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利用高通量遗传筛选鉴定霍乱弧菌xds基因的体内调节因子。

Identification of in vivo regulators of the Vibrio cholerae xds gene using a high-throughput genetic selection.

作者信息

McDonough Emilykate, Lazinski David W, Camilli Andrew

机构信息

Howard Hughes Medical Institute and Department of Molecular Biology and Microbiology, Tufts University School of Medicine, Boston, MA, 02111, USA.

出版信息

Mol Microbiol. 2014 Apr;92(2):302-15. doi: 10.1111/mmi.12557. Epub 2014 Mar 14.

Abstract

Vibrio cholerae, the causative agent of cholera, remains a threat to public health in areas with inadequate sanitation. As a waterborne pathogen, V. cholerae moves between two dissimilar environments, aquatic reservoirs and the intestinal tract of humans. Accordingly, this pathogen undergoes adaptive shifts in gene expression throughout the different stages of its lifecycle. One particular gene, xds, encodes a secreted exonuclease that was previously identified as being induced during infection. Here we sought to identify regulators responsible for the in vivo-specific induction of xds. A transcriptional fusion of xds to two consecutive antibiotic resistance genes was used to select transposon mutants that had inserted within or adjacent to regulatory genes and thereby caused increased expression of the xds fusion under non-inducing conditions. Large pools of selected insertion sites were sequenced in a high throughput manner using Tn-seq to identify potential mechanisms of xds regulation. Our selection identified the two-component system PhoB/R as the dominant activator of xds expression. In vitro validation confirmed that PhoB, a protein which is only active during phosphate limitation, was responsible for xds activation. Using xds expression as a biosensor of the extracellular phosphate level, we observed that the mouse small intestine is a phosphate-limited environment.

摘要

霍乱弧菌是霍乱的病原体,在卫生条件差的地区仍然对公众健康构成威胁。作为一种水传播病原体,霍乱弧菌在两种不同的环境——水生宿主和人类肠道之间移动。因此,这种病原体在其生命周期的不同阶段会经历基因表达的适应性变化。一个特定的基因xds编码一种分泌型核酸外切酶,该酶先前被鉴定为在感染期间被诱导表达。在这里,我们试图确定负责xds体内特异性诱导的调节因子。将xds与两个连续的抗生素抗性基因进行转录融合,用于筛选插入调节基因内部或附近的转座子突变体,从而在非诱导条件下导致xds融合基因的表达增加。使用Tn-seq以高通量方式对大量选定的插入位点进行测序,以确定xds调节的潜在机制。我们的筛选确定了双组分系统PhoB/R是xds表达的主要激活因子。体外验证证实,仅在磷酸盐限制期间具有活性的蛋白质PhoB负责xds的激活。利用xds表达作为细胞外磷酸盐水平的生物传感器,我们观察到小鼠小肠是一个磷酸盐限制的环境。

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