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利用病毒生物活性cDNA克隆引发葡萄感染的实验方案优化

Optimization of a Protocol for Launching Grapevine Infection with the Biologically Active cDNA Clones of a Virus.

作者信息

Shabanian Mehdi, Li Caihong, Ebadi Ali, Dolja Valerian, Meng Baozhong

机构信息

Department of Molecular and Cellular Biology, University of Guelph, Guelph, ON N1G 2W1, Canada.

Department of Horticulture, College of Agriculture and Natural Resources, University of Tehran, Karaj 31587-11167, Iran.

出版信息

Pathogens. 2023 Nov 3;12(11):1314. doi: 10.3390/pathogens12111314.

Abstract

Grapevine leafroll disease (GLRD) is the most globally prevalent and destructive disease complex responsible for significant reductions in grape yield and quality as well as wine production. GLRD is associated with several positive-strand RNA viruses of the family , designated as grapevine leafroll-associated viruses (GLRaVs). However, the specific etiological role of any of these GLRaVs in GLRD has not been demonstrated. Even though GLRaV-3 is considered the chief GLRD agent, little is known about the molecular, cellular, and pathological properties of this virus. Such a knowledge gap is due to multiple factors, including the unavailability of biologically active virus cDNA clones and the lack of reliable experimental systems for launching grapevine infection using such clones. In this work, we tested four methods for inoculating tissue-cultured grapevine plantlets with cDNA clones of GLRaV-3: (i) vacuum agro-infiltration; (ii) agro-pricking; (iii) agro-drenching; and (iv) agro-injection. We showed that vacuum agro-infiltration was the most effective of these methods. Furthermore, we examined the impacts of different experimental conditions on the survival and infectivity rate of grapevines after infiltration. To verify the infectivity rate for different treatments, we used RT-PCR, RT-qPCR, and Western blotting. We found that humidity plays a critical role in the survival of plantlets after agro-infiltration and that the use of RNA silencing suppressor and dormancy treatment both had strong effects on the infection rates. To our knowledge, the experimental protocol reported herein is the most effective system for launching the infection of grapevine using cDNA clones of grapevine viruses featuring up to a 70% infection rate. This system has strong potential to facilitate grapevine virology research including the fulfillment of Koch's postulates for GLRD and other major virus diseases as well as identifying the molecular, cellular, and pathological properties of GLRaVs and, potentially, other important grapevine viruses.

摘要

葡萄卷叶病(GLRD)是全球范围内最普遍且具破坏性的病害复合体,会导致葡萄产量和品质以及葡萄酒产量大幅下降。GLRD与多种正义单链RNA病毒有关,这些病毒属于 科,被命名为葡萄卷叶相关病毒(GLRaVs)。然而,这些GLRaVs中任何一种在GLRD中的具体致病作用尚未得到证实。尽管GLRaV - 3被认为是主要的GLRD病原体,但对该病毒的分子、细胞和病理学特性知之甚少。这种知识差距是由多种因素造成的,包括缺乏具有生物活性的病毒cDNA克隆以及缺乏使用此类克隆引发葡萄感染的可靠实验系统。在这项工作中,我们测试了四种用GLRaV - 3的cDNA克隆接种组织培养葡萄苗的方法:(i)真空农杆菌浸润;(ii)农杆菌针刺;(iii)农杆菌浇灌;(iv)农杆菌注射。我们表明真空农杆菌浸润是这些方法中最有效的。此外,我们研究了不同实验条件对浸润后葡萄苗存活和感染率的影响。为了验证不同处理的感染率,我们使用了逆转录聚合酶链反应(RT - PCR)、实时荧光定量逆转录聚合酶链反应(RT - qPCR)和蛋白质免疫印迹法。我们发现湿度在农杆菌浸润后葡萄苗的存活中起关键作用,并且使用RNA沉默抑制子和休眠处理对感染率都有很大影响。据我们所知,本文报道的实验方案是使用葡萄病毒cDNA克隆引发葡萄感染的最有效系统,感染率高达70%。该系统具有强大的潜力,可促进葡萄病毒学研究,包括完成GLRD和其他主要病毒病害的柯赫氏法则,以及确定GLRaVs以及可能的其他重要葡萄病毒的分子、细胞和病理学特性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f0dc/10674828/e806a8a1b90d/pathogens-12-01314-g001.jpg

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