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In vitro biofilm model for studying tongue flora and malodour

机译:用于研究舌头菌群和恶臭的体外生物膜模型

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Aims: To develop a perfusion biofilm system to model tongue biofilm microflora and their physiological response to sulfur-containing substrates (S-substrates) in terms of volatile sulfide compound (VSC) production. Methods and Results: Tongue-scrape inocula were used to establish in vitro perfusion biofilms which were examined in terms of ecological composition using culture-dependent and independent (PCR-DGGE) approaches. VSC-specific activity of cells was measured by a cell suspension assay, using a portable industrial sulfide monitor which was also used to monitor VSC production from biofilms in situ. Quasi steady states were achieved by 48 h and continued to 96 h. The mean (+/- SEM) growth rate for 72-h biofilms (n = 4) was mu = 0.014 h(-1) (+/- 0.005 h(-1)). Comparison of biofilms, perfusate and original inoculum showed their ecological composition to be similar (Pearson coefficient > 0.64). Perfusate and biofilm cells derived from the same condition (co-sampled) were equivalent with regard to VSC-specific activities which were up-regulated in the presence of S-substrates. Conclusions: The model maintained a stable tongue microcosm suitable for studying VSC production; biofilm growth in the presence of S-substrates up-regulated VSC activity. Significance and Impact of the Study: The method is apt for studying ecological and physiological aspects of oral biofilms and could be useful for screening inhibitory agents.
机译:目的:开发一种灌注生物膜系统,以模拟舌生物膜微生物区系及其对挥发性硫化物化合物(VSC)产生对含硫底物(S-底物)的生理反应。方法和结果:刮刮接种物用于建立体外灌流生物膜,并使用依赖于培养物的和独立的(PCR-DGGE)方法检查其生态成分。使用便携式工业硫化物监测器通过细胞悬浮测定法测量细胞的VSC特异性活性,该监测器也用于监测生物膜原位产生的VSC。在48小时内达到了准稳态,并持续到96小时。 72小时生物膜(n = 4)的平均(+/- SEM)生长速率为mu = 0.014 h(-1)(+/- 0.005 h(-1))。生物膜,灌流液和原始接种物的比较显示它们的生态组成相似(皮尔森系数> 0.64)。在相同的条件下(共采样)获得的灌注液和生物膜细胞在VSC特异活性方面是等效的,这些活性在S底物的存在下被上调。结论:该模型保持了适合研究VSC产生的稳定的舌头缩影。 S底物存在下生物膜的生长上调了VSC活性。研究的意义和影响:该方法适用于研究口腔生物膜的生态和生理方面,可用于筛选抑制剂。

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