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首页> 外文期刊>Journal of Food Science and Technology >Evaluation and implementation of commercial antibodies for improved nanoparticle-based immunomagnetic separation and real-time PCR for faster detection of Listeria monocytogenes
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Evaluation and implementation of commercial antibodies for improved nanoparticle-based immunomagnetic separation and real-time PCR for faster detection of Listeria monocytogenes

机译:基于纳米粒子的免疫磁分离和实时PCR的商业抗体的评价与实施,以便更快地检测Histeria单核细胞增生

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摘要

L. monocytogenes continues to be a major health issue in Europe, as well as worldwide. Faster methods, not only for detection, but also for sample preparation are of great interest particularly for this slow-growing pathogen. Immunomagnetic separation has been previously reported to be an effective way to concentrate bacteria, and remove inhibitors. In the present study, different commercial antibodies were evaluated to select the most appropriate one, in order to develop a highly specific method. Additionally, magnetic nanoparticles, instead of microparticles, were selected due to their reported advantages (higher surface-volume ration and faster kinetics). Finally, the separation protocol, with a calculated capture efficiency of 95%, was combined with real-time PCR for highly sensitive detection of the concentrated bacteria. The optimized IMS-qPCR allowed to reduce hands-on time in the sample treatment, without affecting the overall performance of the method as a very low limit of detection was still obtained (9.7 CFU/ 25 g) with values for sensitivity, specificity, accuracy, positive and negative predictive values of 100%, resulting in a kappa index of concordance of 1.00. These results were obtained in spiked food samples of different types (chicken, fish, milk, hard and fresh cheese), further demonstrating the applicability of the optimized methodology presented.
机译:L.单核细胞增粒仍然是欧洲的主要健康问题,以及全世界。更快的方法,不仅用于检测,而且对于样品制备,特别是对于这种缓慢生长的病原体具有很大的兴趣。先前据报道,预先磁性分离是浓缩细菌的有效方法,并除去抑制剂。在本研究中,评价不同的商业抗体以选择最合适的商业抗体,以便开发一种高度具体的方法。另外,由于其报告的优点(较高的表面积(较高的动力学),选择磁性纳米颗粒代替微粒。最后,具有95%的计算捕获效率的分离方案与实时PCR合并,用于高敏感的浓缩细菌。优化的IMS-QPCR允许减少样品处理中的动手时间,而不会影响该方法的整体性能,因为仍然获得了敏感性,特异性,准确性的值(9.7CFU / 25g)的非常低的检测限阳性和负面预测值100%,导致kappa指数的一致性为1.00。这些结果是在不同类型的尖刺食品样品中获得(鸡肉,鱼类,牛奶,辛辣奶酪),进一步展示了所提供的优化方法的适用性。

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  • 作者单位

    Int Iberian Nanotechnol Lab Nano4Food Food Qual &

    Safety Res Grp Dept Life Sci Av Mestre Jose Veiga S-N P-4715330 Braga Portugal;

    Int Iberian Nanotechnol Lab Nano4Food Food Qual &

    Safety Res Grp Dept Life Sci Av Mestre Jose Veiga S-N P-4715330 Braga Portugal;

    Int Iberian Nanotechnol Lab Nano4Food Food Qual &

    Safety Res Grp Dept Life Sci Av Mestre Jose Veiga S-N P-4715330 Braga Portugal;

    Int Iberian Nanotechnol Lab Nano4Food Food Qual &

    Safety Res Grp Dept Life Sci Av Mestre Jose Veiga S-N P-4715330 Braga Portugal;

    Int Iberian Nanotechnol Lab Nano4Food Food Qual &

    Safety Res Grp Dept Life Sci Av Mestre Jose Veiga S-N P-4715330 Braga Portugal;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 食品工业 ;
  • 关键词

    Rapid methods; Magnetic nanoparticles; IMS-qPCR; hly; Listeria monocytogenes;

    机译:快速方法;磁性纳米颗粒;IMS-QPCR;HLY;李斯特菌单核细胞增生;

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