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首页> 外文期刊>Journal of bacteriology >Transcriptional analysis of the Pseudomonas aeruginosa genes algR, algB, and algD reveals a hierarchy of alginate gene expression which is modulated by algT.
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Transcriptional analysis of the Pseudomonas aeruginosa genes algR, algB, and algD reveals a hierarchy of alginate gene expression which is modulated by algT.

机译:铜绿假单胞菌基因algR,algB和algD的转录分析显示了algT调节的藻酸盐基因表达层次。

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Strains of Pseudomonas aeruginosa which colonize and infect the lungs of cystic fibrosis patients have a mucoid colony morphology due to the overproduction of the exopolysaccharide alginate. The response regulators AlgB and AlgR are required for the transcription of algD, a tightly regulated gene encoding GDP-mannose dehydrogenase, which is critical for P. aeruginosa alginate biosynthesis. Previous studies indicated that mutations in the algT gene of mucoid FRD1 P. aeruginosa result in nonmucoid derivatives. However, the specific role for algT in alginate gene regulation has not been elucidated. In this study, transcription of algB, algD, and algR was characterized by gene fusion and primer extension analysis. Expression of algR and algD was abolished in P. aeruginosa strains containing algT::Tn501 insertions because of lack of transcription initiation at the algR and algD promoters. An algR mutation was constructed in FRD1, and this resulted in the loss of alginate production and a dramatic decrease in algD transcription. RNA and gene fusion analysis revealed that algB is not required for algR expression, nor is algR necessary for transcription of algB. Thus, with the exception of a requirement for AlgT, the AlgB and AlgR pathways appear to be independent of each other. In gel band mobility shift assays, a protein(s) present in extracts from mucoid and algB and algR mutant P. aeruginosa strains formed a specific complex with algD sequences located immediately upstream of the start of transcription. No binding to these sequences was observed when extracts from algT mutant strains were examined. A model proposed suggests that a hierarchy of alginate gene expression exists in which AlgT is required for transcription of the response regulators algB and algR, which in turn are necessary for algD expression. AlgT or a protein under algT control also binds to sequences located within the algD promoter.
机译:定居并感染囊性纤维化患者肺部的铜绿假单胞菌菌株由于胞外藻酸盐藻酸盐的过量产生而具有粘液样菌落形态。响应调节剂AlgB和AlgR是algD转录所必需的,而algD是编码GDP-甘露糖脱氢酶的严格调控的基因,这对铜绿假单胞菌藻酸盐的生物合成至关重要。先前的研究表明,黏液状FRD1铜绿假单胞菌algT基因的突变会导致产生非黏液状衍生物。然而,尚未阐明algT在藻酸盐基因调节中的具体作用。在这项研究中,通过基因融合和引物延伸分析来表征algB,algD和algR的转录。由于在algR和algD启动子上缺乏转录起始,在含algT :: Tn501插入的铜绿假单胞菌菌株中取消了algR和algD的表达。在FRD1中构建了一个algR突变,这导致藻酸盐产量的损失和algD转录的急剧下降。 RNA和基因融合分析显示algR不需要algB表达,也不需要algR转录algB。因此,除了需要AlgT外,AlgB和AlgR途径似乎彼此独立。在凝胶带迁移分析中,存在于粘液样和algB和algR突变铜绿假单胞菌菌株提取物中的一种或多种蛋白质与algD序列形成了一个特定的复合物,该序列位于紧接转录开始的上游。当检查来自algT突变株的提取物时,未观察到与这些序列的结合。提出的模型表明,存在藻酸盐基因表达的层次结构,其中响应调节因子algB和algR的转录需要AlgT,而这对于algD表达是必需的。 AlgT或在algT控制下的蛋白质也与位于algD启动子内的序列结合。

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