Enzyme-specific activation versus leaving group ability

Roseri J A C de Beer; Berry Bögels; Gijs Schaftenaar; Barbara Zarzycka; Peter J L M Quaedflieg; Floris L van Delft; Sander B Nabuurs; Floris P J T Rutjes

doi:10.1002/cbic.201200227

Enzyme-specific activation versus leaving group ability

Chembiochem. 2012 Aug 13;13(12):1785-90. doi: 10.1002/cbic.201200227. Epub 2012 Jul 23.

Authors

Roseri J A C de Beer¹, Berry Bögels, Gijs Schaftenaar, Barbara Zarzycka, Peter J L M Quaedflieg, Floris L van Delft, Sander B Nabuurs, Floris P J T Rutjes

Affiliation

¹ Institute for Molecules and Materials, Radboud University Nijmegen, Heyendaalseweg 135, 6525 AJ Nijmegen, The Netherlands.

Abstract

Enzyme-specific activation and the substrate mimetics strategy are effective ways to circumvent the limited substrate recognition often encountered in protease-catalyzed peptide synthesis. A key structural element in both approaches is the guanidinophenyl (OGp) ester, which enables important interactions for affinity and recognition by the enzyme--at least, this is usually the explanation given for its successful application. In this study we show that leaving group ability is of equal or even greater importance. To this end we used both experimental and computational methods: 1) synthesis of close analogues of OGp, and their evaluation in a dipeptide synthesis assay with trypsin, 2) molecular docking studies to provide insights into the binding mode, and 3) ab initio calculations to evaluate their electronic properties.

Publication types

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

MeSH terms

Biocatalysis
Biological Assay
Dipeptides / chemical synthesis*
Enzyme Activation
Esters
Hydrogen Bonding
Hydrolysis
Models, Molecular
Molecular Mimicry
Protein Conformation
Quantum Theory
Solutions
Substrate Specificity
Trypsin / chemistry*
Trypsin / metabolism

Substances

Dipeptides
Esters
Solutions
Trypsin