A Precise TaqMan-Based Real-Time qPCR Assay for Detecting and Quantifying Blackberry Chlorotic Ringspot Virus, Blueberry Shock Virus, and Plum Pox Virus in Fruit Tree Seedlings.

IF 2.5 3区 农林科学 Q2 PLANT SCIENCES
Na Hee Kim, Minhue Jung, Seung Hyeon Oh, Kook-Hyung Kim
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引用次数: 0

Abstract

We developed a rapid and efficient TaqMan-based realtime reverse transcription quantitative PCR (RT-qPCR) assay for the detection and quantification of viruses infecting fruit trees, including blackberry chlorotic ringspot virus (BCRV), blueberry shock virus (BlShV), and plum pox virus (PPV). The detection limits for each virus were 40 copies (BCRV), 500 copies (BlShV), and 40 copies (PPV), respectively. Two primer-probe sets were selected for each virus, with amplification efficiencies ranging from 90-110%. High specificity was confirmed against other viruses or viroids sharing the same host plants. Multiplex detection of BCRV, BlShV, and PPV was achieved by using FAM and Cy5 fluorescent dyes. All sets maintained high efficiency and sensitivity with varying amounts of RNA extracted from the woody branches of the host plant. This assay will be useful for rapid and accurate diagnosis of plant virus diseases, especially in quarantine stations where leaf tissue is often unavailable upon import.

基于taqman的果树幼苗中黑莓绿斑病毒、蓝莓休克病毒和李子痘病毒的实时荧光定量检测方法
建立了一种基于taqman的实时反转录定量PCR (RT-qPCR)方法,用于检测和定量侵染果树的黑莓绿环斑病毒(BCRV)、蓝莓休克病毒(BlShV)和李子痘病毒(PPV)。每种病毒的检出限分别为40拷贝(BCRV)、500拷贝(BlShV)和40拷贝(PPV)。每种病毒选择两组引物探针,扩增效率在90-110%之间。对具有相同寄主植物的其他病毒或类病毒具有较高的特异性。采用FAM和Cy5荧光染料对BCRV、BlShV和PPV进行多重检测。从寄主植物的木本枝条中提取不同数量的RNA,所有集合都保持了较高的效率和灵敏度。这种检测方法将有助于快速准确地诊断植物病毒病,特别是在进口时往往无法获得叶片组织的检疫站。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Plant Pathology Journal
Plant Pathology Journal 生物-植物科学
CiteScore
4.90
自引率
4.30%
发文量
71
审稿时长
12 months
期刊介绍: Information not localized
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