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革兰氏阴性菌外膜和内膜通透性的同步测量

Contemporaneous Measurement of Outer and Inner Membrane Permeability in Gram-negative Bacteria.

作者信息

Ma Bo, Fang Chao, Zhang Jing, Wang Mingzhi, Luo Xiaoxing, Hou Zheng

机构信息

Department of Pharmacology, School of Pharmacy, Fourth Military Medical University, Xi'an, China.

Department of Nephroloy and Endocrinology, No. 371 Central Hospital of People's Liberation Army, Xinxiang, Henan, China.

出版信息

Bio Protoc. 2020 Mar 5;10(5):e3548. doi: 10.21769/BioProtoc.3548.

Abstract

The emergence and rapid spread of multidrug resistance in bacteria have led to the urgent need for novel antibacterial agents. Membrane permeabilization is the mechanism for many antibacterial molecules that are being developed against gram-negative bacteria. Thus, to determine the efficacy of a potential antibacterial molecule, it is important to assess the change in bacterial membrane permeability after treatment. This study describes the protocol for the assays of outer and inner membrane permeability using the fluorescent probes N-phenyl-1-naphthylamine and propidium iodide. Compared with other experiments, such as electron microscopy and the assay of minimal bactericidal concentration, this methodology provides a simpler, faster, and cost-effective way of estimating the membrane-permeabilizing effect and bactericidal efficacy of antibacterial molecules. This study presents an optimized protocol with respect to the classical protocols by incubating bacteria with antibacterial molecules in the culture condition identical to that of antibacterial assays and then detecting the signal of the fluorescent probe in the buffer without broth and antibacterial molecules. This protocol avoids the effect of nutrient deficiency on the physiological status of bacteria and the interference of antibacterial molecules towards the fluorescent probe. Thus, this method can effectively and precisely evaluate the membrane permeability and match the results obtained from other antibacterial assays, such as minimum inhibitory concentration and time-kill curve assays.

摘要

细菌中多重耐药性的出现和迅速传播导致了对新型抗菌剂的迫切需求。膜通透性改变是许多正在研发的针对革兰氏阴性菌的抗菌分子的作用机制。因此,为了确定一种潜在抗菌分子的疗效,评估处理后细菌膜通透性的变化很重要。本研究描述了使用荧光探针N-苯基-1-萘胺和碘化丙啶测定外膜和内膜通透性的实验方案。与其他实验(如电子显微镜和最低杀菌浓度测定)相比,该方法提供了一种更简单、快速且经济高效的方式来评估抗菌分子的膜通透作用和杀菌效果。本研究针对经典方案提出了一种优化方案,即在与抗菌试验相同的培养条件下,将细菌与抗菌分子孵育,然后在不含肉汤和抗菌分子的缓冲液中检测荧光探针的信号。该方案避免了营养缺乏对细菌生理状态的影响以及抗菌分子对荧光探针的干扰。因此,该方法可以有效且精确地评估膜通透性,并与其他抗菌试验(如最低抑菌浓度和时间-杀菌曲线试验)所得结果相匹配。

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