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Detection of Novel duck reovirus (NDRV) using visual reverse transcription loop-mediated isothermal amplification (RT-LAMP)

机译:使用视觉逆转录环介导的等温扩增(RT-LAMP)检测新型鸭呼肠孤病毒(NDRV)

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摘要

Here we present a visual reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay for detecting the gene encoding the σB major outer-capsid protein of novel duck reovirus (NDRV). A set of primers, composed of two outer primers, two inner primers and two loop primers, was designed based on the gene of interest. The LAMP reaction was conducted in a traditional laboratory water bath at 65 °C for 50 min. We compared the performance of calcein/Mn2+ and SYBR Green I dyes, as well as electrophoresis on agarose gel stained with GoldView nucleic acid dye to detect the RT-LAMP-amplified products and all assays could be employed to discriminate between positive and negative specimens in visible or UV light. Our data showed that there is no cross-reaction with other viruses and the RT-LAMP technique displayed high sensitivity for detecting NDRV with a minimal detection limit of 200 fg RNA input. This assay was more sensitive than conventional PCR in detecting NDRV both in natural and experimental infection. In conclusion, the RT-LAMP technique was remarkably sensitive, specific, rapid, simple and profitable for the identification of NDRV.
机译:在这里,我们提出了一种可视逆转录环介导的等温扩增(RT-LAMP)测定法,用于检测编码新型鸭呼肠孤病毒(NDRV)的σB主要外衣壳蛋白的基因。根据目的基因设计了一组引物,该引物由两个外部引物,两个内部引物和两个环引物组成。 LAMP反应在传统的实验室水浴中于65°C进行50°min。我们比较了钙黄绿素/ Mn 2 + 和SYBR Green I染料的性能,以及在用GoldView核酸染料染色的琼脂糖凝胶上进行电泳以检测RT-LAMP扩增产物的性能,所有测定均可用于区分可见光或紫外光下的正负样本。我们的数据表明与其他病毒没有交叉反应,RT-LAMP技术显示出检测NDRV的高灵敏度,最低检测限为200 fg RNA输入。在自然和实验感染中检测NDRV时,该测定均比常规PCR灵敏。总之,RT-LAMP技术对于鉴定NDRV非常灵敏,特异,快速,简单且有利可图。

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