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Stress-Based Identification and Classification of Antibacterial Agents: Second-Generation Escherichia coli Reporter Strains and Optimization of Detection

机译:基于压力的抗菌剂鉴定和分类:第二代大肠杆菌报告菌株和检测优化

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摘要

Escherichia coli strains bearing single-copy fusions between the lacZ reporter gene and the cspA, ibp, or P3rpoH stress promoters offer a simple means to detect sublethal concentrations of antibacterial agents interfering with prokaryotic translation or cell envelope integrity while simultaneously providing information on the mechanism of action of the test compound (A. A. Bianchi and F. Baneyx, Appl. Environ. Microbiol. >65:5023-5027, 1999). Here, we expand the usefulness of this system by (i) demonstrating that a fusion between the SOS-inducible sulA promoter and lacZ is a highly specific probe for the detection of antimicrobial agents that ultimately interfere with DNA replication, (ii) showing that inactivation of the tolC gene allows efficient detection of very low concentrations of model antibiotics (including aminoglycosides) whereas polymyxin B-mediated outer membrane permeabilization facilitates the identification of intermediate concentrations of hydrophobic compounds, and (iii) validating the potential of detector strains and sensitization strategies for high-throughput screening using a reproducible and internally consistent 96-well microplate assay.
机译:带有lacZ报告基因和cspA,ibp或P3rpoH应激启动子之间单拷贝融合的大肠杆菌菌株提供了一种简单的方法来检测亚致死浓度的抗菌剂干扰原核翻译或细胞包膜完整性,同时提供有关测试化合物的作用(AA Bianchi和F.Baneyx,Appl.Environ.Microbiol。> 65: 5023-5027,1999)。在这里,我们通过(i)证明SOS诱导的sulA启动子和lacZ之间的融合是一种高度特异性的探针来检测最终干扰DNA复制的抗微生物剂,(ii)证明了这种失活作用,扩大了该系统的实用性。 tolC基因的表达允许有效检测极低浓度的模型抗生素(包括氨基糖苷),而多粘菌素B介导的外膜通透性有助于鉴定中等浓度的疏水性化合物,并且(iii)验证了检测菌株的潜力和针对使用可重复且内部一致的96孔微孔板检测进行高通量筛选。

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