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首页> 外文期刊>PLoS One >Development and evaluation of a loop-mediated isothermal amplification (LAMP) assay for the detection of Tomato brown rugose fruit virus (ToBRFV)
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Development and evaluation of a loop-mediated isothermal amplification (LAMP) assay for the detection of Tomato brown rugose fruit virus (ToBRFV)

机译:用于检测番茄棕色皱纹果实病毒(TOBRFV)的环介导的等温扩增(灯)测定的开发和评价

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Tomato brown rugose fruit virus (ToBRFV) is a member of Tobamovirus infecting tomato and pepper. Within North America, both the United States and Mexico consider ToBRFV to be a regulated pest. In Canada, the presence of ToBRFV has been reported, but an efficient diagnostic system has not yet been established. Here, we describe the development and assessment of a loop-mediated isothermal amplification (LAMP)-based assay to detect ToBRFV. The LAMP test was efficient and robust, and results could be obtained within 35 min with an available RNA sample. Amplification was possible when either water bath or oven were used to maintain the temperature at isothermal conditions (65°C), and results could be read by visual observation of colour change. Detection limit of the LAMP was eight target RNA molecules. Under the experimental conditions tested, LAMP was as sensitive as qPCR and 100 times more sensitive than the currently used RT-PCR. We recommend this sensitive, efficient LAMP protocol to be used for routine lab testing of ToBRFV.
机译:番茄棕色皱纹果实病毒(TOBRFV)是传染番茄和胡椒的烟草病毒的成员。在北美洲,美国和墨西哥认为泰国人是一个受管制的害虫。在加拿大,报告了烟草的存在,但尚未建立一个有效的诊断系统。在此,我们描述了基于环介导的等温扩增(灯)的开发和评估,以检测TOBRFV。灯测试是有效且稳健的,并且可以在35分钟内获得结果,可用的RNA样品。当使用水浴或烘箱将温度保持在等温条件(65℃)时,可以进行扩增,并且可以通过视觉观察颜色变化来读取结果。灯的检测极限是八个靶RNA分子。在测试的实验条件下,灯与QPCR一样敏感,比目前使用的RT-PCR更敏感100倍。我们建议使用这种敏感的有效灯具协议,用于触及的常规实验室测试。

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