Effects of Sub-Minimal Inhibitory Concentrations of Antimicrobial Agents on the Cell Surface ofKlebsiella pneumoniaeand Phagocytic Killing Activity

肺炎克雷伯菌 微生物学 抗菌剂 化学 抗菌剂 抗生素 最小抑制浓度 肠杆菌科 细菌 大肠杆菌 生物 生物化学 遗传学 基因
作者
Sachiko Nomura,K. Murata,Ariaki Nagayama
出处
期刊:Journal of Chemotherapy [Taylor & Francis]
卷期号:7 (5): 406-413 被引量:10
标识
DOI:10.1179/joc.1995.7.5.406
摘要

Changes in the phagocytic killing activity, capsule structure, and physicochemical properties such as the hydrophobicity and charge of the cell surface were studied in Klebsiella pneumoniae treated with sub-minimal inhibitory concentrations (MICs) of various antimicrobial agents. The phagocytic killing activity of macrophages was enhanced by penicillins, cephems, and monobactam in the absence of antibodies specific to the capsule or complement. No enhancement was observed with new quinolones, aminoglycosides, macrolide, or car-bapenem. The thickness of the capsule structure was considerably reduced after the treatment with penicillins, cephems, and monobactam compared with the untreated control, and it was slightly reduced by new quinolones. No changes were observed in the capsule structure with aminoglycosides, macrolide, and carbapenem. The hydrophobicity on the cell surface of the bacteria was considerably increased after the treatment with penicillins, cephems, and monobactam compared with the control, slightly increased with new quinolones and carbapenem, and not changed with aminoglycosides and macrolide. The negative charge of the cell surface of the bacteria was reduced by penicillins, cephems, and monobactam compared with the control. It was slightly reduced by new quinolones and carbapenem but was not reduced by aminoglycosides and macrolide. These findings suggest that sub-MIC beta-lactam drugs such as penicillins, cephems, and monobactams cause thinning of the capsule of K. pneumoniae with increases in the hydrophobicity and decreases in the negative charge of the cell surface, which reduces the physical repulsion between the K. pneumoniae and phagocytes and enhances the sensitivity of the bacteria to phagocytic killing activity.
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