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使用扫描电化学显微镜(SECM)测量固定在金电极上羧基封端的烷硫醇单分子层上的细胞色素c的电子转移动力学。

Using scanning electrochemical microscopy (SECM) to measure the electron-transfer kinetics of cytochrome c immobilized on a COOH-terminated alkanethiol monolayer on a gold electrode.

作者信息

Holt Katherine B

机构信息

Department of Chemistry, University College London, 20 Gordon Street, London WC1H 0AJ, United Kingdom.

出版信息

Langmuir. 2006 Apr 25;22(9):4298-304. doi: 10.1021/la0529916.

Abstract

Cytochrome c was electrostatically immobilized onto a COOH-terminated alkanethiol self-assembled monolayer (SAM) on a gold electrode at ionic strengths of less than 40 mM. Scanning electrochemical microscopy (SECM) was used to simultaneously measure the electron transfer (ET) kinetics of the bimolecular ET between a solution-based redox mediator and the immobilized protein and the tunneling ET between the protein and the underlying gold electrode. Approach curves were recorded with ferrocyanide as a mediator at different coverages of cytochrome c and at different substrate potentials, allowing the measurement of k(BI) = 2 x 10(8) mol(-1) cm3 s(-1) for the bimolecular ET and k degrees = 15 s(-1) for the tunneling ET. The kinetics of ET was also found to depend on the immobilization conditions of cytochrome c: covalent attachment gave slightly slower tunneling ET values, and a mixed CH3/COOH-terminated ML gave faster tunneling ET rates. This is consistent with previous studies and is believed to be related to the degree of mobility of cyt c in its binding configuration and its orientation with respect to the underlying electrode surface.

摘要

在离子强度小于40 mM的条件下,细胞色素c通过静电作用固定在金电极上COOH端基化的烷硫醇自组装单分子层(SAM)上。利用扫描电化学显微镜(SECM)同时测量基于溶液的氧化还原介质与固定化蛋白质之间双分子电子转移(ET)的动力学,以及蛋白质与下层金电极之间的隧穿电子转移。以亚铁氰化物作为介质,在细胞色素c的不同覆盖度和不同底物电位下记录逼近曲线,得出双分子电子转移的k(BI) = 2 x 10(8) mol(-1) cm3 s(-1),隧穿电子转移的k degrees = 15 s(-1)。还发现电子转移动力学取决于细胞色素c的固定条件:共价连接导致隧穿电子转移值略慢,而CH3/COOH端基化的混合单分子层给出更快的隧穿电子转移速率。这与先前的研究一致,并且据信与细胞色素c在其结合构型中的移动程度及其相对于下层电极表面的取向有关。

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