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Unraveling the kinetic diversity of microbial 3-dehydroquinate dehydratases of shikimate pathway

机译:阐明sh草酸途径中微生物3-脱氢奎宁酸脱水酶的动力学多样性

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摘要

3-Dehydroquinate dehydratase (DHQase) catalyzes the conversion of 3-dehydroquinic acid to 3-dehydroshikimic acid of the shikimate pathway. In this study, 3180 prokaryotic genomes were examined and 459 DHQase sequences were retrieved. Based on sequence analysis and their original hosts, 38 DHQase genes were selected for chemical synthesis. The selected DHQases were translated into new DNA sequences according to the genetic codon usage bias by both Escherichia coli and Corynebacterium glutamicum. The new DNA sequences were customized for synthetic biological applications by adding Biobrick adapters at both ends and by removal of any related restriction endonuclease sites. The customized DHQase genes were successfully expressed in E. coli, and functional DHQases were obtained. Kinetic parameters of Km, kcat, and Vmax of DHQases were determined with a newly established high-throughput method for DHQase activity assay. Results showed that DHQases possessed broad strength of substrate affinities and catalytic capacities. In addition to the DHQase kinetic diversities, this study generated a DHQase library with known catalytic constants that could be applied to design artificial modules of shikimate pathway for metabolic engineering and synthetic biology.
机译:3-脱氢奎宁酸脱水酶(DHQase)催化the草酸酯途径的3-脱氢奎宁酸转化为3-脱氢shi草酸。在这项研究中,检查了3180个原核基因组,并检索了459个DHQase序列。根据序列分析及其原始宿主,选择了38个DHQase基因进行化学合成。根据大肠杆菌和谷氨酸棒杆菌的遗传密码子使用偏好,将选定的DHQ酶翻译成新的DNA序列。通过在两端添加Biobrick衔接子并去除任何相关的限制性核酸内切酶位点,可以为合成生物学应用定制新的DNA序列。定制的DHQase基因在大肠杆菌中成功表达,并获得功能性DHQase。 DHQase的Km,kcat和Vmax的动力学参数通过新建立的用于DHQase活性测定的高通量方法确定。结果表明,DHQases具有广泛的底物亲和力和催化能力。除了DHQase动力学多样性外,本研究还产生了具有已知催化常数的DHQase文库,可用于设计sh草酸途径的人工模块,用于代谢工程和合成生物学。

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