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作 者:Yufeng Liu Mingzhu Hao Zhemin Zhou Zhongmei Liu
机构地区:[1]School of Biotechnology,Jiangnan University,Wuxi,Jiangsu,China
出 处:《Systems Microbiology and Biomanufacturing》2022年第1期157-164,共8页系统微生物学与生物制造(英文)
基 金:This work was supported by National Key R&D Program of China(2017YFE0129600);the National Natural Science Foundation of China(21878125);the Priority Academic Program Development of Jiangsu Higher Education Institutions,the 111 Project(No.111-2-06).
摘 要:L-Aspartateβ-decarboxylase from Acinetobacter radioresistens(ArASD)has been modifed to convert 3-methylaspartic acid into 2-aminobutyric acid,which activated a novel process for biosynthesis of 2-aminobutyric acid.However,the process is limited by the low activity of the ArASD.Here,the activity of ArASD was signifcantly improved by modifcation based on sequence alignment and structural analysis.The 38th residue of ArASD is speculated to be the key residue for regulating the conformation of the internal aldimine,and site-directed mutagenesis on R38 residue was carried out.A variant,K18A/R38K/V287I,with 2.2 times higher specifc activity was isolated.Molecular dynamics simulation indicated that the torsion angle of the imine bond of the variant decreased,which was benefcial to the protonation of the internal aldimine and the increase in the initial energy of the enzyme.Therefore,the energy barrier of the transition state was reduced,resulting in improved catalytic activity toward 3-methylaspartic acid.These results provide a reference and a new point of view for enzyme modifcation by increasing the energy of the initial state.
关 键 词:L-Aspartateβ-decarboxylase 3-Methylasparic acid The internal aldimine Enzyme engineering Molecular dynamics simulation
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