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体外群体感应抑制的定性和定量测定。

Qualitative and quantitative determination of quorum sensing inhibition in vitro.

作者信息

Jakobsen Tim Holm, van Gennip Maria, Christensen Louise Dahl, Bjarnsholt Thomas, Givskov Michael

机构信息

Department of International Health, Immunology, and Microbiology, Faculty of Health Sciences, University of Copenhagen, Copenhagen, Denmark.

出版信息

Methods Mol Biol. 2011;692:253-63. doi: 10.1007/978-1-60761-971-0_18.

Abstract

The formation of biofilms in conjunction with quorum sensing (QS)-regulated expression of virulence by opportunistic pathogens contributes significantly to immune evasion and tolerance to a variety of antimicrobial treatments. The present protocol describes methods to determine the in vitro efficacy of potential quorum sensing inhibitors (QSIs). Work on Pseudomonas aeruginosa has shown that chemical blockage of QS is a promising new antimicrobial strategy. Several live bacterial reporter systems been developed to screen extracts and pure compounds for QSI activity. Here we describe the usage of reporter strains consisting of a lasB-gfp or rhlA-gfp fusion in P. aeruginosa for qualitative and quantitative evaluation of the inhibition of the two major QS pathways, monitored as reduced expression of green fluorescence. By the use of an in vitro flow cell system it is possible to study the QSI activity by monitoring its ability to interfere with the protective functions of bacterial biofilm. For evaluation of the global effects of QSI compounds, we present a protocol for the DNA microarray-based transcriptomics. Using these in vitro methods it is possible to evaluate the potential of various QSI compounds.

摘要

机会性病原体形成生物膜并通过群体感应(QS)调节毒力表达,这对免疫逃避和耐受多种抗菌治疗有显著作用。本方案描述了测定潜在群体感应抑制剂(QSI)体外疗效的方法。对铜绿假单胞菌的研究表明,QS的化学阻断是一种有前景的新型抗菌策略。已开发出几种活细菌报告系统来筛选提取物和纯化合物的QSI活性。在此,我们描述了使用由铜绿假单胞菌中lasB - gfp或rhlA - gfp融合体组成的报告菌株,通过监测绿色荧光表达降低来定性和定量评估两种主要QS途径的抑制作用。通过使用体外流动细胞系统,能够通过监测其干扰细菌生物膜保护功能的能力来研究QSI活性。为了评估QSI化合物的整体效应,我们提出了基于DNA微阵列的转录组学方案。使用这些体外方法可以评估各种QSI化合物的潜力。

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