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Identification of Viable Listeria Species Based on Reverse Transcription-Multiplex PCR (RT-MPCR) and Restriction Digestion

机译:基于逆转录多重PCR(RT-MPCR)和限制性消化的活李斯特菌物种鉴定

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摘要

A novel method for the identification of viable Listeria species was developed based on reverse transcription-multiplex PCR (RT-MPCR) and restriction digestion. The targets for RT-MPCR were iap mRNAs whose genes are common to all Liseria species. A set of five primers was used in this study. Two of them were genus specific, and the other three were specific to L. mono-cytogenase, L. innocua, and L. grayi respectively. By RT-MPCR, L. monocytogenese, L. innocua, L. grayi, and a group of Listeria species, including L. ivanovii, L. welshimeri, and L. seeligeri, were specifically identified. To differentiate the latter three Listeria species, RT-MPCR products were subjected to digestion with HpaI and ScaI. The sensitivity of RT-MPCR in detecting Listeria species was determined to be 50 CFU/mL. RT-MPCR was found to discriminate between viable and nonviable cells and to detect viable Listeria species in a food model.
机译:基于逆转录多重PCR(RT-MPCR)和限制性酶切,开发了一种鉴定李斯特菌活菌的新方法。 RT-MPCR的靶标是Iap mRNA,其基因对所有痢疾杆菌属都是共有的。在这项研究中使用了一组五个引物。它们中的两个是属特异性的,另外三个分别是单核细胞增生李斯特菌,无毒李斯特菌和灰质李斯特菌的特异性。通过RT-MPCR,特异性地鉴定了单核细胞增生李斯特菌,无毒李斯特菌,灰色李斯特菌和一组利斯特氏菌属种,包括伊凡诺氏杆菌,welshimeri和L. seeligeri。为了区分后三种李斯特菌,RT-MPCR产物用HpaI和ScaI消化。 RT-MPCR在检测李斯特菌物种中的灵敏度确定为50 CFU / mL。发现RT-MPCR可以区分存活细胞和不存活细胞,并可以在食物模型中检测存活李斯特菌。

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