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Cloning of Escherichia coli lacZ and lacY Genes and Their Expression in Gluconobacter oxydans and Acetobacter liquefaciens

机译:大肠杆菌lacZ和lacY基因的克隆及其在氧化葡糖杆菌和液化醋杆菌中的表达

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摘要

An efficient transformation protocol for Gluconobacter oxydans and Acetobacter liquefaciens strains was developed by preparation of electrocompetent cells grown on yeast extract-ethanol medium. Plasmid pBBR122 was used as broad-host-range vector to clone the Escherichia coli lacZY genes in G. oxydans and A. liquefaciens. Although both lac genes were functionally expressed in both acetic acid bacteria, only a few transformants were able to grow on lactose. However, this ability strictly depended on the presence of a plasmid expressing both lac genes. Mutations in the plasmids and/or in the chromosome were excluded as the cause of growth ability on lactose.
机译:通过制备在酵母提取物-乙醇培养基上生长的电感受态细胞,开发了氧化葡糖杆菌和液化醋杆菌菌株的有效转化方案。质粒pBBR122被用作宽宿主范围的载体,以在氧化单歧杆菌和液化曲霉中克隆大肠杆菌lacZY基因。尽管两个lac基因均在两种乙酸细菌中功能性表达,但只有少数转化子能够在乳糖上生长。但是,这种能力严格取决于表达两个lac基因的质粒的存在。排除质粒和/或染色体中的突变作为乳糖生长能力的原因。

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