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Production of the Type IV Secretion System Differs among Brucella Species as Revealed with VirB5- and VirB8-Specific Antisera

机译:VirB5和VirB8特异性抗血清显示布鲁氏菌属物种间IV型分泌系统的产生不同

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Expression of the virB operon, encoding the type IV secretion system required for Brucella suis virulence, occurred in the acidic phagocytic vacuoles of macrophages and could be induced in minimal medium at acidic pH values. To analyze the production of VirB proteins, polyclonal antisera against B. suis VirB5 and VirB8 were generated. Western blot analysis revealed that VirB5 and VirB8 were detected after 3 h in acidic minimal medium and that the amounts increased after prolonged incubation. Unlike what occurs in the related organism Agrobacterium tumefaciens, the periplasmic sugar binding protein ChvE did not contribute to VirB protein production, and B. suis from which chvE was deleted was fully virulent in a mouse model. Comparative analyses of various Brucella species revealed that in all of them VirB protein production increased under acidic conditions. However, in rich medium at neutral pH, Brucella canis and B. suis, as well as the Brucella abortus- and Brucella melitensis-derived vaccine strains S19, RB51, and Rev.1, produced no VirB proteins or only small amounts of VirB proteins, whereas the parental B. abortus and B. melitensis strains constitutively produced VirB5 and VirB8. Thus, the vaccine strains were still able to induce virB expression under acidic conditions, but the VirB protein production was markedly different from that in the wild-type strains at pH 7. Taken together, the data indicate that VirB protein production and probably expression of the virB operon are not uniformly regulated in different Brucella species. Since VirB proteins were shown to modulate Brucella phagocytosis and intracellular trafficking, the differential regulation of the production of these proteins reported here may provide a clue to explain their role(s) during the infection process.
机译:编码 Brucella suis 毒力的IV型分泌系统的 virB 操纵子的表达发生在巨噬细胞的酸性吞噬液泡中,并且可以在酸性pH的最小培养基中诱导价值观。为了分析VirB蛋白的产生,针对 B的多克隆抗血清。 suis VirB5和VirB8已生成。蛋白质印迹分析表明,在酸性基本培养基中3 h后检测到VirB5和VirB8,长时间孵育后其量增加。与相关生物根癌土壤杆菌中发生的变化不同,周质糖结合蛋白ChvE对VirB蛋白和 B的贡献不大。删除了 chvE 的suis 在小鼠模型中具有完全毒性。对各种 Brucella 物种的比较分析表明,在酸性条件下,所有这些物种中的VirB蛋白产量均增加。但是,在中性pH的丰富培养基中,布鲁氏菌 B。 suis ,以及流产布鲁氏菌布鲁氏菌衍生的疫苗株S19,RB51和Rev.1,均未产生VirB蛋白或仅产生少量数量的VirB蛋白,而亲本 B。流产 B。 melitensis 菌株构成了VirB5和VirB8。因此,该疫苗株在酸性条件下仍能诱导 virB 表达,但在pH 7时,VirB蛋白的产生与野生株显着不同。在不同的 Brucella 物种中,VirB蛋白的产生以及 virB 操纵子的表达可能不受统一的调控。由于显示VirB蛋白可调节 Brucella 吞噬作用和细胞内运输,因此本文报道的这些蛋白的生产差异调节可能为解释其在感染过程中的作用提供线索。

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