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鉴定在巨噬细胞中复制存在缺陷的基于希马尔1转座子的土拉弗朗西斯菌突变体。

Identification of Francisella tularensis Himar1-based transposon mutants defective for replication in macrophages.

作者信息

Maier Tamara M, Casey Monika S, Becker Rachel H, Dorsey Caleb W, Glass Elizabeth M, Maltsev Natalia, Zahrt Thomas C, Frank Dara W

机构信息

Department of Microbiology and Molecular Genetics, Medical College of Wisconsin, 8701 Watertown Plank Road, Milwaukee, WI 53226, USA.

出版信息

Infect Immun. 2007 Nov;75(11):5376-89. doi: 10.1128/IAI.00238-07. Epub 2007 Aug 6.

Abstract

Francisella tularensis, the etiologic agent of tularemia in humans, is a potential biological threat due to its low infectious dose and multiple routes of entry. F. tularensis replicates within several cell types, eventually causing cell death by inducing apoptosis. In this study, a modified Himar1 transposon (HimarFT) was used to mutagenize F. tularensis LVS. Approximately 7,000 Km(r) clones were screened using J774A.1 macrophages for reduction in cytopathogenicity based on retention of the cell monolayer. A total of 441 candidates with significant host cell retention compared to the parent were identified following screening in a high-throughput format. Retesting at a defined multiplicity of infection followed by in vitro growth analyses resulted in identification of approximately 70 candidates representing 26 unique loci involved in macrophage replication and/or cytotoxicity. Mutants carrying insertions in seven hypothetical genes were screened in a mouse model of infection, and all strains tested appeared to be attenuated, which validated the initial in vitro results obtained with cultured macrophages. Complementation and reverse transcription-PCR experiments suggested that the expression of genes adjacent to the HimarFT insertion may be affected depending on the orientation of the constitutive groEL promoter region used to ensure transcription of the selective marker in the transposon. A hypothetical gene, FTL_0706, postulated to be important for lipopolysaccharide biosynthesis, was confirmed to be a gene involved in O-antigen expression in F. tularensis LVS and Schu S4. These and other studies demonstrate that therapeutic targets, vaccine candidates, or virulence-related genes may be discovered utilizing classical genetic approaches in Francisella.

摘要

土拉弗朗西斯菌是人类兔热病的病原体,因其感染剂量低且有多种侵入途径,是一种潜在的生物威胁。土拉弗朗西斯菌在多种细胞类型中复制,最终通过诱导凋亡导致细胞死亡。在本研究中,一种改良的Himar1转座子(HimarFT)被用于诱变土拉弗朗西斯菌LVS。基于细胞单层的保留情况,使用J774A.1巨噬细胞筛选了约7000个卡那霉素抗性(Km(r))克隆,以降低细胞致病性。在高通量筛选后,共鉴定出441个与亲本相比具有显著宿主细胞保留的候选菌株。在确定的感染复数下重新测试,随后进行体外生长分析,结果鉴定出约70个候选菌株,代表26个参与巨噬细胞复制和/或细胞毒性的独特基因座。在感染小鼠模型中筛选了在7个假定基因中携带插入突变的突变体,所有测试菌株似乎都减毒了,这验证了最初在培养巨噬细胞上获得的体外结果。互补和逆转录PCR实验表明,取决于用于确保转座子中选择标记转录的组成型groEL启动子区域的方向,与HimarFT插入相邻的基因表达可能会受到影响。一个假定对脂多糖生物合成很重要的假定基因FTL_0706,被证实是土拉弗朗西斯菌LVS和Schu S4中参与O抗原表达的基因。这些研究及其他研究表明,利用经典遗传学方法可在弗朗西斯菌中发现治疗靶点、候选疫苗或毒力相关基因。

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