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首页> 外文期刊>Journal of Microbiological Methods >Assessment of two selective agar media to isolate colistin-resistant bovine Escherichia coli: Correlation with minimal inhibitory concentration and presence of mcr genes
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Assessment of two selective agar media to isolate colistin-resistant bovine Escherichia coli: Correlation with minimal inhibitory concentration and presence of mcr genes

机译:评估两种选择性琼脂培养基,分离耐菌腐植牛大肠杆菌:与最小抑制浓度和MCR基因存在的相关性

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摘要

The identification of colistin-resistant enterobacteria in veterinary medicine is impaired by the absence of first line reliable phenotypic assay. The purpose of this study was to assess two selective agar media for the detection of colistin-resistant bovine pathogenic Escherichia coli. A total of 158 E. coli (46 R resistant >, 96 I intermediate > and 16 S sensitive > at the disk diffusion assay) isolated between 2013 and 2018 from 3 month-old calves suffering enteritis or septicaemia, were (i) tested by the broth dilution assay to determine colistin Minimal Inhibitory Concentrations (MIC); (ii) streaked on CHROMID (R) Colistin_R and CHROMagar (TM) COL-APSE agar plates; (iii) submitted to a pentaplex PCR to identify the presence of mcr-1 to mcr-5 genes. Of the 92 E. coli growing on both agar media, 90 had a MIC > 2.0 mu g/ml as had the 3 E. coli that grew only on the CHROMID (R) Colistin_R agar medium and one E. coil that grew on neither agar media. Therefore, the positive predictive values of the CHROMID Colistin_R and CHROMagarr (TM) COL-APSE agar media were both 0.98 whereas their negative predictive values were 0.98 and 0.94, respectively. Also noteworthy 43 of the 46 R isolates had a MIC > 2.0 mu g/ml and grew on both selective media as did half of the 96 I isolates and only 1 of the S isolates. Conversely, only 30 of the 90 isolates that grew on both agar media and with a MIC > 2.0 mu g/ml tested positive for the mcr-1 or mcr-2 genes with the pentaplex PCR. These two selective agar media can be used to reliably detect colistin-resistant E. coli. Positive growth was highly correlated with R results at the disk diffusion assay, but not with the presence of mcr genes.
机译:通过缺乏第一线可靠的表型测定,耐兽药抗肠细菌的鉴定受到抑制。本研究的目的是评估两种选择性琼脂培养基,用于检测耐霉素抵抗牛病原体大肠杆菌。总共158大肠杆菌(46 r&抗性>,96 i&中间>和16 s&敏感>在磁盘扩散测定中,来自磁盘扩散测定)来自& 3个月大的小腿患有肠炎或败血症,是(i)通过肉汤稀释测定测试,以确定Colistin最小抑制浓度(MIC); (ii)在染色体(r)colistin_r和chromagar(tm)col-apse琼脂板上划为; (iii)将Pentaplex PCR提交以鉴定MCR-1至MCR-5基因的存在。在两个琼脂培养基上生长的92大肠杆菌中,90具有麦克风>2.0μg/ ml,只有在染色体(r)colistin_r琼脂培养基和一个既不长的卷线上琼脂媒体。因此,染色体Colistin_R和ChromaGarr(TM)COL-APSE琼脂介质的阳性预测值均为0.98,而它们的阴性预测值分别为0.98和0.94。 46 R分离物中的43个中也有一个MIC>2.0μg/ ml,并在两种选择介质上增长,如96 I隔离的一半,也只有1个分离物。相反,在琼脂培养基上增加了90个分离物中的30个,并且用Pentaplex PCR测试MCR-1或MCR-2基因的阳性Mur>2.0μg/ ml。这两个选择性琼脂培养基可用于可靠地检测耐霉菌的大肠杆菌。阳性生长与磁盘扩散测定的R导点高度相关,但不存在MCR基因的存在。

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