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利用逆转录环介导等温扩增法快速检测葡萄扇叶病相关病毒 3 型。

Rapid detection of Grapevine leafroll-associated virus type 3 using a reverse transcription loop-mediated amplification method.

机构信息

University of Pretoria, Department of Microbiology and Plant Pathology, Pretoria, South Africa.

出版信息

J Virol Methods. 2013 Dec;194(1-2):308-16. doi: 10.1016/j.jviromet.2013.08.030. Epub 2013 Sep 8.

DOI:10.1016/j.jviromet.2013.08.030
PMID:24025344
Abstract

Grapevine leafroll disease (GLD) is the most important disease of Grapevines in South Africa. Grapevine leafroll-associated virus type 3 (GLRaV-3) has a close association with the disease and is prevalent in South African vineyards. GLD can be controlled using a combination of virus-free planting material, systemic insecticides to control vector populations and removal of infected vines by roguing. Infected vines are identified each autumn using either symptom display (in red cultivars) or ELISA (in white cultivars). While ELISA is a simple, reliable means of testing for GLRaV-3, it is time consuming, laborious and insensitive and a quicker, more sensitive method of detecting GLRaV-3 in the field is needed. A single-tube one-step reverse transcription (RT) loop-mediated isothermal amplification (LAMP) assay combined with a simple RNA extraction protocol was developed for the rapid and easy detection of GLRaV-3. Hydroxy napthol blue was included as an indicator and under isothermal conditions at 60 °C the target viral gene could be amplified in under 2h and positive results could be easily seen by examining the colour change from violet to sky blue. Using this method, 50 samples could be also pooled together with a single positive sample still being detected. A direct comparison of ELISA, nested PCR and RT-LAMP showed that RT-LAMP is as sensitive as nested PCR and could be performed in a much shorter time with less equipment. This assay is may be a possible alternative to ELISA for the detection of GLRaV-3 in the field.

摘要

葡萄卷叶病(GLD)是南非葡萄最重要的病害。与该病害密切相关的葡萄卷叶相关病毒 3 型(GLRaV-3)在南非葡萄园普遍存在。通过使用无病毒种植材料、防治传毒昆虫的系统性杀虫剂以及拔除感染植株(病株)的综合措施可以控制 GLD。每年秋季,通过症状表现(红葡萄品种)或酶联免疫吸附试验(ELISA,白葡萄品种)来识别感染植株。ELISA 是检测 GLRaV-3 的一种简单、可靠方法,但耗时、费力且不敏感,因此需要一种更快速、更敏感的田间检测 GLRaV-3 的方法。本研究开发了一种单管一步逆转录环介导等温扩增(RT-LAMP)检测方法,结合简单的 RNA 提取方案,用于快速、简便地检测 GLRaV-3。羟基萘酚蓝被用作指示剂,在 60°C 的等温条件下,目标病毒基因可在 2 小时内扩增,通过观察颜色从紫色变为天蓝色,可轻松判断阳性结果。使用该方法,可将 50 个样本混合在一起,即使有一个阳性样本也能被检测到。ELISA、巢式 PCR 和 RT-LAMP 的直接比较表明,RT-LAMP 与巢式 PCR 一样敏感,且用时更短,所需设备更少。该检测方法可能是 ELISA 的一种替代方法,可用于田间 GLRaV-3 的检测。

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