首页> 美国卫生研究院文献>Journal of Bacteriology >Proteome Analysis of the Effect of Mucoid Conversion on Global Protein Expression in Pseudomonas aeruginosa Strain PAO1 Shows Induction of the Disulfide Bond Isomerase DsbA
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Proteome Analysis of the Effect of Mucoid Conversion on Global Protein Expression in Pseudomonas aeruginosa Strain PAO1 Shows Induction of the Disulfide Bond Isomerase DsbA

机译:蛋白质组学分析的铜绿假单胞菌菌株PAO1中的粘液样转换对全局蛋白表达的影响表明二硫键异构酶DsbA的诱导。

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摘要

Pseudomonas aeruginosa strains that cause chronic pulmonary infections in cystic fibrosis patients typically undergo mucoid conversion. The mucoid phenotype indicates alginate overproduction and is often due to defects in MucA, an antisigma factor that controls the activity of sigma-22 (AlgT [also called AlgU]), which is required for the activation of genes for alginate biosynthesis. In this study we hypothesized that mucoid conversion may be part of a larger response that activates genes other than those for alginate synthesis. To address this, a two-dimensional (2-D) gel analysis was employed to compare total proteins in strain PAO1 to those of its mucA22 derivative, PDO300, in order to identify protein levels enhanced by mucoid conversion. Six proteins that were clearly more abundant in the mucoid strain were observed. The amino termini of such proteins were determined and used to identify the gene products in the genomic database. Proteins involved in alginate biosynthesis were expected among these, and two (AlgA and AlgD) were identified. This result verified that the 2-D gel approach could identify gene products under sigma-22 control and upregulated by mucA mutation. Two other protein spots were also clearly upregulated in the mucA22 background, and these were identified as porin F (an outer membrane protein) and a homologue of DsbA (a disulfide bond isomerase). Single-copy gene fusions were constructed to test whether these proteins were enhanced in the mucoid strain due to increased transcription. The oprF-lacZ fusion showed little difference in levels of expression in the two strains. However, the dsbA-lacZ fusion showed two- to threefold higher expression in PDO300 than in PAO1, suggesting that its promoter was upregulated by the deregulation of sigma-22 activity. A dsbA-null mutant was constructed in PAO1 and shown to have defects predicted for a cell with reduced disulfide bond isomerase activity, namely, reduction in periplasmic alkaline phosphatase activity, increased sensitivity to dithiothreitol, reduced type IV pilin-mediated twitching motility, and reduced accumulation of extracellular proteases, including elastase. Although efficient secretion of elastase in the dsbA mutant was still demonstrable, the elastase produced appeared to be unstable, possibly as a result of mispaired disulfide bonds. Disruption of dsbA in the mucoid PDO300 background did not affect alginate production. Thus, even though dsbA is coregulated with mucoid conversion, it was not required for alginate production. This suggests that mucA mutation, which deregulates sigma-22, results in a global response that includes other factors in addition to increasing the production of alginate.
机译:在囊性纤维化患者中引起慢性肺部感染的铜绿假单胞菌菌株通常经历粘液样转化。粘液表型表明藻酸盐的过量生产,通常是由于MucA中的缺陷所致,MucA是控制sigma-22(AlgT [也称为AlgU])活性的抗σ因子,这是激活藻酸盐生物合成基因所必需的。在这项研究中,我们假设粘液样转化可能是更大反应的一部分,该反应激活了藻酸盐合成基因以外的其他基因。为了解决这个问题,采用了二维(2-D)凝胶分析来比较菌株PAO1中的总蛋白与其mucA22衍生物PDO300的蛋白,以鉴定通过粘液样转化增强的蛋白水平。观察到在粘液样菌株中明显更丰富的六个蛋白质。确定了这类蛋白质的氨基末端,并用于鉴定基因组数据库中的基因产物。在这些蛋白中,预期与藻酸盐生物合成有关的蛋白被鉴定出两种(AlgA和AlgD)。该结果证实了2-D凝胶方法可以鉴定在sigma-22控制下并由mucA突变上调的基因产物。在mucA22背景中,另外两个蛋白点也明显上调,这些蛋白点被鉴定为孔蛋白F(外膜蛋白)和DsbA的同源物(二硫键异构酶)。构建单拷贝基因融合体以测试这些蛋白是否因转录增加而在粘液样菌株中增强。 oprF-lacZ融合体在两种菌株中的表达水平几乎没有差异。但是,dsbA-lacZ融合体在PDO300中的表达比在PAO1中高2至3倍,这表明其启动子因sigma-22活性的失调而被上调。在PAO1中构建了一个dsbA-null突变体,发现该突变体具有预测的缺陷,该缺陷具有降低的二硫键异构酶活性的细胞,即,胞质碱性磷酸酶活性的降低,对二硫苏糖醇的敏感性增加,IV型菌毛蛋白介导的抽搐运动性降低和降低包括弹性蛋白酶在内的细胞外蛋白酶的积累。尽管仍然可以证明dsbA突变体中弹性蛋白酶的有效分泌,但是产生的弹性蛋白酶似乎不稳定,可能是由于二硫键配对不正确所致。在粘液状PDO300背景中破坏dsbA不会影响藻酸盐的产生。因此,即使dsbA与粘液样转化成粒,但藻酸盐生产并不需要它。这表明,使sigma-22失控的mucA突变会导致总体反应,除了增加藻酸盐的产生外,其还包括其他因素。

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