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用于从植物纯化RNA和粗提物中检测和定量李痘病毒的一步法逆转录-液滴数字PCR的开发与验证

Development and Validation of One-Step Reverse Transcription-Droplet Digital PCR for Plum Pox Virus Detection and Quantification from Plant Purified RNA and Crude Extract.

作者信息

Bertinelli Giorgia, Tizzani Lorenza, Luigi Marta, Monticelli Simona, Ilardi Vincenza

机构信息

CREA Research Centre for Plant Protection and Certification, Via C.G. Bertero 22, 00156 Rome, Italy.

CREA Research Centre for Olive, Fruit and Citrus Crops, Via di Fioranello 52, 00134 Rome, Italy.

出版信息

Plants (Basel). 2024 Nov 22;13(23):3276. doi: 10.3390/plants13233276.

Abstract

Plum pox virus (PPV) is the etiological agent of sharka, the most important viral disease of stone fruit worldwide. In this study, a one-step reverse transcription real-time PCR test (RT-qPCR) was modified and translated as a one-step RT-droplet digital PCR (RT-ddPCR) for sensitive, direct, and accurate detection and quantification of PPV. The modified RT-qPCR and RT-ddPCR PPV detection tests were validated using both plant purified total RNA (TRNA) and crude extract as templates. The proposed tests were sensitive, specific, selective, repeatable, and reproducible in detecting PPV from fresh, lyophilized, and plant samples. RT-ddPCR was more sensitive than RT-qPCR in detecting PPV using purified TRNA while showing the same sensitivity using crude extract. This work highlights the robustness, time-saving, and cost-effective nature of the proposed one-step RT-ddPCR test, offering a potential reduction in resources for PPV detection and quantification even with raw extracts.

摘要

李痘病毒(PPV)是李属果树木痘病的病原体,是全球核果类最重要的病毒性疾病。在本研究中,一种一步法逆转录实时PCR检测(RT-qPCR)被改进并转化为一步法RT-液滴数字PCR(RT-ddPCR),用于对PPV进行灵敏、直接且准确的检测和定量。改进后的RT-qPCR和RT-ddPCR PPV检测方法使用植物纯化总RNA(TRNA)和粗提物作为模板进行了验证。所提出的检测方法在从新鲜、冻干和植物样本中检测PPV时具有灵敏性、特异性、选择性、可重复性和再现性。在使用纯化TRNA检测PPV时,RT-ddPCR比RT-qPCR更灵敏,而在使用粗提物时两者灵敏度相同。这项工作突出了所提出的一步法RT-ddPCR检测方法的稳健性、省时性和成本效益,即使使用粗提物,也能潜在地减少PPV检测和定量所需的资源。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c9dc/11644555/56e7cc75c472/plants-13-03276-g001.jpg

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