Abstract
ConspectusEnzymes are the essential catalytic components of biology and adsorbing redox-active enzymes on electrode surfaces enables the direct probing of their function. Through standard electrochemical measurements, catalytic activity, reversibility and stability, potentials of redox-active cofactors, and interfacial electron transfer rates can be readily measured. Mechanistic investigations on the high electrocatalytic rates and selectivity of enzymes may yield inspiration for the design of synthetic molecular and heterogeneous electrocatalysts. Electrochemical investigations of enzymes also aid in our understanding of their activity within their biological environment and why they evolved in their present structure and function. However, the conventional array of electrochemical techniques (e.g., voltammetry and chronoamperometry) alone offers a limited picture of the enzyme–electrode interface.How many enzymes are loaded onto an electrode? In which orientation(s) are they bound? What fraction is active, and are single or multilayers formed? Does this static picture change over time, applied voltage, or chemical environment? How does charge transfer through various intraprotein cofactors contribute to the overall performance and catalytic bias? What is the distribution of individual enzyme activities within an ensemble of active protein films? These are central questions for the understanding of the enzyme–electrode interface, and a multidisciplinary approach is required to deliver insightful answers.Complementing standard electrochemical experiments with an orthogonal set of techniques has recently allowed to provide a more complete picture of enzyme–electrode systems. Within this framework, we first discuss a brief history of achievements and challenges in enzyme electrochemistry. We subsequently describe how the aforementioned challenges can be overcome by applying advanced electrochemical techniques, quartz-crystal microbalance measurements, and spectroscopic, namely, resonance Raman and infrared, analysis. For example, rotating ring disk electrochemistry permits the simultaneous determination of reaction kinetics and quantification of generated products. In addition, recording changes in frequency and dissipation in a quartz crystal microbalance allows to shed light into enzyme loading, relative orientation, clustering, and denaturation at the electrode surface. Resonance Raman spectroscopy yields information on ligation and redox state of enzyme cofactors, whereas infrared spectroscopy provides insights into active site states and the protein secondary and tertiary structure. The development of these emerging methods for the analysis of the enzyme–electrode interface is the primary focus of this Account. We also take a critical look at the remaining gaps in our understanding and challenges lying ahead toward attaining a complete mechanistic picture of the enzyme–electrode interface.
Highlights
The study of enzymes enhances our knowledge of catalysis and biology while leading to applications in medicine, sensing, energy, and more
The electrochemistry of proteinmodified electrodes known as protein film electrochemistry (PFE) has served as a powerful tool for probing the thermodynamic and kinetic properties of redox-active proteins and enzymes since the second half of the 20th century.[1−3] The topic is mature, and several excellent reviews have been published describing the information available from immobilized enzymes and routine PFE experiments.[4−7] The unique insights provided by PFE are largely enabled by direct interfacial electron transfer between the electrode surface and the enzyme cofactors, including its active site
The results indicated that the enzyme conserved its structure upon adsorption and was in excellent electronic contact to the electrode
Summary
The study of enzymes enhances our knowledge of catalysis and biology while leading to applications in medicine, sensing, energy, and more. SERR spectroscopic investigations of the non-heme DNA-repairing enzyme endonuclease III revealed redox activity of the [4Fe− 4S] cluster in the absence of DNA-binding.[65] electron transfer from the electrode to a membrane-bound [NiFe] H2ase heterotrimer was demonstrated to predominantly occur through the enzyme’s HoxGK subunit rather than the terminal HoxZ subunit on the basis of the SERRderived reduction rate of the heme b cofactors in HoxZ.[66] Important to these studies is that SERR spectroscopy allows for selectively monitoring of protein cofactors even at very low surface coverages. Article copy has been applied to monitor formation of a hybrid complex of PSI and a H2ase utilized toward photochemical H2 generation.[72]
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