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荧光氨基糖苷类抗生素及准确监测细菌摄取的方法。

Fluorescent Aminoglycoside Antibiotics and Methods for Accurately Monitoring Uptake by Bacteria.

机构信息

Université Paris-Saclay, CEA, CNRS, Institute for Integrative Biology of the Cell (I2BC), 91198 Gif-sur-Yvette, France.

Université Paris-Saclay, CEA, Service de Chimie Bio-organique et de Marquage, 91191 Gif-sur-Yvette, France.

出版信息

ACS Infect Dis. 2020 May 8;6(5):1008-1017. doi: 10.1021/acsinfecdis.9b00421. Epub 2020 Mar 30.

DOI:10.1021/acsinfecdis.9b00421
PMID:32195576
Abstract

Characterizing how multidrug-resistant bacteria circumvent the action of clinically used or novel antibiotics requires a detailed understanding of how the antibiotics interact with and cross bacterial membranes to accumulate in the cells and exert their action. When monitoring the interactions of drugs with bacteria, it remains challenging to differentiate functionally relevant internalized drug levels from nonspecific binding. Fluorescence is a method of choice for observing dynamics of biomolecules. In order to facilitate studies involving aminoglycoside antibiotics, we have generated fluorescently labeled aminoglycoside derivatives with uptake and bactericidal activities similar, albeit with a moderate loss, to those of the parent drug. The method combines fluorescence microscopy with fluorescence-activated cell sorting (FACS) using neomycin coupled to nonpermeable cyanine dyes. Fluorescence imaging allowed membrane-bound antibiotic to be distinguished from molecules in the cytoplasm. Patterns of uptake were assigned to different populations in the FACS analysis. Our study illustrates how fluorescent derivatives of an aminoglycoside enable a robust characterization of the three components of uptake: membrane binding, EDPI, and EDPII. Because EDPI levels are weak compared to the two other types of accumulation and critical for the action of these drugs, the three components of uptake must be taken into account separately when drawing conclusions about aminoglycoside function.

摘要

要描述多药耐药细菌如何规避临床使用或新型抗生素的作用,需要详细了解抗生素如何与细菌膜相互作用并穿过细菌膜,从而在细胞内积累并发挥作用。在监测药物与细菌相互作用时,仍然难以将功能相关的内化药物水平与非特异性结合区分开来。荧光是观察生物分子动态的首选方法。为了便于研究氨基糖苷类抗生素,我们已经生成了荧光标记的氨基糖苷类衍生物,其摄取和杀菌活性与母体药物相似,尽管略有损失。该方法结合了荧光显微镜和使用与不可渗透的氰染料偶联的新霉素的荧光激活细胞分选(FACS)。荧光成像可区分细胞膜结合的抗生素与细胞质中的分子。摄取模式在 FACS 分析中被分配到不同的群体。我们的研究说明了氨基糖苷类抗生素的荧光衍生物如何能够对摄取的三个组成部分(膜结合、EDPI 和 EDPII)进行稳健的表征。由于与另外两种积累类型相比,EDPI 水平较弱,并且对这些药物的作用至关重要,因此在得出关于氨基糖苷类功能的结论时,必须分别考虑摄取的三个组成部分。

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