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Nucleotide sequences of 16 transmissible plasmids identified in nine multidrug-resistant Escherichia coli isolates expressing an ESBL phenotype isolated from food-producing animals and healthy humans

机译:在9种耐多药大肠杆菌菌株中鉴定出16种可传播质粒的核苷酸序列,这些菌株表达了从食品生产动物和健康人中分离出的ESBL表型

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摘要

Objectives Nine extended-spectrum β-lactamase (ESBL)-producing Escherichia coli isolated from healthy humans and food-producing animals were found to transfer their cefotaxime resistance marker at high frequency in laboratory conjugation experiments. The objective of this study was to completely characterize 16 transmissible plasmids that were detected in these bacterial isolates. Methods The nucleotide sequences of all 16 plasmids were determined from transconjugants using next-generation sequencing technology. Open reading frames were assigned using Rapid Annotation using Subsystem Technology and analysed by BLASTn and BLASTp. The standard method was used for plasmid multilocus sequence typing (pMLST) analysis. Plasmid structures were subsequently confirmed by PCR amplification of selected regions. Results The complete circularized nucleotide sequence of 14 plasmids was determined, along with that of a further two plasmids that could not be confirmed as closed. These ranged in size from 1.8 to 166.6 kb. Incompatibility groups and pMLSTs identified included IncI1/ST3, IncI1/ST36, IncN/ST1, IncF and IncB/O, and those of the same Inc types presented a similar backbone structure despite being isolated from different sources. Eight plasmids contained blaCTX-M-1 genes that were associated with either ISEcp1 or IS26 insertion sequence elements. Six plasmids isolated from humans and chickens were identical or closely related to the IncI1 reference plasmid, R64. Conclusions These data, based on comparative sequence analysis, highlight the successful spread of blaESBL-harbouring plasmids of different Inc types among isolates of human and food-producing animal origin and provide further evidence for potential dissemination routes
机译:目的在实验室结合实验中,从健康人和产食动物中分离出的九种产广谱β-内酰胺酶(ESBL)大肠杆菌被高频转移其头孢噻肟抗性标记。这项研究的目的是完全鉴定在这些细菌分离物中检测到的16种可传播质粒。方法采用下一代测序技术,从转接合子中确定全部16个质粒的核苷酸序列。使用子系统技术使用快速注释分配开放阅读框,并通过BLASTn和BLASTp分析。标准方法用于质粒多基因座序列分型(pMLST)分析。随后通过PCR扩增所选区域来确认质粒结构。结果确定了14个质粒的完整环化核苷酸序列,以及另外两个无法确认为封闭的质粒。它们的大小在1.8到166.6 kb之间。鉴定出的不相容性基团和pMLST包括IncI1 / ST3,IncI1 / ST36,IncN / ST1,IncF和IncB / O,尽管来自不同来源,但具有相同Inc.类型的那些都表现出相似的骨架结构。八个质粒包含与ISEcp1或IS26插入序列元件相关的blaCTX-M-1基因。从人和鸡中分离的六个质粒与IncI1参考质粒R64相同或密切相关。结论基于比较序列分析的这些数据突出了不同Inc类型的blaESBL携带质粒在人和食源性动物来源的分离物中的成功传播,并为潜在的传播途径提供了进一步的证据

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