Modulating D-amino acid oxidase substrate specificity: production of an enzyme for analytical determination of all D-amino acids by directed evolution

doi:10.1093/protein/gzh064

PEDS Advance Access originally published online on August 13, 2004
Protein Engineering Design and Selection 2004 17(6):517-525; doi:10.1093/protein/gzh064

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Modulating D-amino acid oxidase substrate specificity: production of an enzyme for analytical determination of all D-amino acids by directed evolution

Silvia Sacchi, Elena Rosini, Gianluca Molla, Mirella S. Pilone and Loredano Pollegioni¹

Department of Biotechnology and Molecular Sciences, University of Insubria, via J.H. Dunant 3, 21100 Varese, Italy

¹ To whom correspondence should be addressed. E-mail: loredano.pollegioni{at}uninsubria.it

Recent research on the flavoenzyme D-amino acid oxidase fromRhodotorula gracilis (RgDAAO) has revealed new, intriguing propertiesof this catalyst and offers novel biotechnological applications.Among them, the reaction of RgDAAO has been exploited in theanalytical determination of the D-amino acid content in biologicalsamples. However, because the enzyme does not oxidize acidicD-amino acids, it cannot be used to detect the total amountof D-amino acids. We now present the results obtained usinga random mutagenesis approach to produce RgDAAO mutants witha broader substrate specificity. The libraries of RgDAAO mutantswere generated by error-prone PCR, expressed in BL21(DE3)pLysSEscherichia coli cells and screened for their ability to oxidizedifferent substrates by means of an activity assay. Five randommutants that have a ‘modified’ substrate specificity,more useful for the analytical determination of the entire contentof D-amino acids than wild-type RgDAAO, have been isolated.With the only exception of Y223 and G199, none of the effectiveamino acid substitutions lie in segments predicted to interactdirectly with the bound substrate. The substitutions appearto cluster on the protein surface: it would not have been possibleto predict that these substitutions would enhance DAAO activity.We can only conclude that these substitutions synergisticallygenerate small structural changes that affect the dynamics and/orstability of the protein in a way that enhances substrate bindingor subsequently catalytic turnover.

Received June 1, 2004; revised July 21, 2004; accepted August 4, 2004.

Edited by Dan Tawfik

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