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在丁香假单胞菌番茄致病变种 DC3000 中,碳源和细胞密度对 III 型分泌系统基因表达的调控作用。

Carbon source and cell density-dependent regulation of type III secretion system gene expression in Pseudomonas syringae pathovar tomato DC3000.

机构信息

Department of Biology, University of Missouri-St. Louis, St. Louis, MO 63121, USA.

出版信息

Res Microbiol. 2012 Sep-Oct;163(8):531-9. doi: 10.1016/j.resmic.2012.08.005. Epub 2012 Aug 23.

DOI:10.1016/j.resmic.2012.08.005
PMID:22944041
Abstract

Pseudomonas syringae utilizes a type III secretion system (T3SS) encoded by the hrp/hrc genes to translocate virulence proteins called effectors into plant cells. To ensure that the T3SS functions at appropriate times during infection, hrp/hrc and effector gene expression is modulated by environmental conditions and a complex network of transcription factors. The sigma factor HrpL activates hrp/hrc and effector genes, while σ(54) and enhancer binding proteins HrpR and HrpS regulate hrpL. To better understand how environmental conditions control the T3SS regulatory cascade in P. syringae pathovar tomato strain DC3000, we tested the effects of various growth media and carbon sources on expression of the hrpRS operon, hrpL, and the effector avrPto. Fructose optimally induced hrpRS expression, while most other carbon sources had only mild stimulatory effects. In contrast, hrpL and avrPto were highly induced by several sugars and organic acids, yet expression decreased as cultures reached higher cell densities. This cell density-dependent regulation was not due to alteration of the pH of the medium, although involvement of a quorum sensing signal was also not apparent. Our findings may explain conflicting results from previous studies and additionally indicate that culture conditions should be considered carefully when examining T3SS gene expression.

摘要

丁香假单胞菌利用由 hrp/hrc 基因编码的 III 型分泌系统 (T3SS) 将毒力蛋白效应子易位到植物细胞中。为了确保 T3SS 在感染过程中的适当时间发挥作用,hrp/hrc 和效应子基因的表达受到环境条件和转录因子复杂网络的调节。σ 因子 HrpL 激活 hpr/hrc 和效应子基因,而 σ(54)和增强子结合蛋白 HrpR 和 HrpS 调节 HrpL。为了更好地理解环境条件如何控制丁香假单胞菌番茄亚种 DC3000 中的 T3SS 调控级联,我们测试了各种生长培养基和碳源对 hprRS 操纵子、hrpL 和效应子 avrPto 的表达的影响。果糖最能诱导 hprRS 的表达,而大多数其他碳源只有轻微的刺激作用。相比之下,hrpL 和 avrPto 被几种糖和有机酸高度诱导,但随着培养物达到更高的细胞密度,表达量下降。这种细胞密度依赖性调节不是由于培养基 pH 的改变引起的,尽管也没有明显涉及群体感应信号。我们的发现可以解释以前研究中的矛盾结果,并表明在研究 T3SS 基因表达时,应该仔细考虑培养条件。

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