Straightforward Regeneration of Reduced Flavin Adenine Dinucleotide Required for Enzymatic Tryptophan Halogenation

Journal article (2019)

Authors

M.B.M. Ismail Helwan University, Ain Helwan, Bielefeld University
Lea Schroeder Bielefeld University
Marcel Frese Bielefeld University
Tilman Kottke Bielefeld University
F. Hollmann BT/Biocatalysis - AS
C.E. Paul Wageningen University & Research, BT/Biocatalysis - AS
Norbert Sewald Bielefeld University
Research Group
BT/Biocatalysis (AS) (TU Delft)
Copyright: © 2019 M.B.M. Ismail, Lea Schroeder, Marcel Frese, Tilman Kottke, F. Hollmann, C.E. Paul, Norbert Sewald
DOI: https://doi.org/10.1021/acscatal.8b04500
Hydride transfer Enzymatic cofactor regeneration FADH Flavin-dependent halogenases NADH mimics Regioselective chlorination
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Published Date

2019

Language

English

Faculty

Applied Sciences

Department

BT/Biotechnologie

Research Group

BT/Biocatalysis

Abstract

Flavin-dependent halogenases are known to regioselectively introduce halide substituents into aromatic moieties, for example, the indole ring of tryptophan. The process requires halide salts and oxygen instead of molecular halogen in the chemical halogenation. However, the reduced cofactor flavin adenine dinucleotide (FADH2) has to be regenerated using a flavin reductase. Consequently, coupled biocatalytic steps are usually applied for cofactor regeneration. Nicotinamide adenine dinucleotide (NADH) mimics can be employed stoichiometrically to replace enzymatic cofactor regeneration in biocatalytic halogenation. Chlorination of l-tryptophan is successfully performed using such NADH mimics. The efficiency of this approach has been compared to the previously established enzymatic regeneration system using the two auxiliary enzymes flavin reductase (PrnF) and alcohol dehydrogenase (ADH). The reaction rates of some of the tested mimics were found to exceed that of the enzymatic system. Continuous enzymatic halogenation reaction for reaction scale-up is also possible.