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Molecular genetic analysis of cephalosporinase production and its role in beta-lactam resistance in clinical isolates of Enterobacter cloacae.

机译:阴沟肠杆菌临床分离株中头孢菌素酶产生及其在β-内酰胺抗性中的作用的分子遗传学分析。

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摘要

Two strains of Enterobacter cloacae were isolated from a patient before (strain MHN1) and during (strain MHN2) treatment with moxalactam and gentamicin. Strain MHN1 exhibited inducible ampC cephalosporinase production. In contrast, strain MHN2 expressed the enzyme constitutively at a 3,000-fold higher level. With the Escherichia coli ampC gene as a hybridization probe it was shown that the genomic arrangement of the ampC region was the same in both strains. To gain more insight into regulatory phenomena, the ampC genes were cloned, and their expression was studied in E. coli K-12. The ampC gene from MHN1 behaved normally and conferred inducible beta-lactam resistance. A regulatory region of at least 800 base pairs involved in controlling repression-induction was located immediately upstream of ampC. Surprisingly, when present in E. coli the ampC gene from MHN2 no longer overproduced the cephalosporinase, and inducible expression was observed. This indicates that in MHN2 stable cephalosporinase overproduction is controlled by another factor which is not linked to the ampC gene.
机译:在用莫拉西坦和庆大霉素治疗之前(患者MHN1)和治疗期间(患者MHN2),从患者中分离出两株阴沟肠杆菌。菌株MHN1表现出可诱导的ampC头孢菌素酶产生。相反,菌株MHN2以3,000倍高水平组成性表达该酶。用大肠杆菌ampC基因作为杂交探针,表明在两个菌株中ampC区的基因组排列是相同的。为了深入了解调节现象,克隆了ampC基因,并在大肠杆菌K-12中研究了它们的表达。 MHN1的ampC基因表现正常,并赋予可诱导的β-内酰胺抗性。至少800个碱基对的调控区位于ampC的上游。令人惊讶地,当存在于大肠杆菌中时,来自MHN2的ampC基因不再过量产生头孢菌素酶,并且观察到诱导型表达。这表明在MHN2中,稳定的头孢菌素酶的过量生产受到另一个与ampC基因无关的因素控制。

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