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首页> 外文期刊>Biotechnology and Bioengineering >Engineering of a Butyraldehyde Dehydrogenase of Clostridium saccharoperbutylacetonicum to Fit an Engineered 1,4-Butanediol Pathway in Escherichia coli
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Engineering of a Butyraldehyde Dehydrogenase of Clostridium saccharoperbutylacetonicum to Fit an Engineered 1,4-Butanediol Pathway in Escherichia coli

机译:糖化梭菌梭状芽孢杆菌丁醛脱氢酶的工程设计,以适合大肠杆菌中的工程化1,4-丁二醇途径。

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1,4-Butanediol (1,4-BDO) is currently produced from succinate via six enzymatic reactions in an engineered Escherichia coli strain. Butyraldehyde dehydrogenase (Bld) and butanol dehydrogenase of Clostridium saccharoperbutylacetonicum were selected based on their activities of catalyzing the final two reactions in the 1,4-BDO pathway. To fit Bld into the non-natural 1,4-BDO pathway, we engineered it through random mutagenesis. Five Bld mutants were then isolated using a colorimetric Schiff 's reagent-based method. Subsequent site-directed mutagenesis of Bld generated the two best Bld mutants, L273I and L273T, which produced 1,4-BDO titers fourfold greater than those of wild-type Bld. The enhanced 1,4-BDO titers obtained using L273I and L273T clearly correlated with their enhanced activities, which were caused by amino acid mutations at position 273 of Bld. The highest titer of 1,4-BDO (660±40 mg/L) was obtained in a knock-out E. coli strain [DldhA DpflB DadhE DlpdA::K. lpd(E354K) Dmdh DarcA gltA(R164L)] coexpressing Bld273T+Bdh.
机译:目前,在工程化的大肠杆菌菌株中,琥珀酸通过6种酶促反应生成琥珀酸1,4-丁二醇(1,4-BDO)。糖基丙酮丁醇梭状芽孢杆菌的丁醛脱氢酶(Bld)和丁醇脱氢酶是基于它们催化1,4-BDO途径中最后两个反应的活性而选择的。为了使Bld适应非天然的1,4-BDO途径,我们通过随机诱变对其进行了工程改造。然后使用比色Schiff试剂为基础的方法分离出五个Bld突变体。随后的Bld的定点诱变产生了两个最佳的Bld突变体L273I和L273T,它们产生的1,4-BDO滴度比野生型Bld高四倍。使用L273I和L273T获得的增强的1,4-BDO滴度与它们增强的活性明显相关,这是由Bld的273位氨基酸突变引起的。在敲除的大肠杆菌菌株[DldhA DpflB DadhE DlpdA :: K]中获得最高滴度的1,4-BDO(660±40 mg / L)。 lpd(E354K)Dmdh DarcA gltA(R164L)]共表达Bld273T + Bdh。

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