首页> 美国卫生研究院文献>PLoS Pathogens >Connecting Quorum Sensing c-di-GMP Pel Polysaccharide and Biofilm Formation in Pseudomonas aeruginosa through Tyrosine Phosphatase TpbA (PA3885)
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Connecting Quorum Sensing c-di-GMP Pel Polysaccharide and Biofilm Formation in Pseudomonas aeruginosa through Tyrosine Phosphatase TpbA (PA3885)

机译:通过酪氨酸磷酸酶TpbA连接铜绿假单胞菌中的群体感应c-di-GMPPel多糖和生物膜形成(PA3885)

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摘要

With the opportunistic pathogen Pseudomonas aeruginosa, quorum sensing based on homoserine lactones was found to influence biofilm formation. Here we discern a mechanism by which quorum sensing controls biofilm formation by screening 5850 transposon mutants of P. aeruginosa PA14 for altered biofilm formation. This screen identified the PA3885 mutant, which had 147-fold more biofilm than the wild-type strain. Loss of PA3885 decreased swimming, abolished swarming, and increased attachment, although this did not affect production of rhamnolipids. The PA3885 mutant also had a wrinkly colony phenotype, formed pronounced pellicles, had substantially more aggregation, and had 28-fold more exopolysaccharide production. Expression of PA3885 in trans reduced biofilm formation and abolished aggregation. Whole transcriptome analysis showed that loss of PA3885 activated expression of the pel locus, an operon that encodes for the synthesis of extracellular matrix polysaccharide. Genetic screening identified that loss of PelABDEG and the PA1120 protein (which contains a GGDEF-motif) suppressed the phenotypes of the PA3885 mutant, suggesting that the function of the PA3885 protein is to regulate 3,5-cyclic diguanylic acid (c-di-GMP) concentrations as a phosphatase since c-di-GMP enhances biofilm formation by activating PelD, and c-di-GMP inhibits swarming. Loss of PA3885 protein increased cellular c-di-GMP concentrations; hence, PA3885 protein is a negative regulator of c-di-GMP production. Purified PA3885 protein has phosphatase activity against phosphotyrosine peptides and is translocated to the periplasm. Las-mediated quorum sensing positively regulates expression of the PA3885 gene. These results show that the PA3885 protein responds to AHL signals and likely dephosphorylates PA1120, which leads to reduced c-di-GMP production. This inhibits matrix exopolysaccharide formation, which leads to reduced biofilm formation; hence, we provide a mechanism for quorum sensing control of biofilm formation through the pel locus and suggest PA3885 should be named TpbA for tyrosine phosphatase related to biofilm formation and PA1120 should be TpbB.
机译:对于机会病原体铜绿假单胞菌,基于高丝氨酸内酯的群体感应被发现会影响生物膜的形成。在这里,我们辨别了一种机制,群体感应通过筛选铜绿假单胞菌PA14的5850个转座子突变体来改变生物膜的形成,从而控制生物膜的形成。此筛选确定了PA3885突变体,该突变体的生物膜比野生型菌株多147倍。虽然不影响鼠李糖脂的产生,但丧失PA3885可以减少游泳,消除蜂群和增加依恋。 PA3885突变体还具有皱纹的菌落表型,形成明显的薄膜,具有明显更多的聚集,并且胞外多糖产量增加了28倍。反式中PA3885的表达减少了生物膜的形成并消除了聚集。整个转录组分析表明,PA3885的缺失激活了pel位点的表达,pel位点是一种操纵子,编码细胞外基质多糖的合成。遗传筛选发现,PelABDEG和PA1120蛋白(包含GGDEF-基序)的缺失抑制了PA3885突变体的表型,表明PA3885蛋白的功能是调节3,5-环二鸟苷酸(c-di-由于c-di-GMP通过激活PelD增强了生物膜的形成,而c-di-GMP抑制了蜂群生长,因此将其作为磷酸酶浓缩。 PA3885蛋白的丢失增加了细胞c-di-GMP的浓度;因此,PA3885蛋白是c-di-GMP产生的负调节剂。纯化的PA3885蛋白具有针对磷酸酪氨酸肽的磷酸酶活性,并易位至周质。拉斯维加斯介导的群体感应正调控PA3885基因的表达。这些结果表明,PA3885蛋白响应AHL信号,并可能使PA1120去磷酸化,从而导致c-di-GMP生成减少。这会抑制基质胞外多糖的形成,从而减少生物膜的形成;因此,我们提供了一种通过群体位点来控制群体生物膜形成的群体感应控制的机制,并建议将与生物膜形成相关的酪氨酸磷酸酶的PA3885命名为TpbA,而将PA1120命名为TpbB。

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