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弗朗西斯氏土拉菌在节肢动物媒介中增殖的分子基础。

Molecular bases of proliferation of Francisella tularensis in arthropod vectors.

机构信息

Department of Microbiology and Immunology, University of Louisville College of Medicine, Louisville, KY 40292, USA.

出版信息

Environ Microbiol. 2010 Sep;12(9):2587-612. doi: 10.1111/j.1462-2920.2010.02230.x. Epub 2010 May 7.

Abstract

Arthropod vectors are important vehicles for transmission of Francisella tularensis between mammals, but very little is known about the F. tularensis-arthropod vector interaction. Drosophila melanogaster has been recently developed as an arthropod vector model for F. tularensis. We have shown that intracellular trafficking of F. tularensis within human monocytes-derived macrophages and D. melanogaster-derived S2 cells is very similar. Within both evolutionarily distant host cells, the Francisella-containing phagosome matures to a late endosome-like phagosome with limited fusion to lysosomes followed by rapid bacterial escape into the cytosol where the bacterial proliferate. To decipher the molecular bases of intracellular proliferation of F. tularensis within arthropod-derived cells, we screened a comprehensive library of mutants of F. tularensis ssp. novicida for their defect in intracellular proliferation within D. melanogaster-derived S2 cells. Our data show that 394 genes, representing 22% of the genome, are required for intracellular proliferation within D. melanogaster-derived S2 cells, including many of the Francisella Pathogenicity Island (FPI) genes that are also required for proliferation within mammalian macrophages. Functional gene classes that exhibit growth defect include metabolic (25%), FPI (2%), type IV pili (1%), transport (16%) and DNA modification (5%). Among 168 most defective mutants in intracellular proliferation in S2 cells, 80 are defective in lethality and proliferation within adult D. melanogaster. The observation that only 135 of the 394 mutants that are defective in S2 cells are also defective in human macrophages indicates that F. tularensis utilize common as well as distinct mechanisms to proliferate within mammalian and arthropod cells. Our studies will facilitate deciphering the molecular aspects of F. tularensis-arthropod vector interaction and its patho-adaptation to infect mammals.

摘要

节肢动物媒介是土拉弗朗西斯菌在哺乳动物之间传播的重要载体,但对土拉弗朗西斯菌与节肢动物媒介的相互作用知之甚少。黑腹果蝇最近被开发为土拉弗朗西斯菌的节肢动物媒介模型。我们已经表明,土拉弗朗西斯菌在人单核细胞衍生的巨噬细胞和黑腹果蝇衍生的 S2 细胞中的细胞内转运非常相似。在这两种进化上相距甚远的宿主细胞中,含有弗朗西斯菌的吞噬体成熟为晚期内体样吞噬体,与溶酶体融合有限,随后迅速将细菌逃逸到细胞质中,细菌在细胞质中增殖。为了解土拉弗朗西斯菌在节肢动物衍生细胞内的细胞内增殖的分子基础,我们筛选了土拉弗朗西斯菌 ssp 的一个全面突变体文库。 novicida 在黑腹果蝇衍生的 S2 细胞中检测其细胞内增殖缺陷。我们的数据表明,394 个基因,代表基因组的 22%,是在黑腹果蝇衍生的 S2 细胞内增殖所必需的,包括许多弗朗西斯菌致病性岛(FPI)基因,这些基因也需要在哺乳动物巨噬细胞中增殖。表现出生长缺陷的功能基因类包括代谢(25%)、FPI(2%)、IV 型菌毛(1%)、运输(16%)和 DNA 修饰(5%)。在 S2 细胞中增殖缺陷最严重的 168 个突变体中,有 80 个在成年黑腹果蝇中致死和增殖缺陷。观察到只有 135 个在 S2 细胞中增殖缺陷的 394 个突变体也在人巨噬细胞中缺陷,表明土拉弗朗西斯菌利用共同和独特的机制在哺乳动物和节肢动物细胞内增殖。我们的研究将有助于阐明土拉弗朗西斯菌与节肢动物媒介的相互作用及其对感染哺乳动物的病理适应的分子方面。

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