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Transcriptional Activation of the Staphylococcus aureus putP Gene by Low-Proline-High Osmotic Conditions and during Infection of Murine and Human Tissues

机译:低脯氨酸-高渗透压条件下及小鼠和人类组织感染过程中金黄色葡萄球菌putP基因的转录激活。

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摘要

Staphylococcus aureus can grow virtually anywhere in the human body but needs to import proline through low- and high-affinity proline transporters to survive. This study examined the regulation of the S. aureus putP gene, which encodes a high-affinity proline permease. putP::lacZ and putP::lux transcriptional fusions were constructed and integrated into the genomes of several S. aureus strains. Enzyme activity was measured after growth in media with various osmolyte concentrations. As osmolarity rose, putP expression increased, with a plateau at 2 M for NaCl in strain LL3-1. Proline concentrations as low as 17.4 μM activated expression of the putP gene. The putP::lux fusion was also integrated into the genomes of S. aureus strains that were either SigB inactive (LL3-1, 8325-4, and SH1003) or SigB active (Newman and SH1000). SigB inactive strains showed increased putP gene expression as NaCl concentrations rose, whereas SigB active strains displayed a dramatic decrease in putP expression, suggesting that the alternative sigma factor B plays a negative role in putP regulation. Mice inoculated with S. aureus strains containing the putP::lux fusion exhibited up to a 715-fold increase in putP expression, although levels in the various murine organs differed. Moreover, urine from human patients infected with S. aureus showed elevated putP levels by use of a PCR procedure, whereas blood and some abscess material had no significant increase. Thus, putP is transcriptionally activated by a low-proline and high osmotic environment both in growth media and in murine or human clinical specimens.
机译:金黄色葡萄球菌几乎可以在人体任何地方生长,但需要通过低亲和力和高亲和力的脯氨酸转运蛋白进口脯氨酸才能生存。这项研究检查了金黄色葡萄球菌putP基因的调控,该基因编码高亲和力脯氨酸通透酶。构建了putP :: lacZ和putP :: lux转录融合体,并将其整合到几种金黄色葡萄球菌菌株的基因组中。在具有各种渗透压浓度的培养基中生长后,测量酶活性。随着渗透压的升高,putP表达增加,菌株LL3-1中的NaCl处于2 M的平台期。低至17.4μM的脯氨酸浓度可激活putP基因的表达。 putP :: lux融合基因也整合到了无SigB活性(LL3-1、8325-4和SH1003)或SigB活性(Newman和SH1000)的金黄色葡萄球菌菌株的基因组中。随着NaCl浓度的升高,无活性的SigB菌株显示出putP基因表达增加,而具有活性的SigB的菌株显示出putP表达急剧下降,表明替代的sigma因子B在putP调节中起负作用。接种含有 putP :: lux 融合蛋白的金黄色葡萄球菌菌株的小鼠的 putP 表达增加了多达715倍。各种小鼠器官各不相同。而且,人类患者的尿液感染了 S。通过PCR方法,金黄色葡萄球菌显示升高的 putP 水平,而血液和一些脓肿物质没有显着增加。因此, putP 在生长培养基以及鼠类或人类临床标本中均被低脯氨酸和高渗透环境转录激活。

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