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A Comparison of Culture- and PCR-Based Methods to Detect Six Major Non-O157 Serogroups of Shiga Toxin-Producing Escherichia coli in Cattle Feces

机译:基于文化和PCR方法检测牛粪便中产生志贺毒素的大肠杆菌的六个主要非O157血清型的比较

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摘要

Culture-based methods to detect the six major non-O157 (O26, O45, O103, O111, O121 and O145) Shiga toxin-producing E. coli (STEC) are not well established. Our objectives of this study were to develop a culture-based method to detect the six non-O157 serogroups in cattle feces and compare the detection with a PCR method. Fecal samples (n = 576) were collected in a feedlot from 24 pens during a 12-week period and enriched in E. coli broth at 40° C for 6 h. Enriched samples were subjected to immunomagnetic separation, spread-plated onto a selective chromogenic medium, and initially pooled colonies, and subsequently, single colonies were tested by a multiplex PCR targeting six serogroups and four virulence genes, stx1, stx2, eae, and ehxA (culture method). Fecal suspensions, before and after enrichment, were also tested by a multiplex PCR targeting six serogroups and four virulence genes (PCR method). There was no difference in the proportions of fecal samples that tested positive (74.3 vs. 77.4%) for one or more of the six serogroups by either culture or the PCR method. However, each method detected one or more of the six serogroups in samples that were negative by the other method. Both culture method and PCR indicated that O26, O45, and O103 were the dominant serogroups. Higher proportions (P < 0.05) of fecal samples were positive for O26 (44.4 vs. 22.7%) and O121 (22.9 vs. 2.3%) serogroups by PCR than by the culture method. None of the fecal samples contained more than four serogroups. Only a small proportion of the six serogroups (23/640; 3.6%) isolated carried Shiga toxin genes. The culture method and the PCR method detected all six serogroups in samples negative by the other method, highlighting the importance of subjecting fecal samples to both methods for accurate detection of the six non-O157 STEC in cattle feces.
机译:基于文化的检测六种主要非O157(O26,O45,O103,O111,O121和O145)志贺毒素生产大肠杆菌(STEC)的方法尚未建立。我们这项研究的目的是开发一种基于培养的方法来检测牛粪中的六个非O157血清群,并将其与PCR方法进行比较。在12周的时间内从24支猪的饲养场中收集粪便样品(n = 576),并在40°C的大肠杆菌肉汤中浓缩6小时。将富集的样品进行免疫磁分离,铺平到选择性发色培养基上,并最初合并菌落,随后通过针对6个血清群和4个毒力基因stx1,stx2,eae和ehxA(培养方法)。富集前后的粪便悬浮液也通过针对六个血清群和四个毒力基因的多重PCR(PCR方法)进行了测试。通过培养或PCR方法检测的六个血清群中的一个或多个血清阳性的粪便样本比例没有差异(74.3%:77.4%)。但是,每种方法都检测到另一种方法阴性的六个血清组中的一个或多个。培养方法和PCR均表明O26,O45和O103是主要的血清群。通过PCR,粪便样品中O26(44.4 vs. 22.7%)和O121(22.9 vs. 2.3%)血清组的阳性样品比例较高(P <0.05),比培养方法阳性。粪便样本均不超过四个血清群。分离出的六个血清群中只有一小部分(23/640; 3.6%)携带志贺毒素基因。培养方法和PCR方法通过另一种方法检测到阴性样品中的所有六个血清群,这突出了对粪便样品进行两种方法以准确检测牛粪中六种非O157 STEC的重要性。

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