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Voltammetry and In Situ Scanning Tunneling Microscopy of Cytochrome c Nitrite Reductase on Au(111) Electrodes

机译:在Au(111)电极上的细胞色素c亚硝酸盐还原酶的伏安法和原位扫描隧道显微镜

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摘要

Escherichia coli cytochrome c nitrite reductase (NrfA) catalyzes the six-electron reduction of nitrite to perform an important role in the biogeochemical cycling of nitrogen. Here we describe NrfA adsorption on single-crystal Au(111) electrodes as an electrocatalytically active film in which the enzyme undergoes direct electron exchange with the electrode. The adsorbed NrfA has been imaged to molecular resolution by in situ scanning tunneling microscopy (in situ STM) under full electrochemical potential control and under conditions where the enzyme is electrocatalytically active. Details of the density and orientational distribution of NrfA molecules are disclosed. The submonolayer coverage resolved by in situ STM is readily reconciled with the failure to detect nonturnover signals in cyclic voltammetry of the NrfA films. The molecular structures show a range of lateral dimensions. These are suggestive of a distribution of orientations that could account for the otherwise anomalously low turnover number calculated for the total population of adsorbed NrfA molecules when compared with that determined for solutions of NrfA. Thus, comparison of the voltammetric signals and in situ STM images offers a direct approach to correlate electrocatalytic and molecular properties of the protein layer, a long-standing issue in protein film voltammetry.
机译:大肠杆菌细胞色素c亚硝酸还原酶(NrfA)催化亚硝酸盐的六电子还原,从而在氮的生物地球化学循环中发挥重要作用。在这里,我们将NrfA吸附在单晶Au(111)电极上作为一种电催化活性膜,其中酶与电极进行直接电子交换。已吸附的NrfA在完全电化学势能控制下和酶具有电催化活性的条件下,通过原位扫描隧道显微镜(原位STM)成像至分子分辨率。公开了NrfA分子的密度和取向分布的细节。通过原位STM解决的亚单分子层覆盖率很容易与NrfA膜的循环伏安法中未检测到非翻转信号的情况相吻合。分子结构显示出一系列横向尺寸。这些暗示了取向的分布,该取向的分布可能解释了当与针对NrfA的溶液所确定的相比时,对于吸附的NrfA分子的总群体计算出的异常低的营业额。因此,比较伏安信号和原位STM图像提供了一种直接方法来关联蛋白质层的电催化和分子特性,这是蛋白质膜伏安法中的一个长期存在的问题。

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