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Detection of bioterror agents in air samples using real-time PCR.

机译:使用实时PCR检测空气样本中的生物恐怖剂。

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Aims: To use real-time PCR for the detection of bacterial bioterror agents in a liquid air sample containing potential airborne interferences, including bacteria, without the need for DNA extraction. Methods and Results: Bacteria in air were isolated after passive sedimentation onto R2A agar plates and characterized by 16S rRNA sequencing. Real-time PCR was used to identify different bacterial bioterror agents in an artificial air sample consisting of a liquid air sample and a mixture of miscellaneous airborne bacteria showing different colony morphology on R2A agar plates. No time-consuming DNA extraction was performed. Specifically designed fluorescent hybridization probes were used for identification. Conclusions: Fourteen different bacterial genera were classified by 16S rRNA gene sequencing of selected bacterial colonies showing growth on R2A agar plates. Real-time PCR amplification of all the bacterial bioterror agents was successfully obtained in the artificial air sample containing commonly found airborne bacteria and other potential airborne PCR interferences. Significance and Impact of the Study: Bacterial bioterror agents can be detected within 1 h in a liquid air sample containing a variety of commonly found airborne bacteria using real-time PCR. Airborne viable bacteria at Kjeller (Norway) were classified to the genera level using 16S rRNA gene sequencing.
机译:目的:使用实时PCR检测含有潜在空气传播干扰物(包括细菌)的液态空气样品中的细菌生物恐怖剂,而无需提取DNA。方法和结果:将细菌被动沉降到R2A琼脂平板上后分离出空气中的细菌,并通过16S rRNA测序对其进行了表征。实时荧光定量PCR用于鉴定人工空气样品中的不同细菌生物恐怖剂,该人工空气样品由液体空气样品和其他杂种空气传播细菌的混合物组成,在R2A琼脂平板上显示出不同的菌落形态。没有进行费时的DNA提取。使用专门设计的荧光杂交探针进行鉴定。结论:通过选择的细菌菌落的16S rRNA基因测序对14个不同的细菌属进行了分类,这些菌落在R2A琼脂板上生长。在包含常见空气传播细菌和其他潜在空气传播PCR干扰的人工空气样品中,成功获得了所有细菌生物恐怖剂的实时PCR扩增。研究的意义和影响:使用实时荧光定量PCR可在包含多种常见空气传播细菌的液态空气样本中1小时内检测到细菌生物恐怖剂。使用16S rRNA基因测序将Kjeller(挪威)的空气传播活细菌分类到属水平。

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