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Development of a multiplex loop-mediated isothermal amplification method for the simultaneous detection of Salmonella spp. and Vibrio parahaemolyticus

机译:同时检测沙门氏菌的多重环介导的等温扩增方法的开发。和副溶血性弧菌

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摘要

Rapid detection of food-borne pathogens is important in the food industry, to monitor and prevent the spread of these pathogens through contaminated food products. We therefore established a multiplex real-time loop-mediated isothermal amplification (LAMP) assay to simultaneously detect and distinguish Salmonella spp. and Vibrio parahaemolyticus DNA in a single reaction. Two target sequences, one specific for Salmonella and the other specific for Vibrio parahaemolyticus, were amplified by specific LAMP primers in the same reaction tube. After amplification at 65 °C for 60 min, the amplified products were subjected to melting curve analysis and thus could be distinguished based on the different melting temperatures (Tm values) of the two specifically amplified products. The specificity of the multiplex LAMP assay was evaluated using 19 known bacterial strains, including one V. parahaemolyticus and seven Salmonella spp. strains. The multiplex LAMP showed 100% inclusivity and exclusivity, and a detection limit similar to that of multiplex PCR. In addition, we observed and corrected preferential amplification induced by what we call LAMP selection in the multiplex LAMP reaction. In conclusion, our assay was rapid, specific, and quantitative, making it a useful tool for the food industry.
机译:食源性病原体的快速检测在食品工业中很重要,以监视和防止这些病原体通过受污染的食品传播。因此,我们建立了多重实时环介导的等温扩增(LAMP)分析方法,以同时检测和区分沙门氏菌。与副溶血弧菌DNA在一个反应​​中。在同一反应管中,通过特异性LAMP引物扩增了两个靶序列,一个对沙门氏菌具有特异性,而另一个对副溶血弧菌具有特异性。在65°C下扩增60分钟后,对扩增产物进行了熔解曲线分析,因此可以根据两种特异性扩增产物的不同熔解温度(Tm值)进行区分。使用19种已知细菌菌株(包括1种副溶血弧菌和7种沙门氏菌)评估了多重LAMP分析的特异性。株。多重LAMP表现出100%的包容性和排他性,检测限与多重PCR相似。此外,我们观察并纠正了由多重LAMP反应中所谓的LAMP选择引起的优先扩增。总之,我们的测定是快速,特异性和定量的,使其成为食品工业的有用工具。

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