Wiley David J, Nordfeldth Roland, Rosenzweig Jason, DaFonseca Christopher J, Gustin Richard, Wolf-Watz Hans, Schesser Kurt
Department of Microbiology and Immunology, University of Miami School of Medicine, Miami, FL 33101, USA.
Microb Pathog. 2006 May;40(5):234-43. doi: 10.1016/j.micpath.2006.02.001. Epub 2006 Apr 19.
The Yersinia protein kinase A (YpkA) is injected into host cells by the yersinial type three secretion system (TTSS). YpkA is widely believed to function within the host cell based on the fact that its kinase domain is clearly homologous to eukaryotic Ser/Thr kinases and that its enzymatic activity, when assayed in vitro, is dependent on eukaryotic-derived host factors. Whether this activity is required for virulence has not been addressed. Here, we report that a Yersinia pseudotuberculosis strain expressing a kinase-inactive YpkA(D270A) variant is greatly attenuated in the mouse model of infection compared to the isogenic wild-type strain. The ypkA(D270A) mutant strain was likewise attenuated in a cell culture infection assay indicating that the kinase activity of YpkA enhances the viability of host cell-associated bacteria. To begin to understand what cellular activities are targeted, we expressed YpkA and its variants in two different yeast model systems. In agreement with previous studies, we found that when rapidly induced and expressed at high levels in Saccharomyces cerevisiae, YpkA-mediated toxicity occurred extremely swiftly. Under these conditions toxicity was dependent on the structurally distinct GTPase-binding domain of YpkA and was entirely independent of its kinase activity. Therefore, to probe for kinase-dependent effects we expressed YpkA and its kinase-inactive variant at comparatively moderate levels in the fission yeast Schizosaccharomyces pombe. S. pombe is particularly well suited for actin cytoskeletal studies due to its easily quantifiable, well defined pattern of actin localization. S. pombe transformed with a wild-type YpkA-encoding plasmid displayed a pronounced actin mislocalization phenotype, the severity of which was directly proportional to the level of YpkA expressed in the cell. In cells expressing the kinase-inactive YpkA variant, the degree of actin mislocalization was reduced, but not entirely abrogated, suggesting that YpkA affects the eukaryotic cytoskeleton through kinase-dependent and kinase-independent mechanisms. Collectively, our yeast-derived results show how critical expression levels and exposure periods are for assaying virulence factor activities in heterologous model systems. More generally, our finding that the 'eukaryotic-like' kinase domain of YpkA is important for virulence illustrates how a bacterium can utilize a host-like factor or activity in order to enhance its survival following host cell contact.
耶尔森氏菌蛋白激酶A(YpkA)通过耶尔森氏菌三型分泌系统(TTSS)注入宿主细胞。基于其激酶结构域与真核丝氨酸/苏氨酸激酶明显同源,以及在体外测定时其酶活性依赖于真核来源的宿主因子这一事实,人们普遍认为YpkA在宿主细胞内发挥作用。这种活性是否是毒力所必需的尚未得到探讨。在此,我们报告,与同基因野生型菌株相比,表达激酶失活的YpkA(D270A)变体的假结核耶尔森氏菌菌株在小鼠感染模型中显著减毒。ypkA(D270A)突变菌株在细胞培养感染试验中同样减毒,表明YpkA的激酶活性增强了与宿主细胞相关细菌的活力。为了开始了解YpkA靶向哪些细胞活动,我们在两种不同的酵母模型系统中表达了YpkA及其变体。与先前的研究一致,我们发现,当在酿酒酵母中快速诱导并高水平表达时,YpkA介导的毒性迅速发生。在这些条件下,毒性依赖于YpkA结构上不同的GTPase结合结构域,并且完全独立于其激酶活性。因此,为了探究激酶依赖性效应,我们在裂殖酵母粟酒裂殖酵母中以相对适中的水平表达了YpkA及其激酶失活变体。粟酒裂殖酵母因其易于定量、明确的肌动蛋白定位模式,特别适合用于肌动蛋白细胞骨架研究。用编码野生型YpkA的质粒转化的粟酒裂殖酵母表现出明显的肌动蛋白定位错误表型,其严重程度与细胞中表达的YpkA水平直接相关。在表达激酶失活的YpkA变体的细胞中,肌动蛋白定位错误的程度降低,但并未完全消除,这表明YpkA通过激酶依赖性和激酶非依赖性机制影响真核细胞骨架。总的来说,我们从酵母中获得的结果表明,表达水平和暴露时间对于在异源模型系统中测定毒力因子活性至关重要。更一般地说,我们发现YpkA的“类真核”激酶结构域对毒力很重要,这说明了细菌如何利用类似宿主的因子或活性来增强其与宿主细胞接触后的生存能力。
