首页> 外文期刊>FEMS Microbiology Letters >CONSTRUCTION AND USE OF A NEW VECTOR/TRANSPOSON, PLBT--MINI-TN1O-LAC-KAN, TO IDENTIFY ENVIRONMENTALLY RESPONSIVE GENES IN A MARINE BACTERIUM
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CONSTRUCTION AND USE OF A NEW VECTOR/TRANSPOSON, PLBT--MINI-TN1O-LAC-KAN, TO IDENTIFY ENVIRONMENTALLY RESPONSIVE GENES IN A MARINE BACTERIUM

机译:新型载体/转座子PLBT-MINI-TN1O-LAC-KAN的构建和使用,以鉴定海洋细菌中的环境敏感基因

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摘要

The previously described pLOFKm transposon delivery plasmid (J. Bacteriol. (1990) 172, 6557-6567) was engineered such that a promoterless lacZ gene was cloned within the transposon cassette, generating the vector pLBT. Using pLBT, stable insertion mutations were generated at high frequencies in Vibrio sp. S141 and Pseudomonas sp. S91, and the interrupted genes could be monitored for their pattern of regulation. Genetic screens isolated mutants defective in a variety of activities. We describe the construction and use of pLBT as a tool for reporter gene mutant analysis in bacteria other than well-characterized laboratory strains. [References: 24]
机译:对先前描述的pLOFKm转座子递送质粒(J.Bacteriol。(1990)172,6557-6567)进行改造,使得无启动子的lacZ基因被克隆到转座子盒中,从而产生载体pLBT。使用pLBT,在弧菌中高频率产生稳定的插入突变。 S141和假单胞菌属。 S91,并可以监测中断的基因的调控方式。遗传筛选分离出在各种活动中有缺陷的突变体。我们描述pLBT的构建和使用,作为除特征明确的实验室菌株以外的细菌中的报告基因突变分析工具。 [参考:24]

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