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Construction and Characterization of a proU-gfp Transcriptional Fusion That Measures Water Availability in a Microbial Habitat†

机译:proU-gfp转录融合蛋白的构建和表征,该融合蛋白可测量微生物栖息地中的水利用率†

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We constructed and characterized a transcriptional fusion that measures the availability of water to a bacterial cell. This fusion between the proU promoter from Escherichia coli and the reporter gene gfp was introduced into strains of E. coli, Pantoea agglomerans, and Pseudomonas syringae. The proU-gfp fusion in these bacterial biosensor strains responded in a quantitative manner to water deprivation caused by the presence of NaCl, Na2SO4, KCl, or polyethylene glycol (molecular weight, 8000). The fusion was induced to a detectable level by NaCl concentrations of as low as 10 mM in all three bacterial species. Water deprivation induced proU-gfp expression in both planktonic and surface-associated cells; however, it induced a higher level of expression in the surface-associated cells. Following the introduction of P. agglomerans biosensor cells onto bean leaves, the cells detected a significant decrease in water availability within only 5 min. After 30 min, the populations were exposed, on average, to a water potential equivalent to that imposed by approximately 55 mM NaCl. These results demonstrate the effectiveness of a proU-gfp-based biosensor for evaluating water availability on leaves. Furthermore, the inducibility of proU-gfp in multiple bacterial species illustrates the potential for tailoring proU-gfp-based biosensors to specific habitats.
机译:我们构建并表征了一种转录融合体,可测量细菌细胞中水的可用性。来自大肠杆菌的proU启动子和报告基因gfp之间的这种融合被引入到大肠杆菌,聚结泛菌和丁香假单胞菌的菌株中。这些细菌生物传感器菌株中的proU-gfp融合物以定量方式响应由NaCl,Na2SO4,KCl或聚乙二醇(分子量为8000)的存在引起的水缺乏。在所有三个细菌物种中,通过低至10 mM的NaCl浓度将融合诱导到可检测的水平。缺水诱导浮游细胞和表面相关细胞中的proU-gfp表达;然而,它在表面相关细胞中诱导了更高水平的表达。在将P. aglomerans生物传感器细胞引入豆叶后,这些细胞仅在5分钟内就检测到了水利用率的显着下降。 30分钟后,这些种群平均受到的水势相当于大约55 mM NaCl施加的水势。这些结果证明了基于proU-gfp的生物传感器在评估叶片水分利用率方面的有效性。此外,proU-gfp在多种细菌物种中的可诱导性说明了针对特定栖息地定制基于proU-gfp的生物传感器的潜力。

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