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连接血红素和钼结构域的多肽连接物中大规模氨基酸取代对人亚硫酸氧化酶催化作用的影响。

Effects of large-scale amino acid substitution in the polypeptide tether connecting the heme and molybdenum domains on catalysis in human sulfite oxidase.

机构信息

Department of Chemistry and Biochemistry, The University of Arizona, 1306 E. University Blvd., Tucson, AZ 85721, USA.

出版信息

Metallomics. 2010 Nov;2(11):766-70. doi: 10.1039/c0mt00021c. Epub 2010 Sep 20.

DOI:10.1039/c0mt00021c
PMID:21072368
Abstract

Sulfite oxidase (SO) is a molybdenum-cofactor-dependent enzyme that catalyzes the oxidation of sulfite to sulfate, the final step in the catabolism of the sulfur-containing amino acids, cysteine and methionine. The catalytic mechanism of vertebrate SO involves intramolecular electron transfer (IET) from molybdenum to the integral b-type heme of SO and then to exogenous cytochrome c. However, the crystal structure of chicken sulfite oxidase (CSO) has shown that there is a 32 Å distance between the Fe and Mo atoms of the respective heme and molybdenum domains, which are connected by a flexible polypeptide tether. This distance is too long to be consistent with the measured IET rates. Previous studies have shown that IET is viscosity dependent (Feng et al., Biochemistry, 2002, 41, 5816) and also dependent upon the flexibility and length of the tether (Johnson-Winters et al., Biochemistry, 2010, 49, 1290). Since IET in CSO is more rapid than in human sulfite oxidase (HSO) (Feng et al., Biochemistry, 2003, 42, 12235) the tether sequence of HSO has been mutated into that of CSO, and the resultant chimeric HSO enzyme investigated by laser flash photolysis and steady-state kinetics in order to study the specificity of the tether sequence of SO on the kinetic properties. Surprisingly, the IET kinetics of the chimeric HSO protein with the CSO tether sequence are slower than wildtype HSO. This observation raises the possibility that the composition of the non-conserved tether sequence of animal SOs may be optimized for individual species.

摘要

亚硫酸氧化酶 (SO) 是一种钼辅因子依赖性酶,可催化亚硫酸盐氧化为硫酸盐,这是含硫氨基酸半胱氨酸和蛋氨酸分解代谢的最后一步。脊椎动物 SO 的催化机制涉及钼到 SO 整联 b 型血红素的分子内电子转移 (IET),然后到外源性细胞色素 c。然而,鸡亚硫酸氧化酶 (CSO) 的晶体结构表明,其血红素和钼结构域的 Fe 和 Mo 原子之间的距离为 32 Å,由柔性多肽连接。这个距离太长,与测量的 IET 速率不一致。以前的研究表明,IET 是粘度依赖性的 (Feng 等人,生物化学,2002,41,5816),并且还取决于连接物的灵活性和长度 (Johnson-Winters 等人,生物化学,2010,49,1290)。由于 CSO 中的 IET 比人亚硫酸氧化酶 (HSO) 更快 (Feng 等人,生物化学,2003,42,12235),因此 HSO 的连接序列被突变为 CSO,然后通过激光闪光光解和稳态动力学研究嵌合 HSO 酶,以研究 SO 连接序列对动力学特性的特异性。令人惊讶的是,具有 CSO 连接序列的嵌合 HSO 蛋白的 IET 动力学比野生型 HSO 慢。这一观察结果提出了这样一种可能性,即动物 SO 非保守连接序列的组成可能针对特定物种进行了优化。

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引用本文的文献

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Probing the role of a conserved salt bridge in the intramolecular electron transfer kinetics of human sulfite oxidase.探究保守盐桥在人亚硫酸盐氧化酶分子内电子转移动力学中的作用。
J Biol Inorg Chem. 2013 Aug;18(6):645-53. doi: 10.1007/s00775-013-1010-8. Epub 2013 Jun 19.
2
Kinetic and thermodynamic effects of mutations of human sulfite oxidase.人亚硫酸盐氧化酶突变的动力学和热力学效应
Chem Biodivers. 2012 Sep;9(9):1621-34. doi: 10.1002/cbdv.201200010.
3
Determination of the distance between the Mo(V) and Fe(III) heme centers of wild type human sulfite oxidase by pulsed EPR spectroscopy.
通过脉冲 EPR 光谱法测定野生型人亚硫酸氧化酶中 Mo(V)和 Fe(III)血红素中心之间的距离。
J Phys Chem B. 2012 Feb 16;116(6):1942-50. doi: 10.1021/jp210578f. Epub 2012 Feb 3.
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Elucidating the catalytic mechanism of sulfite oxidizing enzymes using structural, spectroscopic, and kinetic analyses.利用结构、光谱和动力学分析阐明亚硫酸盐氧化酶的催化机制。
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