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首页> 外文期刊>Letters in Applied Microbiology >A real-time polymerase chain reaction-based method for rapid and specific detection of spoilage Alicyclobacillus spp. in apple juice
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A real-time polymerase chain reaction-based method for rapid and specific detection of spoilage Alicyclobacillus spp. in apple juice

机译:一种基于实时聚合酶链反应的方法,用于快速,特异性地检测腐败菌脂环酸杆菌属。在苹果汁中

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摘要

Aims: To develop a real-time PCR-based rapid detection method for spoilage Alicyclobacillus spp. in juice products. Methods and Results: The squalene-hopene cyclase-encoding gene was targeted for primer-and-probe development. Gene fragments from representative strains were cloned, and PCR primers and probe were designed by DNA sequence comparison. Selected bacteria were examined for cross-reactivity by the new method. Cells wereserially diluted in apple juice and saline, and examined by the new method to establish detection sensitivity. Using the newly developed Taqman~R real-time PCR-based method, strains of Alicyclobacillus acidocaldarius and A. acidoterrestris were detected without cross reactivity with other common food-borne micro-organisms. Detection of <10 cells per PCR reaction from juice samples was accomplished within 3-5 h. Conclusion: This is the first reported real-time PCR-based detection method for Alicyclobacillus spp. and its application in juice products is demonstrated. Significance and Impact of the Study: As a favourable alternative for the laborious and time-consuming culture- or biochemical characterization-based techniques, the system has great potential for industrial applications from raw material screening to final product quality control.
机译:目的:建立基于实时PCR的腐败菌脂环菌快速检测方法。在果汁产品中。方法和结果:角鲨烯-戊环化酶编码基因的目标是引物和探针的发展。克隆了代表菌株的基因片段,并通过DNA序列比较设计了PCR引物和探针。通过新方法检查所选细菌的交叉反应性。将细胞在苹果汁和盐水中进行血清稀释,并通过新方法进行检查以建立检测灵敏度。使用新开发的基于Taqman〜R实时PCR的方法,检测到了酸热脂环酸杆菌和酸热拟南芥菌株,而没有与其他常见的食源微生物发生交叉反应。每个PCR反应中从果汁样品中检测到<10个细胞都在3-5小时内完成。结论:这是首次报道的基于实时PCR的脂环芽孢杆菌属检测方法。并演示了其在果汁产品中的应用。研究的意义和影响:作为费力且费时的基于培养或生化表征的技术的有利替代方案,该系统在从原材料筛选到最终产品质量控制的工业应用中具有巨大的潜力。

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