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经消毒剂处理后蛋白质涂层钛表面存活黏附性血链球菌细胞的定量分析。

Quantification of vital adherent Streptococcus sanguinis cells on protein-coated titanium after disinfectant treatment.

机构信息

Institute of Preventive Dentistry and Oral Microbiology, School of Dental Medicine, University of Basel, Basel, Switzerland.

出版信息

J Mater Sci Mater Med. 2011 Sep;22(9):2045-51. doi: 10.1007/s10856-011-4377-5. Epub 2011 Jun 14.

Abstract

The quantification of vital adherent bacteria is challenging, especially when efficacy of antimicrobial agents is to be evaluated. In this study three different methods were compared in order to quantify vital adherent Streptococcus sanguinis cells after exposure to disinfectants. An anaerobic flow chamber model accomplished initial adhesion of S. sanguinis on protein-coated titanium. Effects of chlorhexidine, Betadine®, Octenidol®, and ProntOral® were assessed by quantifying vital cells using Live/Dead BacLight™, conventional culturing and isothermal microcalorimetry (IMC). Results were analysed by Kruskal-Wallis one-way analysis of variance. Live/dead staining revealed highest vital cell counts (P < 0.05) and demonstrated dose-dependent effect for all disinfectants. Microcalorimetry showed time-delayed heat flow peaks that were proportioned to the remaining number of viable cells. Over 48 h there was no difference in total heat between treated and untreated samples (P > 0.05), indicating equivalent numbers of bacteria were created and disinfectants delayed growth but did not eliminate it. In conclusion, contrary to culturing, live/dead staining enables detection of cells that may be viable but non-cultivable. Microcalorimetry allows unique evaluation of relative disinfectant effects by quantifying differences in time delay of regrowth of remaining vital cells.

摘要

定量检测重要黏附菌具有挑战性,特别是在评估抗菌剂的功效时。本研究比较了三种不同的方法,以定量检测经消毒剂处理后的黏附性存活口腔链球菌细胞。在蛋白包被钛金属表面,采用厌氧流动室模型完成口腔链球菌的初始黏附。通过使用 Live/Dead BacLight™、常规培养和等温微量热法(IMC)定量检测活菌,评估洗必泰、聚维酮碘、奥替尼啶和普瑞沃口腔抗菌溶液对口腔链球菌的作用。采用 Kruskal-Wallis 单向方差分析对结果进行分析。活/死染色显示出最高的活菌计数(P < 0.05),并显示出所有消毒剂的剂量依赖性效应。微量热法显示出延迟的热流峰,与存活细胞的数量成正比。在 48 小时内,处理组和未处理组之间的总热量没有差异(P > 0.05),表明产生的细菌数量相等,消毒剂仅延迟了细菌生长,但没有消灭细菌。总之,与培养法相反,活/死染色能够检测到可能存活但不可培养的细胞。微量热法通过量化剩余存活细胞再生时间延迟的差异,可独特地评估相对消毒剂的效果。

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