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阴沟肠杆菌临床分离株中两种耐药机制与对亚胺培南的高水平耐药性的关联。

Association of two resistance mechanisms in a clinical isolate of Enterobacter cloacae with high-level resistance to imipenem.

作者信息

Lee E H, Nicolas M H, Kitzis M D, Pialoux G, Collatz E, Gutmann L

机构信息

Laboratoire de Microbiologie Médicale, Université Paris VI, France.

出版信息

Antimicrob Agents Chemother. 1991 Jun;35(6):1093-8. doi: 10.1128/AAC.35.6.1093.

Abstract

Carbapenem resistance was studied in a clinical isolate of Enterobacter cloacae, strain 201 (MIC of imipenem and meropenem, 16 micrograms/ml). This strain was analyzed comparatively with the carbapenem-susceptible parent strain 200, an equally susceptible revertant, 201-Rev, and in vitro-selected mutants with different levels of carbapenem resistance. All strains produced similarly high amounts of the same cephalosporinase (pIapp = 8.8). Strain 201 apparently lacked two major outer membrane proteins of ca. 37 and 38 kDa, while 201-Rev produced only the 37-kDa protein. The permeability coefficient, determined with cephaloridine, was reduced up to ninefold in the resistant strains which also showed a substantial reduction in the uptake of [14C]meropenem. The introduction of the plasmid-borne ampD gene (whose product decreases the expression of ampC) resulted in almost complete cessation of cephalosporinase production in all strains and a substantial decrease in the MICs of the carbapenems which remained, however, 8- to 16-fold higher than those determined for the susceptible strains containing the ampD gene. This "residual" resistance was attributed to reduced outer membrane permeability. The contribution of cephalosporinase production was verified in a reverse experiment, in which the introduction of ampC into a low-level cephalosporinase producer resulted in a fourfold increase in the carbapenem MICs. From these results, we infer that reduced outer membrane permeability and high-level cephalosporinase production can operate in conjunction in clinical isolates of E. cloacae to confer imipenem resistance.

摘要

对阴沟肠杆菌临床分离株201(亚胺培南和美罗培南的MIC为16微克/毫升)的碳青霉烯耐药性进行了研究。将该菌株与碳青霉烯敏感的亲本菌株200、同样敏感的回复株201-Rev以及体外筛选的具有不同水平碳青霉烯耐药性的突变体进行了比较分析。所有菌株产生的同一种头孢菌素酶量都同样高(表观pI = 8.8)。菌株201显然缺乏约37和38 kDa的两种主要外膜蛋白,而201-Rev只产生37-kDa的蛋白。用头孢菌素测定的通透系数在耐药菌株中降低了9倍,这些菌株对[14C]美罗培南的摄取也大幅减少。引入质粒携带的ampD基因(其产物可降低ampC的表达)导致所有菌株几乎完全停止产生头孢菌素酶,碳青霉烯类药物的MIC大幅降低,然而,仍比含有ampD基因的敏感菌株测定值高8至16倍。这种“残余”耐药性归因于外膜通透性降低。在反向实验中证实了头孢菌素酶产生的作用,在该实验中,将ampC引入低水平头孢菌素酶产生菌中导致碳青霉烯MIC增加了4倍。从这些结果中,我们推断外膜通透性降低和高水平头孢菌素酶产生可共同作用于阴沟肠杆菌临床分离株,使其产生亚胺培南耐药性。

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