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首页> 外文期刊>Applied Microbiology and Biotechnology >Response surface methodology to design a selective enrichment broth for rapid detection of Salmonella spp. by SYBR Green Ι real-time PCR
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Response surface methodology to design a selective enrichment broth for rapid detection of Salmonella spp. by SYBR Green Ι real-time PCR

机译:响应面分析法设计了可快速检测沙门氏菌的选择性富集肉汤。通过SYBR GreenΙ实时PCR

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摘要

In order to meet dominant growth of Salmonella spp. in a composed system of five pathogens for accurate detection, designing an appropriate selective enrichment broth was clearly needed. First, we built a high-throughput assay procedure based on SYBR Green Ι real-time PCR, which possessed the necessary specificity for Salmonella spp., a good linear standard curve with typical R~2 value (0.9984) and high amplification efficiency (99.0 %). Further, for the larger target biomass in the mixed microflora, acarbose, LiCl and bile salt were selected to optimize their concentrations using response surface methodology (RSM). A central composite design was employed to collect the data and fit the response. A quadratic polynomial model was derived by computer simulation. Statistical analysis was carried out to explore the action and interaction of the variables on the response. In the end, a novel broth (Sal-5) was formulated to allow the efficient enrichment of Salmonella spp. and inhibit the growth of other tested strains. A detection platform was developed, including selective enrichment in Sal-5, DNA extraction by the boiling lysis method and real-time PCR test based on SYBR Green Ι. This work could extend the application of RSM and real-time PCR in the design of other selective enrichment media for common pathogens.
机译:为了满足沙门氏菌的优势生长。在由五种病原体组成的系统中以进行准确检测,显然需要设计合适的选择性富集肉汤。首先,我们建立了基于SYBR Green实时荧光定量PCR的高通量检测程序,该程序对沙门氏菌具有必要的特异性,具有典型R〜2值(0.9984)和良好的扩增效率(99.0)的良好线性标准曲线%)。此外,对于混合微生物区系中较大的目标生物量,使用响应表面方法(RSM)选择了阿卡波糖,LiCl和胆汁盐以优化其浓度。采用中央复合设计来收集数据并拟合响应。通过计算机仿真得出二次多项式模型。进行统计分析以探讨变量对响应的作用和相互作用。最后,配制了一种新型肉汤(Sal-5),可有效富集沙门氏菌。并抑制其他测试菌株的生长。开发了一种检测平台,包括选择性富集Sal-5,通过沸腾裂解法提取DNA以及基于SYBR Green I的实时PCR测试。这项工作可以扩展RSM和实时PCR在其他常见病原体选择性富集培养基设计中的应用。

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