Kumar Ravinder, Kaundal Priyanka, Tiwari Rahul Kumar, Lal Milan Kumar, Kumari Hema, Kumar Rakesh, Sagar Vinay, Singh Brajesh
ICAR-Central Potato Research Institute, Shimla, Himachal Pradesh 171001 India.
Present Address: ICAR-Indian Agricultural Research Institute, New Delhi, 110012 India.
3 Biotech. 2023 Nov;13(11):373. doi: 10.1007/s13205-023-03791-w. Epub 2023 Oct 16.
Vegetative propagation of potatoes makes it possible for potato viruses to be transmitted through tubers. Potato virus A (PVA) is one of these viruses, which belongs to the genus in the family. Potato tuber yield can be reduced by 30-40% by PVA alone. Losses can be further exacerbated by potato virus X and/or potato virus Y infection. PVA is transmitted primarily by several species of aphids in non-persistent manner. With the aim of resolving this problem, we developed one-step reverse transcription-recombinase polymerase amplification (RT-RPA), a highly sensitive and cost-effective method for detecting PVA in both potato tubers and leaves. Detection and amplification are performed using isothermal conditions in this method. There was good amplification of the coat protein gene in PVA with all three primers tested. To conduct this study, a primer set that can amplify specific 185 base pair (bp) product was selected. PVA detection was optimized by 30-min amplification reactions, which showed no cross-reactivity with other potato viruses. A simple heating block or water bath was used to amplify PVA product using RT-RPA at a temperature range of 38-42 °C. In comparison to conventional reverse transcription-polymerase chain reaction (RT-PCR), the newly developed RT-RPA protocol exhibited high sensitivity for both potato leaves and tuber tissues. Using cellular paper-based simple RNA extraction procedure, the virus was detected in leaf samples as efficiently as purified total RNA. We also found that combining LiCl-based RNA precipitation with cellular paper discs allowed us to successfully optimize RNA extraction for one-step RT-RPA for detecting PVA in tubers. Tests using this simplified one-step RT-RPA method were successfully applied to 300 samples of both leaves and tubers from various potato cultivars. In our knowledge, this is the first report of an RT-RPA assay utilizing simple RNA obtained from either cellular disc paper or LiCl coupled with cellular disc paper to detect PVA. As a result, this method was equally sensitive and specific for detecting PVA in potatoes. The developed RT-RPA assay is more versatile, durable, and do not require highly purified RNA templates, thus providing an effective alternative to RT-PCR assays for screening of germplasm, certifying planting materials, breeding for virus resistance, and real-time monitoring of PVA.
马铃薯的营养繁殖使得马铃薯病毒能够通过块茎传播。马铃薯A病毒(PVA)就是其中一种病毒,它属于该科的某个属。仅PVA就能使马铃薯块茎产量降低30%-40%。马铃薯X病毒和/或马铃薯Y病毒感染会进一步加剧损失。PVA主要由几种蚜虫以非持久性方式传播。为了解决这个问题,我们开发了一步法逆转录-重组酶聚合酶扩增(RT-RPA)技术,这是一种检测马铃薯块茎和叶片中PVA的高灵敏度且经济高效的方法。该方法在等温条件下进行检测和扩增。用所测试的所有三种引物对PVA的外壳蛋白基因都进行了良好的扩增。为开展本研究,选择了一组能扩增出185个碱基对(bp)特异性产物的引物。通过30分钟的扩增反应优化了PVA检测,该反应与其他马铃薯病毒无交叉反应。使用简单的加热块或水浴在38-42°C的温度范围内通过RT-RPA扩增PVA产物。与传统逆转录-聚合酶链反应(RT-PCR)相比,新开发的RT-RPA方法对马铃薯叶片和块茎组织均表现出高灵敏度。使用基于细胞滤纸的简单RNA提取程序,在叶片样品中检测病毒的效率与纯化的总RNA相同。我们还发现,将基于LiCl的RNA沉淀与细胞滤纸圆盘相结合,能够成功优化用于一步法RT-RPA检测块茎中PVA的RNA提取。使用这种简化的一步法RT-RPA方法对来自不同马铃薯品种的300份叶片和块茎样品进行检测均获得成功。据我们所知,这是首次报道利用从细胞圆盘滤纸或LiCl与细胞圆盘滤纸结合获得的简单RNA进行RT-RPA检测PVA的研究。因此,该方法在检测马铃薯中的PVA时同样灵敏且特异。所开发的RT-RPA检测方法更通用、耐用,且不需要高度纯化的RNA模板,从而为种质筛选、种植材料认证、抗病毒育种以及PVA实时监测提供了一种有效的RT-PCR检测替代方法。
