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揭示肺炎克雷伯菌的毒力:构建用于耐药病原体转录分析的广泛宿主范围生物发光报告载体

Shedding light on Klebsiella pneumoniae virulence: Engineering of broad host range bioluminescence reporter vectors for transcriptional analysis in drug resistant pathogens.

作者信息

Chandrashekarappa Dakshayini G, Van Allen Mia E, Bina X Renee, Bina James E

机构信息

University of Pittsburgh School of Medicine, Department of Microbiology and Molecular Genetics, Pittsburgh, PA 15219, United States of America.

University of Pittsburgh School of Medicine, Department of Microbiology and Molecular Genetics, Pittsburgh, PA 15219, United States of America.

出版信息

Plasmid. 2024 Sep-Nov;131-132:102734. doi: 10.1016/j.plasmid.2024.102734. Epub 2024 Oct 29.

Abstract

In this work, we report the construction of four bacterial luciferase-based promoter probe vectors with an expanded set of selectable markers, designed to facilitate their use in antibiotic-resistant bacteria. These vectors contain the low-copy-number, broad-host-range pBBR origin of replication and an origin of transfer, allowing efficient conjugative transformation into various bacterial genera. The broad host range origin also enables their use in bacterial strains that harbor other plasmids, as the pBBR origin is compatible with a wide variety of other plasmid replication systems. The utility of these vectors was demonstrated by quantifying capsule gene expression in both classical and hypervirulent Klebsiella pneumoniae strains lacking tolC, which encodes the outer membrane pore protein for tripartite transport systems. Our results revealed that the tolC mutation reduced capsule gene expression, highlighting a critical role for tolC in K. pneumoniae pathobiology and the utility of bioluminescence for studying gene expression in real time. These new vectors provide a flexible platform for circumventing antibiotic resistance phenotypes and studying gene expression across diverse bacterial species, including strains containing additional plasmids.

摘要

在本研究中,我们报告了四种基于细菌荧光素酶的启动子探针载体的构建,这些载体具有扩展的选择标记集,旨在便于在抗生素抗性细菌中使用。这些载体包含低拷贝数、广宿主范围的pBBR复制起点和转移起点,能够高效接合转化到各种细菌属中。广宿主范围的复制起点还使它们能够用于携带其他质粒的细菌菌株,因为pBBR复制起点与多种其他质粒复制系统兼容。通过量化缺乏tolC(编码三重运输系统外膜孔蛋白)的经典和高毒力肺炎克雷伯菌菌株中的荚膜基因表达,证明了这些载体的实用性。我们的结果表明,tolC突变降低了荚膜基因表达,突出了tolC在肺炎克雷伯菌病理生物学中的关键作用以及生物发光在实时研究基因表达中的实用性。这些新载体为规避抗生素抗性表型和研究包括含有额外质粒的菌株在内的各种细菌物种中的基因表达提供了一个灵活的平台。

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