover conditions. Together with the kinetic data, our bioinformatics analysis reveals that PRF is poised to metabolize thiosulfate to sulfite in a sulfur assimilation pathway rather than in sulfide stress response as seen, for example, with the PRF or sulfide oxidation and disposal as observed with the homologous mammalian proteins.

摘要

硫化氢(HS)是一种信号分子,在浓度升高时具有毒性。在真核生物中,它通过线粒体硫化物氧化途径清除,该途径包括硫化物醌氧化还原酶、过硫化物双加氧酶(PDO)、硫氰酸酶和亚硫酸盐氧化酶,可将HS转化为硫代硫酸盐和硫酸盐。在一些细菌中存在含非血红素铁的PDO与硫醇硫转移酶硫氰酸酶之间的天然融合。然而,关于PDO-硫氰酸酶融合(PRF)蛋白在硫代谢中的作用知之甚少。在此,我们报道了一种来自革兰氏阴性内生细菌的PRF的动力学特性和晶体结构。分别在1.8 Å、2.4 Å和2.7 Å分辨率下测定了野生型PRF以及有和没有谷胱甘肽的硫转移酶失活的C314S突变体的晶体结构。我们发现两个活性位点相距较远,没有直接通讯的证据。该PRF表现出强大的PDO活性,优先催化硫从硫代硫酸盐向亚硫酸盐和谷胱甘肽过硫化物的转移方向;仅在有限的周转条件下才能检测到反向硫转移。结合动力学数据,我们的生物信息学分析表明,PRF倾向于在硫同化途径中将硫代硫酸盐代谢为亚硫酸盐,而不是像例如PRF那样在硫化物应激反应中,也不是像同源哺乳动物蛋白那样进行硫化物氧化和处理。

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