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Microtiter susceptibility testing of microbes growing on peg lids: A miniaturized biofilm model for high-throughput screening

机译:钉盖上生长的微生物的微量滴定度敏感性测试:用于高通量筛选的微型生物膜模型

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Batch culture of biofilms on peg lids is a versatile method that can be used for microtiter determinations of biofilm antimicrobial susceptibility. In this paper, we describe a core protocol and a set of parameters (surface composition, the rate of rocking or orbital motion, temperature, cultivation time, inoculum size, atmospheric gases and nutritional medium) that can be adjusted to grow single-or multispecies biofilms on peg surfaces. Mature biofilms formed on peg lids can then be fitted into microtiter plates containing test agents. After a suitable exposure time, biofilm cells are disrupted into a recovery medium using sonication. Microbicidal endpoints can be determined qualitatively using optical density measurements or quantitatively using viable cell counting. Once equipment is calibrated and growth conditions are at an optimum, the procedure requires 5 h of work over 4-6 d. This efficient method allows antimicrobial agents and exposure conditions to be tested against biofilms on a high-throughput scale.
机译:在桩盖上分批培养生物膜是一种通用的方法,可用于微量滴定法测定生物膜的抗菌敏感性。在本文中,我们描述了可以调整以生长单物种或多物种的核心协议和一组参数(表面成分,摇摆或轨道运动的速率,温度,培养时间,接种量,大气气体和营养培养基)钉表面上的生物膜。然后可以将形成在桩盖上的成熟生物膜装到装有测试剂的微量滴定板中。在合适的暴露时间后,使用超声将生物膜细胞破坏到恢复培养基中。杀微生物终点可以使用光密度测量进行定性确定,也可以使用活细胞计数进行定量确定。一旦对设备进行校准并且生长条件达到最佳,该过程需要在4-6 d内进行5小时的工作。这种有效的方法允许以高通量规模针对生物膜测试抗菌剂和暴露条件。

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