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通过表面增强共振拉曼光谱和电化学方法联合研究表面结合的人亚硫酸氧化酶的氧化还原性质和催化活性。

Redox properties and catalytic activity of surface-bound human sulfite oxidase studied by a combined surface enhanced resonance Raman spectroscopic and electrochemical approach.

机构信息

Technische Universität Berlin, Institut für Chemie, Sekr. PC 14, Strasse des 17. Juni 135, D-10623 Berlin, Germany.

出版信息

Phys Chem Chem Phys. 2010 Jul 28;12(28):7894-903. doi: 10.1039/b927226g. Epub 2010 May 26.

DOI:10.1039/b927226g
PMID:20502841
Abstract

Human sulfite oxidase (hSO) was immobilised on SAM-coated silver electrodes under preservation of the native heme pocket structure of the cytochrome b5 (Cyt b5) domain and the functionality of the enzyme. The redox properties and catalytic activity of the entire enzyme were studied by surface enhanced resonance Raman (SERR) spectroscopy and cyclic voltammetry (CV) and compared to the isolated heme domain when possible. It is shown that heterogeneous electron transfer and catalytic activity of hSO sensitively depend on the local environment of the enzyme. Increasing the ionic strength of the buffer solution leads to an increase of the heterogeneous electron transfer rate from 17 s(-1) to 440 s(-1) for hSO as determined by SERR spectroscopy. CV measurements demonstrate an increase of the apparent turnover rate for the immobilised hSO from 0.85 s(-1) in 100 mM buffer to 5.26 s(-1) in 750 mM buffer. We suggest that both effects originate from the increased mobility of the surface-bound enzyme with increasing ionic strength. In agreement with surface potential calculations we propose that at high ionic strength the enzyme is immobilised via the dimerisation domain to the SAM surface. The flexible loop region connecting the Moco and the Cyt b5 domain allows alternating contact with the Moco interaction site and the SAM surface, thereby promoting the sequential intramolecular and heterogeneous electron transfer from Moco via Cyt b5 to the electrode. At lower ionic strength, the contact time of the Cyt b5 domain with the SAM surface is longer, corresponding to a slower overall electron transfer process.

摘要

人亚硫酸盐氧化酶 (hSO) 在保持细胞色素 b5 (Cyt b5) 结构域的天然血红素口袋结构和酶的功能的情况下固定在 SAM 涂层的银电极上。通过表面增强共振拉曼 (SERR) 光谱和循环伏安法 (CV) 研究了整个酶的氧化还原性质和催化活性,并尽可能与分离的血红素结构域进行了比较。结果表明,hSO 的异相电子转移和催化活性敏感地依赖于酶的局部环境。通过 SERR 光谱测定,缓冲溶液离子强度的增加导致 hSO 的异相电子转移速率从 17 s(-1)增加到 440 s(-1)。CV 测量表明,固定化 hSO 的表观周转率从 100 mM 缓冲液中的 0.85 s(-1)增加到 750 mM 缓冲液中的 5.26 s(-1)。我们认为这两种效应都源于随着离子强度的增加表面结合酶的迁移率增加。与表面电势计算一致,我们提出在高离子强度下,酶通过二聚化结构域固定在 SAM 表面上。连接 Moco 和 Cyt b5 结构域的柔性环区允许与 Moco 相互作用位点和 SAM 表面交替接触,从而促进从 Moco 通过 Cyt b5 到电极的顺序分子内和异相电子转移。在较低的离子强度下,Cyt b5 结构域与 SAM 表面的接触时间更长,对应于较慢的整体电子转移过程。

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