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首页> 外文期刊>Journal of Virological Methods >In-field capable loop-mediated isothermal amplification detection of Turnip yellows virus in plants and its principal aphid vector Myzus persicae
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In-field capable loop-mediated isothermal amplification detection of Turnip yellows virus in plants and its principal aphid vector Myzus persicae

机译:植物中萝卜黄色病毒的现场能力的循环介导的等温扩增检测及其主要蚜虫载体肌酐

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Widespread Turnip yellows virus (TuYV) infection causes severe seed yield and quality losses in rapeseed (Brassica napus) crops grown in broadacre agricultural systems worldwide. Current TuYV detection protocols are expensive and time consuming, and can have poor specificity and sensitivity. Typically, they are used as a diagnostic tool to test already symptomatic plants, limiting their practical value to reactive disease management. To improve diagnostic services so that they provide earlier, cheaper, faster, more specific and sensitive TuYV detection, novel and innovative protocols that utilise new technology are required. A reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed to detect TuYV in crude and total RNA extractions of leaf material and its principal aphid vector Myzus persicae. The assay was based on a set of six primers, highly sensitive and specific to TuYV, derived from a TuYV isolate originating from the south-west Australian grainbelt. TuYV was readily detected in 1 in 100 dilutions of (i) infected to uninfected leaf material, and (ii) viruliferous to non-viruliferous M. persicae. Furthermore, detection was successful in a majority of aphids stored for at least 8 weeks in various trapping and storage substances, including 30% ethylene glycol, sticky trap glue and 70% ethanol. This RT-LAMP assay protocol enables quicker and cheaper diagnosis for TuYV than currently adopted laboratory-based diagnostic techniques. Ultimately, it has the potential for earlier in-field TuYV detection in combination with aphid trapping surveillance programs.
机译:广泛的萝卜yellows病毒(Tuyv)感染导致在全球崎岖农业系统中生长的油菜籽(Brassica Napus)作物的严重种子产量和质量损失。目前的TUYV检测协议是昂贵且耗时的,并且可以具有差的特异性和灵敏度。通常,它们被用作诊断工具来测试已经有症状的植物,限制了它们对反应性疾病管理的实际价值。为了改善诊断服务,使他们提供更早,更便宜,更快,更具体,更敏感的TUYV检测,新颖和创新协议,即利用新技术。开发了逆转录回归介导的等温扩增(RT灯)测定以检测叶片材料的原油和总RNA萃取的TuyV及其主要蚜虫载体肌肌瘤。该测定基于一组六个引物,高度敏感和特异于Tuyv,来自于源自西南澳大利亚谷物斑纹的Tuyv隔离物。 Tuyv在感染未感染的叶片材料的100个(I)中,在100次(I)中,viruligibers viguligibers persicae viguliberation。此外,检测在各种捕集物质中储存至少8周的大多数蚜虫中,包括30%乙二醇,粘滞捕集胶和70%乙醇。该RT-LAMP测定协议可以更快和更便宜地对TUYV诊断而不是目前采用的基于实验室的诊断技术。最终,它具有早期的现场TUYV检测与蚜虫捕获监控程序的潜力。

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