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利用实时 PCR 结合免疫磁分离和全基因组扩增技术快速检测家禽环境样本中的沙门氏菌。

Rapid detection of Salmonella in poultry environmental samples using real-time PCR coupled with immunomagnetic separation and whole genome amplification.

机构信息

Center for Food Safety, Department of Food Science and Technology, University of Georgia, Griffin, GA 30223.

Department of Poultry Science, University of Georgia, Athens, GA 30602.

出版信息

Poult Sci. 2019 Dec 1;98(12):6973-6979. doi: 10.3382/ps/pez425.

Abstract

We evaluated the combination of immunomagnetic separation (IMS), multiple displacement amplification (MDA), and real-time PCR to detect Salmonella from poultry environmental samples. The limits of detection (LODs) of IMS-MDA real-time PCR with different culture enrichment hours (0, 4, 6, and 8 h) were determined in artificially inoculated litter samples from a specific pathogen-free (SPF) poultry farm. In addition, Salmonella detection rate of IMS-MDA real-time PCR with 8-h culture enrichment was compared with that of conventional real-time PCR and culture-based detection by analyzing 174 poultry environmental samples (boot swabs, drag swabs, and litter), and the levels of Salmonella in the samples were quantified using the most probably number method. The LODs of IMS-MDA real-time PCR with 0, 4 to 6, and 8-h enrichment were 10, 1, and 0.1 CFU/g, respectively. Salmonella was detected in 25 of the 174 environmental samples (14.4%) by IMS-MDA real-time PCR, compared with 24 (13.8%) by conventional real-time PCR and 19 (10.9%) by culturing. Cohen's kappa index indicated strong concordance (0.79) between IMS-MDA real-time PCR and culture detection. We demonstrated the potential of the IMS-MDA real-time PCR assay as a faster and more sensitive alternative to culture-based Salmonella detection from poultry environmental samples.

摘要

我们评估了免疫磁分离(IMS)、多次置换扩增(MDA)和实时 PCR 的组合,以检测家禽环境样本中的沙门氏菌。在特定无病原体(SPF)家禽养殖场的人工接种垫料样本中,确定了不同培养富集时间(0、4、6 和 8 小时)的 IMS-MDA 实时 PCR 的检测限(LOD)。此外,通过分析 174 份家禽环境样本(靴拭子、拖拭子和垫料),比较了 8 小时培养富集的 IMS-MDA 实时 PCR 与传统实时 PCR 和基于培养的检测方法的沙门氏菌检测率,并使用最可能数法定量样本中的沙门氏菌水平。0、4 至 6 和 8 小时富集的 IMS-MDA 实时 PCR 的 LOD 分别为 10、1 和 0.1 CFU/g。在 174 份环境样本中,有 25 份(14.4%)通过 IMS-MDA 实时 PCR 检测到沙门氏菌,而通过传统实时 PCR 检测到 24 份(13.8%),通过培养检测到 19 份(10.9%)。Cohen's kappa 指数表明 IMS-MDA 实时 PCR 与培养检测之间具有很强的一致性(0.79)。我们证明了 IMS-MDA 实时 PCR 检测法作为一种更快、更敏感的替代方法,用于从家禽环境样本中检测沙门氏菌的潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8ac2/8913963/83e180bae697/gr1.jpg

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