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用于革兰氏阴性菌的新型广宿主范围lacZ转录融合载体pHRP309的构建与应用

Construction and use of a new broad-host-range lacZ transcriptional fusion vector, pHRP309, for gram- bacteria.

作者信息

Parales R E, Harwood C S

机构信息

Department of Microbiology, University of Iowa, Iowa City 52242.

出版信息

Gene. 1993 Oct 29;133(1):23-30. doi: 10.1016/0378-1119(93)90220-w.

Abstract

A new lacZ transcriptional fusion vector, pHRP309, based on the IncQ plasmid RSF1010, was constructed and shown to be easily mobilized into a variety of Gram- eubacteria. We also developed a two-step cloning procedure to facilitate the cloning of small promoter fragments into the fusion vector. A set of 'cohort' vectors was constructed which allowed directed cloning of fragments downstream from an omega streptomycin/spectinomycin-resistance cassette while maintaining multiple flanking restriction sites. The omega cassette provides a selectable antibiotic-resistance marker for cloning promoters into the fusion vector and makes mapping to determine fragment orientation unnecessary. The presence of the omega cassette also decreases background beta-galactosidase activity by decreasing readthrough transcription from plasmid sequences. The fusion vector carries a gentamicin-resistance-encoding gene as the selectable marker and can therefore be used in Tn5 (kanamycin-resistant) and Tn10 (tetracycline-resistant) mutant strains. Since pHRP309 is a member of the IncQ incompatibility group, it is compatible with IncP cloning vectors and can be used in strains carrying cloned regulatory genes. Using this system, we cloned the positively regulated Pseudomonas putida pcaI promoter and studied its regulation.

摘要

构建了一种基于IncQ质粒RSF1010的新型lacZ转录融合载体pHRP309,并证明其易于转移到多种革兰氏真细菌中。我们还开发了一种两步克隆程序,以促进将小的启动子片段克隆到融合载体中。构建了一组“群组”载体,这些载体允许将片段定向克隆到ω链霉素/壮观霉素抗性盒下游,同时保留多个侧翼限制性位点。ω盒为将启动子克隆到融合载体中提供了一个可选择的抗生素抗性标记,并且无需进行定位以确定片段方向。ω盒的存在还通过减少来自质粒序列的通读转录来降低背景β-半乳糖苷酶活性。融合载体携带一个编码庆大霉素抗性的基因作为选择标记,因此可用于Tn5(卡那霉素抗性)和Tn10(四环素抗性)突变菌株。由于pHRP309是IncQ不相容组的成员,它与IncP克隆载体兼容,可用于携带克隆调控基因的菌株。使用该系统,我们克隆了正调控的恶臭假单胞菌pcaI启动子并研究了其调控。

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