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The Stringent Response of Staphylococcus aureus and Its Impact on Survival after Phagocytosis through the Induction of Intracellular PSMs Expression

机译:金黄色葡萄球菌的严格反应及其通过吞噬细胞内PSMs表达对吞噬后存活的影响

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摘要

The stringent response is initiated by rapid (p)ppGpp synthesis, which leads to a profound reprogramming of gene expression in most bacteria. The stringent phenotype seems to be species specific and may be mediated by fundamentally different molecular mechanisms. In Staphylococcus aureus, (p)ppGpp synthesis upon amino acid deprivation is achieved through the synthase domain of the bifunctional enzyme RSH (RelA/SpoT homolog). In several firmicutes, a direct link between stringent response and the CodY regulon was proposed. Wild-type strain HG001, rshSyn, codY and rshSyn, codY double mutants were analyzed by transcriptome analysis to delineate different consequences of RSH-dependent (p)ppGpp synthesis after induction of the stringent response by amino-acid deprivation. Under these conditions genes coding for major components of the protein synthesis machinery and nucleotide metabolism were down-regulated only in rsh positive strains. Genes which became activated upon (p)ppGpp induction are mostly regulated indirectly via de-repression of the GTP-responsive repressor CodY. Only seven genes, including those coding for the cytotoxic phenol-soluble modulins (PSMs), were found to be up-regulated via RSH independently of CodY. qtRT-PCR analyses of hallmark genes of the stringent response indicate that an RSH activating stringent condition is induced after uptake of S. aureus in human polymorphonuclear neutrophils (PMNs). The RSH activity in turn is crucial for intracellular expression of psms. Accordingly, rshSyn and rshSyn, codY mutants were less able to survive after phagocytosis similar to psm mutants. Intraphagosomal induction of psmα1-4 and/or psmβ1,2 could complement the survival of the rshSyn mutant. Thus, an active RSH synthase is required for intracellular psm expression which contributes to survival after phagocytosis.
机译:严格的响应由快速(p)ppGpp合成引发,这导致大多数细菌中基因表达的深刻重编程。严格的表型似乎是物种特异性的,并且可能由根本不同的分子机制介导。在金黄色葡萄球菌中,氨基酸缺失后的(p)ppGpp合成是通过双功能酶RSH的合酶结构域实现的(RelA / SpoT同源物)。在一些公司中,提出了严格反应与CodY调节剂之间的直接联系。通过转录组分析对野生型菌株HG001,rshSyn,codY和rshSyn,codY双突变体进行了分析,以描绘出通过氨基酸剥夺诱导严格反应后RSH依赖性(p)ppGpp合成的不同结果。在这些条件下,仅在rsh阳性菌株中编码蛋白质合成机制和核苷酸代谢主要成分的基因被下调。 (p)ppGpp诱导后被激活的基因大部分是通过抑制GTP反应性阻遏物CodY间接调控的。发现只有7个基因,包括那些编码细胞毒性酚溶性调节蛋白(PSMs)的基因,都通过RSH独立于CodY被上调。对严格应答的标志基因的qtRT-PCR分析表明,在人类多形核中性粒细胞(PMN)中摄取金黄色葡萄球菌后,会诱导出RSH激活严格条件。反过来,RSH活性对于psms的细胞内表达至关重要。因此,类似于psm突变体,rshSyn和rshSyn,codY突变体在吞噬作用后存活的能力较弱。噬菌体内对psmα1-4和/或psmβ1,2的诱导可以补充rshSyn突变体的存活。因此,细胞内psm表达需要活性RSH合酶,其有助于吞噬后的存活。

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