How to engineer glucose oxidase for mediated electron transfer

Erik Arango Gutierrez; Anne-Maria Wallraf; Alexandra Balaceanu; Marco Bocola; Mehdi D Davari; Thomas Meier; Hartmut Duefel; Ulrich Schwaneberg

doi:10.1002/bit.26785

How to engineer glucose oxidase for mediated electron transfer

Biotechnol Bioeng. 2018 Oct;115(10):2405-2415. doi: 10.1002/bit.26785. Epub 2018 Jul 25.

Authors

Erik Arango Gutierrez¹, Anne-Maria Wallraf¹, Alexandra Balaceanu^{1

2

3}, Marco Bocola¹, Mehdi D Davari¹, Thomas Meier⁴, Hartmut Duefel⁴, Ulrich Schwaneberg^{1

5}

Affiliations

¹ Lehrstuhl für Biotechnologie, RWTH Aachen University, Aachen, Germany.
² The Barcelona Institute of Science and Technology, Institute for Research in Biomedicine (IRB Barcelona), Barcelona, Spain.
³ Joint BSC-IRB Research Program in Computational Biology, Barcelona, Spain.
⁴ Roche Diagnostics GmbH, Enzyme Technology DXREAF.6164, Penzberg, Germany.
⁵ DWI an der RWTH Aachen e.V., Aachen, Germany.

PMID: 29959868
DOI: 10.1002/bit.26785

Abstract

Glucose oxidase (GOx) is of high industrial interest for glucose sensing because of its high β-d-glucose specificity. The efficient and specific electrochemical communication between the redox center and electrodes is crucial to ensure accurate glucose determination. The efficiency of the electron transfer rates (ETR) with GOx, together with quinone diamine based mediators, is low and differs even among mediator derivatives. To design optimized enzyme-mediator couples and to describe a mediator binding model, a joint experimental and computational study was performed based on an oxygen-independent GOx variant V7 and two quinone diimine based electron mediators (QDM-1 and QDM-2), which differ in polarity and size, and ferrocenemethanol (FM). A site saturation library at position 414 was screened with all three mediators and yielded four beneficial substitutions Tyr, Met, Leu, and Val. The variants showed increased mediator activity for the more polar QDM-2 with a simultaneously decreased activity for the less polar and smaller QDM-1 and for FM. The variant GOx V7-I414Y exhibited the biggest change for the quinone diimine derivatives compared with V7 (QDM-1: 55.9 U/mg V7, 33.2 U/mg V7-I414Y; QDM-2: 2.7 U/mg V7, 12.9 U/mg V7-I414Y). Theoretical ETR calculated based on the Marcus theory were in good agreement with the experimental results. Molecular docking studies revealed a preferable binding of the two QD mediators directly in the active site, 3.5 Å away from the N5 atom of the flavin adenine dinucleotide (FAD) and in direct vicinity to position 414. In summary, position 414 in the active site was identified to modulate the electron shuttling from the FAD of the GOx to small water-soluble mediators dependent on the polarity and size of residue 414 and on the polarity and size of the mediator. The presented mediator binding model offers a promising possibility for the design of optimized enzyme-mediator couples.

Keywords: Marcus theory; directed evolution; electron mediators; glucose oxidase (GOx); molecular docking; protein engineering.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Benzoquinones / chemistry*
Catalytic Domain
Electron Transport
Glucose / chemistry*
Glucose Oxidase / chemistry*
Glucose Oxidase / genetics
Molecular Docking Simulation*
Oxygen / chemistry*
Protein Engineering*
Recombinant Proteins / chemistry
Recombinant Proteins / genetics

Substances

Benzoquinones
Recombinant Proteins
quinone
Glucose Oxidase
Glucose
Oxygen