Overproduction and characterization of a recombinant D-amino acid oxidase from Arthrobacter protophormiae

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作者
Birgit Geueke
Andrea Weckbecker
Werner Hummel
机构
[1] Heinrich Heine University Düsseldorf,Institute of Molecular Enzyme Technology
[2] Research Centre Jülich,undefined
[3] Swiss Federal Institute of Aquatic Science (Eawag),undefined
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Flavin Adenine Dinucleotide; Flavin Adenine Dinucleotide; High Cell Density Fermentation; Isoelectric Focussing; Universal GenomeWalker;
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摘要
A screening of soil samples for d-amino acid oxidase (d-AAO) activity led to the isolation and identification of the gram-positive bacterium Arthrobacter protophormiae. After purification of the wild-type d-AAO, the gene sequence was determined and designated dao. An alignment of the deduced primary structure with eukaryotic d-AAOs and d-aspartate oxidases showed that the d-AAO from A. protophormiae contains five of six conserved regions; the C-terminal type 1 peroxisomal targeting signal that is typical for d-AAOs from eukaryotic origin is missing. The dao gene was cloned and expressed in Escherichia coli. The purified recombinant d-AAO had a specific activity of 180 U mg protein−1 for d-methionine and was slightly inhibited in the presence of l-methionine. Mainly, basic and hydrophobic d-amino acids were oxidized by the strictly enantioselective enzyme. After a high cell density fermentation, 2.29 × 106 U of d-AAO were obtained from 15 l of fermentation broth.
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页码:1240 / 1247
页数:7
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