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Complexity of Antibiotic Resistance in Commensal Escherichia coli Derived from Pigs from an Intensive-Production Farm

机译:集约化养殖场猪衍生的普通大肠杆菌中抗生素抗药性的复杂性

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摘要

Antibiotics in animal husbandry are used to maintain welfare, but lead to the generation of resistant strains. We analyzed commensal multidrug-resistant Escherichia coli from pigs at the beginning and end of the production cycle in a farm with a farrow-to-finish system in order to investigate whether clonal spread or horizontal gene transfer constitutes the main factor responsible for the prevalence of resistance in this environment. Among 380 isolates, 56 multidrug-resistant E. coli with a similar resistant phenotype were selected for more detailed investigations including a genomic similarity analysis and the detection of mobile elements. Isolates carried blaTEM-1, aadA1, strA/B, tetA, tetB, tetC, dfrA1, dfrA5, dfrA7, dfrA12, sul1, sul2, sul3, and qnrS resistance genes, with the common co-occurrence of genes encoding the same resistance phenotype. A pulse-field gel electrophoresis analysis of the genomic similarity of multidrug-resistant E. coli showed ≤65% similarity of most of the tested strains and did not reveal a dominant clone responsible for the prevalence of resistance. Class 1 and 2 integrons and transposons 7 and 21 were detected among mobile elements; however, some were truncated. Plasmids were represented by 11 different incompatibility groups (K, FIB, I1, FIIA, FIC, FIA, Y, P, HI1, B/O, and T). Genetic resistance traits were unevenly spread in the clonal groups and suggested the major rearrangement of genetic material by horizontal gene transfer. The present results revealed that in commensal E. coli from pigs in a homogeneous farm environment, there was no dominant clone responsible for the spread of resistance and persistence in the population.
机译:畜牧业中使用抗生素来维持福利,但会导致产生耐药菌株。为了研究克隆传播或水平基因转移是否是造成猪流行的主要因素,我们在分娩到最终系统的农场的生产周期的开始和结束时对猪的多药耐药性大肠杆菌进行了分析。在这种环境下的抵抗力。在380株分离物中,选择了56种具有相似耐药表型的耐多药大肠杆菌进行更详细的研究,包括基因组相似性分析和移动元素检测。分离株携带blaTEM-1,aadA1,strA / B,tetA,tetB,tetC,dfrA1,dfrA5,dfrA7,dfrA12,sul1,sul2,sul3和 qnrS 抗性基因编码相同抗性表型的基因。多重耐药性 E基因组相似性的脉冲场凝胶电泳分析。大肠杆菌与大多数测试菌株的相似度均≤65%,并且未发现导致耐药性流行的显性克隆。在移动元件中检测到1类和2类整合素以及转座子7和21;但是,有些被截断了。质粒由11个不同的不相容性组(K,FIB,I1,FIIA,FIC,FIA,Y,P,HI1,B / O和T)代表。遗传抗性特征在克隆组中分布不均,表明水平基因转移对遗传物质的主要重排。目前的结果表明,在 E表彰。在同质农场环境中从猪中分离出大肠埃希菌,没有显性克隆造成耐药性和持久性在种群中的传播。

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