AI Article Synopsis
- Enzyme action is characterized by enantioselective bond making and breaking, but changing this selectivity often requires complex work with mutant libraries.
- This study shows that modifying one key area of the enzyme pyruvate decarboxylase allows for the production of both enantiomers of important pharmaceutical precursors like acetoin and phenylacetylcarbinol, even starting from a non-selective wild-type version.
- The research employs protein crystallography to explain how selectivity is controlled and emphasizes the effectiveness of targeted protein design for improving and changing enzyme selectivity through focused exploration of a single active site.
Article Abstract
Enantioselective bond making and breaking is a hallmark of enzyme action, yet switching the enantioselectivity of the reaction is a difficult undertaking, and typically requires extensive screening of mutant libraries and multiple mutations. Here, we demonstrate that mutational diversification of a single catalytic hot spot in the enzyme pyruvate decarboxylase gives access to both enantiomers of acyloins acetoin and phenylacetylcarbinol, important pharmaceutical precursors, in the case of acetoin even starting from the unselective wild-type protein. Protein crystallography was used to rationalize these findings and to propose a mechanistic model of how enantioselectivity is controlled. In a broader context, our studies highlight the efficiency of mechanism-inspired and structure-guided rational protein design for enhancing and switching enantioselectivity of enzymatic reactions, by systematically exploring the biocatalytic potential of a single hot spot.
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| http://dx.doi.org/10.1002/cbic.201500529 | DOI Listing |
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