Benzylic and aryl hydroxylations of m-xylene by o-xylene dioxygenase from Rhodococcus sp. strain DK17

被引:0
作者
Dockyu Kim
Ki Young Choi
Miyoun Yoo
Jung Nam Choi
Choong Hwan Lee
Gerben J. Zylstra
Beom Sik Kang
Eungbin Kim
机构
[1] Korea Polar Research Institute,Polar BioCenter
[2] KORDI,Department of Biology
[3] Yonsei University,Division of Life Bioscience and Biotechnology, IBST
[4] Konkuk University,Biotechnology Center for Agriculture and the Environment
[5] Cook College,School of Life Science and Biotechnology
[6] Rutgers University,Department of Molecular Biology and Genetics
[7] Kyungpook National University,undefined
[8] Johns Hopkins University School of Medicine,undefined
来源
Applied Microbiology and Biotechnology | 2010年 / 86卷
关键词
-Xylene dioxygenase; Benzylic hydroxylation; effect;
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摘要
Escherichia coli cells expressing Rhodococcus DK17 o-xylene dioxygenase genes were used for bioconversion of m-xylene. Gas chromatography–mass spectrometry analysis of the oxidation products detected 3-methylbenzylalcohol and 2,4-dimethylphenol in the ratio 9:1. Molecular modeling suggests that o-xylene dioxygenase can hold xylene isomers at a kink region between α6 and α7 helices of the active site and α9 helix covers the substrates. m-Xylene is unlikely to locate at the active site with a methyl group facing the kink region because this configuration would not fit within the substrate-binding pocket. The m-xylene molecule can flip horizontally to expose the meta-position methyl group to the catalytic motif. In this configuration, 3-methylbenzylalcohol could be formed, presumably due to the meta effect. Alternatively, the m-xylene molecule can rotate counterclockwise, allowing the catalytic motif to hydroxylate at C-4 yielding 2,4-dimethylphenol. Site-directed mutagenesis combined with structural and functional analyses suggests that the alanine-218 and the aspartic acid-262 in the α7 and the α9 helices play an important role in positioning m-xylene, respectively.
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页码:1841 / 1847
页数:6
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