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肠沙门氏菌渗透压诱导丝的特性。

Characterization of osmotically induced filaments of Salmonella enterica.

机构信息

Department of Bacteriology, University of Wisconsin-Madison, Madison, Wisconsin, USA.

出版信息

Appl Environ Microbiol. 2012 Sep;78(18):6704-13. doi: 10.1128/AEM.01784-12. Epub 2012 Jul 13.

Abstract

Salmonella enterica forms aseptate filaments with multiple nucleoids when cultured in hyperosmotic conditions. These osmotic-induced filaments are viable and form single colonies on agar plates even though they contain multiple genomes and have the potential to divide into multiple daughter cells. Introducing filaments that are formed during osmotic stress into culture conditions without additional humectants results in the formation of septa and their division into individual cells, which could present challenges to retrospective analyses of infectious dose and risk assessments. We sought to characterize the underlying mechanisms of osmotic-induced filament formation. The concentration of proteins and chromosomal DNA in filaments and control cells was similar when standardized by biomass. Furthermore, penicillin-binding proteins in the membrane of salmonellae were active in vitro. The activity of penicillin-binding protein 2 was greater in filaments than in control cells, suggesting that it may have a role in osmotic-induced filament formation. Filaments contained more ATP than did control cells in standardized cell suspensions, though the levels of two F(0)F(1)-ATP synthase subunits were reduced. Furthermore, filaments could septate and divide within 8 h in 0.2 × Luria-Bertani broth at 23°C, while nonfilamentous control cells did not replicate. Based upon the ability of filaments to septate and divide in this diluted broth, a method was developed to enumerate by plate count the number of individual, viable cells within a population of filaments. This method could aid in retrospective analyses of infectious dose of filamented salmonellae.

摘要

当沙门氏菌在高渗条件下培养时,会形成无隔膜的丝状,其中包含多个核体。这些渗透压诱导的丝状结构是有活力的,即使它们包含多个基因组并有潜力分裂成多个子细胞,也可以在琼脂平板上形成单个菌落。将渗透压应激过程中形成的丝状结构引入没有额外保湿剂的培养条件中,会导致隔膜的形成及其分裂成单个细胞,这可能对传染性剂量和风险评估的回溯分析带来挑战。我们试图描述渗透压诱导丝状形成的潜在机制。标准化生物量后,丝状体和对照细胞中的蛋白质和染色体 DNA 浓度相似。此外,沙门氏菌细胞膜中的青霉素结合蛋白在体外具有活性。与对照细胞相比,丝状体中的青霉素结合蛋白 2 的活性更高,表明它可能在渗透压诱导的丝状形成中发挥作用。在标准化细胞悬浮液中,丝状体比对照细胞含有更多的 ATP,但两个 F(0)F(1)-ATP 合酶亚基的水平降低。此外,在 23°C 下,0.2×Luria-Bertani 肉汤中,丝状结构可以在 8 小时内进行隔膜分裂和分裂,而无丝状的对照细胞不会复制。基于丝状结构在这种稀释肉汤中进行隔膜分裂和分裂的能力,开发了一种通过平板计数来计数丝状沙门氏菌群体中单个、有活力细胞数量的方法。这种方法可以帮助回溯分析丝状沙门氏菌的感染剂量。

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