Construction of Uniform Monolayer- and Orientation-Tunable Enzyme Electrode by a Synthetic Glucose Dehydrogenase without Electron-Transfer Subunit via Optimized Site-Specific Gold-Binding Peptide Capable of Direct Electron Transfer

Yoo Seok Lee; Seungwoo Baek; Hyeryeong Lee; Stacy Simai Reginald; Yeongeun Kim; Hyunsoo Kang; In-Geol Choi; In Seop Chang

doi:10.1021/acsami.8b08876

Construction of Uniform Monolayer- and Orientation-Tunable Enzyme Electrode by a Synthetic Glucose Dehydrogenase without Electron-Transfer Subunit via Optimized Site-Specific Gold-Binding Peptide Capable of Direct Electron Transfer

ACS Appl Mater Interfaces. 2018 Aug 29;10(34):28615-28626. doi: 10.1021/acsami.8b08876. Epub 2018 Aug 15.

Authors

Yoo Seok Lee¹, Seungwoo Baek², Hyeryeong Lee¹, Stacy Simai Reginald¹, Yeongeun Kim¹, Hyunsoo Kang¹, In-Geol Choi², In Seop Chang¹

Affiliations

¹ School of Earth Sciences and Environmental Engineering , Gwangju Institute of Science and Technology (GIST) , 123 Cheomdan-gwagiro , Buk-gu, Gwangju 61005 , Republic of Korea.
² Department of Biotechnology, College of Life Sciences and Biotechnology , Korea University , Seoul 02841 , Republic of Korea.

PMID: 30067023
DOI: 10.1021/acsami.8b08876

Abstract

Direct electron transfer (DET) between enzymes and electrodes is a key issue for practical use of bioelectrocatalytic devices as a bioenergy process, such as enzymatic electrosynthesis, biosensors, and enzyme biofuel cells. To date, based on the DET of bioelectrocatalysis, less than 1% of the calculated theoretical current was transferred to final electron acceptor due to energy loss at enzyme-electrode interface. This study describes the design and construction of a synthetic glucose dehydrogenase (GDH; α and γ subunits) combined with a gold-binding peptide at its amino or carboxy terminus for direct contact between enzyme and electrode. The fused gold-binding peptide facilitated stable immobilization of GDH and constructed uniform monolayer of GDH onto a Au electrode. Depending on the fused site of binding peptide to the enzyme complex, nine combinations of recombinant GDH proteins on the electrode show significantly different direct electron-transfer efficiency across the enzyme-electrode interface. The fusion of site-specific binding peptide to the catalytic subunit (α subunit, carboxy terminus) of the enzyme complex enabled apparent direct electron transfer (DET) across the enzyme-electrode interface even in the absence of the electron-transfer subunit (i.e., β subunit having cytochrome domain). The catalytic glucose oxidation current at an onset potential of ca. (-)0.46 V vs Ag/AgCl was associated with the appearance of an flavin adenine dinucleotide (FAD)/FADH₂ redox wave and a stabilized bioelectrocatalytic current of more than 100 μA, determined from chronoamperometric analysis. Electron recovery was 7.64%, and the catalytic current generation was 249 μA per GDH enzyme loading unit (U), several orders of magnitude higher than the values reported previously. These observations corroborated that the last electron donor facing to electrode was controlled to be in close proximity without electron-transfer intermediates and the native affinity for glucose was preserved. The design and construction of the site-specific "sticky-ended" proteins without loss of catalytic activity could be applied to other redox enzymes having a buried active site.

Keywords: direct electron transfer; electron tunneling distance; gold-binding peptide; orientation; synthetic glucose dehydrogenase.

MeSH terms

Biosensing Techniques
Electrodes*
Electron Transport
Electrons
Enzymes, Immobilized
Glucose
Glucose 1-Dehydrogenase
Gold
Peptides

Substances

Enzymes, Immobilized
Peptides
Gold
Glucose 1-Dehydrogenase
Glucose