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Use of a Novel Escherichia coli-Leuconostoc Shuttle Vector for Metabolic Engineering of Leuconostoc citreum To Overproduce d-Lactate

机译:一种新型的大肠杆菌-Leuconostoc穿梭载体在柠檬亮氨酸代谢工程中过量生产d-乳酸的应用

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Determination of the complete nucleotide sequence of a cryptic plasmid, pMBLT00, from Leuconostoc mesenteroides subsp. mesenteroides KCTC13302 revealed that it contains 20,721 bp, a G+C content of 38.7%, and 18 open reading frames. Comparative sequence and mung been nuclease analyses of pMBLT00 showed that pMBLT00 replicates via the theta replication mechanism. A new, stable Escherichia coli-Leuconostoc shuttle vector, pMBLT02, which was constructed from a theta-replicating pMBLT00 replicon and an erythromycin resistance gene of pE194, was successfully introduced into Leuconostoc , Lactococcus lactis , and Pediococcus . This shuttle vector was used to engineer Leuconostoc citreum 95 to overproduce d-lactate. The L. citreum 95 strain engineered using plasmid pMBLT02, which overexpresses d-lactate dehydrogenase, exhibited enhanced production of optically pure d-lactate (61 g/liter, which is 6 times greater than the amount produced by the control strain) when cultured in a reactor supplemented with 140 g/liter glucose. Therefore, the shuttle vector pMBLT02 can serve as a useful and stable plasmid vector for further development of a d-lactate overproduction system in other Leuconostoc strains and Lactococcus lactis .
机译:确定来自肠膜液明暗亚种的隐性质粒pMBLT00的完整核苷酸序列。 mesenteroides KCTC13302含有20,721 bp,G + C含量为38.7%,有18个开放阅读框。 pMBLT00的比较序列和绿色核酸酶分析表明pMBLT00通过theta复制机制复制。由θ复制型pMBLT00复制子和pE194的红霉素抗性基因构建的新的稳定的大肠杆菌-Leuconostoc穿梭载体pMBLT02已成功地引入了Leuconostoc,乳酸乳球菌和Pediococcus。该穿梭载体被用于改造柠檬酸亮丙三醇95以过量产生d-乳酸。用质粒pMBLT02改造的柠檬酸乳酸杆菌95菌株在培养时,过量表达d-乳酸脱氢酶,其光学纯d-乳酸的产量提高了(61 g /升,比对照菌株的产量高6倍)。补充有140克/升葡萄糖的反应器。因此,穿梭载体pMBLT02可作为有用的和稳定的质粒载体,用于进一步开发其他乳突球菌菌株和乳酸乳球菌中的d-乳酸过量生产系统。

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