乳基质中肠球菌万古霉素耐药转移的临床意义评估

M. R. Terra, N. F. Tosoni, M. C. Furlaneto, L. Furlaneto-Maia
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引用次数: 3

摘要

肠球菌万古霉素耐药性的传播与可移动遗传因子的水平转移有关。本研究的目的是评价乳基质是否为支持万古霉素耐药(vanA)基因从临床万古霉素耐药粪肠球菌向万古霉素敏感粪肠球菌转移的适宜环境。首先对肠球菌菌株进行cpd(诱导性信息素决定基因)、vanA和tetL(万古霉素和四环素耐药标记)和gelE(细胞外金属内肽酶)基因的筛选,确定交配对。基于这些选择标记,我们研究了粪肠杆菌携带的8种质粒携带的vanA (vanA+、cpd-、tetL-和gelE-)在乳基质中向2种粪肠杆菌(vanA-、cpd+、tetL +和gelE+)受体菌株转移的能力。以1:1的比例在7%的重组乳中配种,37℃孵育。在孵育2小时内,所有16个配对都出现了转偶联物,并通过双抗生素耐药性(万古霉素和四环素)得到了证明。即使在非选择性培养基上10次传代后,交叉缀合物的万古霉素耐药性仍保持不变。转缀合物表达vanA、tel和gelE基因阳性。本研究提示乳基质是肠球菌间基因交换的适宜环境。
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Assessment of vancomycin resistance transfer among enterococci of clinical importance in milk matrix
Abstract Dissemination of vancomycin resistance in enterococci has been associated with horizontal transfer of mobile genetic elements. Aim of the study was to evaluate if milk matrix is a suitable environment to support transferability of vancomycin resistance (vanA) gene from clinical vancomycin-resistant Enterococcus faecium to vancomycin-sensitive Enterococcus faecalis. Enterococci strains were firstly screened for the presence of cpd (inducible sex pheromone determinant) gene, vanA and tetL genes (vancomycin and tetracycline resistance markers, respectively) and the gelE (extracellular metalloendopeptidase) gene to define the mating pairs. Based on these selection markers, we investigated the transferability of eight plasmid-borne vanA harbored by E. faecium (vanA+, cpd-, tetL- and gelE-) into two E. faecalis (vanA-, cpd+, tetL + and gelE+) recipient strains in milk matrix. The strains were mated in a 1:1 ratio in 7% reconstituted milk and incubated at 37 °C. Transconjugants emerged from all 16 matings within 2 h of incubation and were evidenced by dual antibiotic resistance (vancomycin and tetracycline). The vancomycin-resistance of trasconjugants was maintained even after ten subsequent passages on nonselective medium. Transconjugants were positive for vanA, tetL and gelE genes. This study indicates milk matrix as suitable environment to support gene exchange between Enterococcus species.
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