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Development and validation of a multiplex PCR-based DNA microarray hybridisation method for detecting bacterial antibiotic resistance genes in cheese

机译:开发和验证基于多重PCR的DNA微阵列杂交方法来检测奶酪中的细菌抗生素抗性基因

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摘要

The aim of this study was to develop a method for detecting antibiotic resistance (AR) genes in cheese based on a combination of multiplex PCR and a DNA microarray hybridisation system. Twenty oligonucleotide probes were designed targeting 10 common AR genes, namely aac(6′)-Ie-aph(2″)-Ia, aadE, aphA-3, ermB, tet(L), tet(M), tet(O), tet(S), vanA and vanB. Specificity of the probes was tested by hybridising against DNA from Enterococcus strains harbouring known AR genes. DNA was labelled through two multiplex PCR reactions with fluorescent nucleotides and specific primers flanking the probe sequences. Sensitivity of the microarray was assessed by contamination of a cheese with an Enterococcus faecium strain carrying vanA gene. Two tetracycline resistance genes, tet(M) and tet(S), proved to be present in a series of retail cheeses, while genes aadE, aphA3, ermB, tet(L) and tet(O) were occasionally detected. This method is envisioned as a valuable tool for identification of AR genes in foods. © 2010 Elsevier Ltd.
机译:这项研究的目的是基于多重PCR和DNA微阵列杂交系统的组合,开发一种检测奶酪中抗生素抗性(AR)基因的方法。设计了针对20个常见AR基因的20个寡核苷酸探针,即aac(6')-Ie-aph(2'')-Ia,aadE,aphA-3,ermB,tet(L),tet(M),tet(O) ,tet(S),vanA和vanB。通过与来自携带已知AR基因的肠球菌菌株的DNA杂交来测试探针的特异性。通过两次多重PCR反应,使用荧光核苷酸和探针序列两侧的特异性引物标记DNA。通过用携带vanA基因的粪肠球菌菌株对干酪的污染来评估微阵列的敏感性。证明一系列零售奶酪中存在两个四环素抗性基因tet(M)和tet(S),而偶尔检测到基因aadE,aphA3,ermB,tet(L)和tet(O)。该方法被认为是鉴定食品中AR基因的有价值的工具。 ©2010爱思唯尔有限公司。

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