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Identification of a gene essential for O-acetylation of the Staphylococcus aureus type 5 capsular polysaccharide.

机译:鉴定了金黄色葡萄球菌5型荚膜多糖O-乙酰化所必需的基因。

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The Staphylococcus aureus serotype 5 capsular polysaccharide (CP5) has a trisaccharide repeating unit of (-->4)-3-O-Ac-beta-D-ManNAcAp-(1-->4)-alpha-L-FucNAcp-(1-->3 )-beta-D-FucNAcp-(1-->). Tn918 mutagenesis of strain Reynolds yielded a mutant that produced wild-type levels of O-deacetylated CP5. The site and orientation of the single transposon insertion in mutant JL232 were determined by analysis of Southern blots and amplification of DNA flanking the transposon. DNA sequencing revealed that Tn918 was inserted within an open reading frame of 627 bp. The predicted amino acid sequence encodes a protein of approximately 26 kDa with homology to members of the NodL-LacA-CysE family of bacterial acetyltransferases. Southern blot analysis showed that genes similar to cap5H were present only in strains of S. aureus belonging to capsular serotypes 2, 4 and 5. In an in vitro assay, the parental strain was more resistant to opsonophagocytic killing than the mutant strain. In a mouse model of staphylococcal infection, the parental strain was able to seed the bloodstream from the peritoneal cavity and colonize the kidneys more efficiently than the O-deacetylated mutant. When cap5H was provided to the mutant in trans, it fully restored CP5 O-acetylation. The virulence of the complemented mutant strain closely approximated that of the parental strain.
机译:金黄色葡萄球菌血清5型荚膜多糖(CP5)具有(-> 4)-3-O-Ac-beta-D-ManNAcAp-(1-> 4)-alpha-L-FucNAcp-( 1-> 3)-beta-D-FucNAcp-(1->)。雷诺菌株的Tn918诱变产生了一个突变体,该突变体产生了野生型的O-去乙酰化CP5。通过Southern印迹分析和转座子侧翼DNA的扩增,确定突变体JL232中单个转座子插入的位点和方向。 DNA测序表明Tn918插入了627 bp的开放阅读框内。预测的氨基酸序列编码与细菌乙酰转移酶的NodL-LacA-CysE家族成员同源的约26 kDa的蛋白质。 Southern印迹分析表明,类似于cap5H的基因仅存在于属于荚膜血清型2、4和5的金黄色葡萄球菌菌株中。在体外测定中,亲本菌株对调理吞噬细胞的杀伤力比突变菌株更高。在葡萄球菌感染的小鼠模型中,与O-脱乙酰化突变体相比,亲本菌株能够从腹膜腔播种血流并更有效地定居肾脏。当将cap5H反式提供给突变体时,它完全恢复了CP5 O-乙酰化。互补突变株的毒力非常接近亲本株的毒力。

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