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一种来自乳品屎肠球菌分离株的、持续性、毒素-抗毒素系统独立、编码四环素抗性的质粒。

Persistent, toxin-antitoxin system-independent, tetracycline resistance-encoding plasmid from a dairy Enterococcus faecium isolate.

机构信息

Department of Food Science, The Ohio State University, Columbus, OH 43210-1007, USA.

出版信息

Appl Environ Microbiol. 2011 Oct;77(20):7096-103. doi: 10.1128/AEM.05168-11. Epub 2011 Jul 22.

Abstract

A tetracycline-resistant (Tet(r)) dairy Enterococcus faecium isolate designated M7M2 was found to carry both tet(M) and tet(L) genes on a 19.6-kb plasmid. After consecutive transfer in the absence of tetracycline, the resistance-encoding plasmid persisted in 99% of the progenies. DNA sequence analysis revealed that the 19.6-kb plasmid contained 28 open reading frames (ORFs), including a tet(M)-tet(L)-mob gene cluster, as well as a 10.6-kb backbone highly homologous (99.9%) to the reported plasmid pRE25, but without an identified toxin-antitoxin (TA) plasmid stabilization system. The derived backbone plasmid without the Tet(r) determinants exhibited a 100% retention rate in the presence of acridine orange, suggesting the presence of a TA-independent plasmid stabilization mechanism, with its impact on the persistence of a broad spectrum of resistance-encoding traits still to be elucidated. The tet(M)-tet(L) gene cluster from M7M2 was functional and transmissible and led to acquired resistance in Enterococcus faecalis OG1RF by electroporation and in Streptococcus mutans UA159 by natural transformation. Southern hybridization showed that both the tet(M) and tet(L) genes were integrated into the chromosome of S. mutans UA159, while the whole plasmid was transferred to and retained in E. faecalis OG1RF. Quantitative real-time reverse transcription-PCR (RT-PCR) indicated tetracycline-induced transcription of both the tet(M) and tet(L) genes of pM7M2. The results indicated that multiple mechanisms might have contributed to the persistence of antibiotic resistance-encoding genes and that the plasmids pM7M2, pIP816, and pRE25 are likely correlated evolutionarily.

摘要

一株四环素耐药(Tet(r))的牛奶屎肠球菌 M7M2 分离株被发现携带 tet(M)和 tet(L)基因,位于一个 19.6kb 的质粒上。在没有四环素的连续传代后,耐药编码质粒在 99%的后代中得以保留。DNA 序列分析表明,19.6kb 的质粒包含 28 个开放阅读框(ORFs),包括 tet(M)-tet(L)-mob 基因簇,以及与报道的质粒 pRE25 高度同源(99.9%)的 10.6kb 骨架,但没有鉴定出毒素-抗毒素(TA)质粒稳定系统。在吖啶橙存在的情况下,没有 Tet(r)决定因素的衍生骨架质粒保留率为 100%,表明存在一种 TA 独立的质粒稳定机制,其对广谱耐药编码特征的持续存在的影响仍有待阐明。M7M2 的 tet(M)-tet(L)基因簇具有功能和可转移性,并通过电穿孔导致粪肠球菌 OG1RF 获得耐药性,通过自然转化导致变形链球菌 UA159 获得耐药性。Southern 杂交表明,tet(M)和 tet(L)基因都整合到变形链球菌 UA159 的染色体中,而整个质粒被转移到并保留在粪肠球菌 OG1RF 中。定量实时 RT-PCR(RT-PCR)表明,四环素诱导了 pM7M2 中 tet(M)和 tet(L)基因的转录。结果表明,多种机制可能有助于抗生素耐药编码基因的持续存在,并且质粒 pM7M2、pIP816 和 pRE25 可能在进化上相关。

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