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Functional identification of the fatty acid reductase components encoded in the luminescence operon of Vibrio fischeri.

机译:费氏弧菌发光操纵子中编码的脂肪酸还原酶成分的功能鉴定。

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摘要

A clone of DNA, obtained from the luminescent bacterium Vibrio fischeri ATCC 7744 and inserted into pBR322, was found to express luminescence in Escherichia coli. Polypeptides involved in biosynthesis of the fatty aldehyde substrate for the light reaction were identified by fatty acid acylation of proteins synthesized in E. coli from the recombinant plasmid. The cloned region was similar to that reported for the V. fischeri MJ1 luminescence system (Engebrecht et al., Cell 32:773-781), except for some differences in endonuclease restriction sites and the requirement of a lower temperature for the expression of light in our cloned system. Fatty acid reductase activity could be detected in extracts of E. coli harboring the recombinant plasmid but not in extracts of the parental V. fischeri strain. Using in vivo labeling with [3H]tetradecanoic acid, we showed that the acylated polypeptides synthesized in the cloned system corresponded to the labeled polypeptides in V. fischeri (34, 42, and 54 kilodaltons) and that they could only be detected after induction of luminescence. These results provide direct evidence that the genes coding for the fatty acid reductase polypeptides are an integral part of the luminescence operon in the V. fischeri luminescence system.
机译:发现从发光细菌费氏弧菌ATCC 7744获得并插入pBR322的DNA克隆在大肠杆菌中表达发光。通过重组质粒在大肠杆菌中合成的蛋白质的脂肪酸酰化作用,可以鉴定参与光醛反应的脂肪醛底物生物合成的多肽。克隆的区域与费氏弧菌MJ1发光系统报道的区域相似(Engebrecht等,Cell 32:773-781),除了核酸内切酶限制位点的某些差异以及需要较低的温度来表达光在我们的克隆系统中。可以在带有重组质粒的大肠杆菌提取物中检测到脂肪酸还原酶的活性,而在亲代费氏弧菌菌株的提取物中则不能检测到。使用[3H]十四烷酸进行体内标记,我们显示在克隆的系统中合成的酰化多肽对应于费氏弧菌(34、42和54道尔顿)中的标记多肽,并且只有在诱导后才能检测到它们。发光。这些结果提供直接证据,证明脂肪酸还原酶多肽的编码基因是费氏弧菌发光系统中发光操纵子的组成部分。

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