Enzyme Engineering Enables Inversion of Substrate Stereopreference of the Halogenase WelO5*
Moritz Voss (Zurich University of Applied Science (ZHAW))
Sean Hüppi (Zurich University of Applied Science (ZHAW), TU Delft - Applied Sciences)
Daniela Schaub (Zurich University of Applied Science (ZHAW))
Takahiro Hayashi (Mitsubishi Chemical Corporation, Yokohama, Zurich University of Applied Science (ZHAW))
Mathieu Ligibel (Novartis Pharma)
Emine Sager (Novartis Pharma)
Kirsten Schroer (Novartis Pharma)
Radka Snajdrova (Novartis Pharma)
Rebecca Buller (Zurich University of Applied Science (ZHAW))
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Abstract
Enzymatic late-stage diversification of small molecules has the potential to rapidly generate diversity in compound libraries dedicated to drug discovery. In this context, freestanding Fe(II)/α-ketoglutarate-dependent halogenases have raised particular interest as this enzyme family allows the otherwise difficult regio- and stereoselective halogenation of unactivated C(sp3)−H bonds. Here, we report the development of two engineered variants of the halogenase WelO5* for the racemic resolution of a mixture of stereoisomers generated in the synthesis of a bioactive martinelline-derived fragment. By screening a 3-site combinatorial variant library, we could identify two variants exhibiting exquisite substrate selectivity towards the desired enantiomers. Strikingly, the inversion of substrate stereopreference between the halogenase variants was achieved by varying only three residues in the active site. Protein crystallization and subsequent structure elucidation of the wildtype enzyme and a WelO5* variant shed light on the factors governing substrate acceptance and selectivity.
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