用于快速检测大高良姜奇克病毒的逆转录酶-重组酶聚合酶扩增（RT-RPA）检测方法的开发。

Development of reverse transcriptase-recombinase polymerase amplification (RT-RPA) assay for rapid detection of large cardamom chirke virus.

作者信息

Malavika P, Bhat A I, Greeshma M

机构信息

ICAR-Indian Institute of Spices Research, Kozhikode, Kerala 673012 India.

出版信息

Virusdisease. 2024 Jun;35(2):302-309. doi: 10.1007/s13337-024-00861-2. Epub 2024 Apr 15.

DOI:10.1007/s13337-024-00861-2

PMID:39071872

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11269538/

Abstract

UNLABELLED

Large cardamom chirke virus (LCCV) causing disease of large cardamom is a major production constraint of this crop. Rapid and accurate detection of LCCV is important for managing the disease. In the present study an isothermal assay namely, reverse transcriptase-recombinase polymerase amplification (RT-RPA) was developed for the detection of LCCV. Total RNA isolated by two different methods and crude extracts isolated using five different methods as templates were assessed for their ability to detect LCCV. Of these, only the total RNA isolated by both methods gave consistent and repeatable results while all the crude extracts used as templates gave non-specific amplification. RT-RPA was up to 1000 times more sensitive than conventional RT-PCR for the detection of LCCV. The detection limit of RPA was 10 fg when recombinant plasmid was used as the template. The RT-RPA assay was validated using field samples and found suitable for large-scale screening of large cardamom plants against LCCV for the selection of virus-free plants.

SUPPLEMENTARY INFORMATION

The online version contains supplementary material available at 10.1007/s13337-024-00861-2.

摘要

未标注

导致小豆蔻患病的大粒小豆蔻奇尔克病毒（LCCV）是这种作物产量的主要限制因素。快速准确地检测LCCV对于病害管理至关重要。在本研究中，开发了一种等温检测方法，即逆转录重组酶聚合酶扩增（RT-RPA）用于检测LCCV。评估了通过两种不同方法分离的总RNA以及使用五种不同方法分离的粗提物作为模板检测LCCV的能力。其中，只有通过两种方法分离的总RNA给出了一致且可重复的结果，而所有用作模板的粗提物均产生非特异性扩增。对于LCCV的检测，RT-RPA比传统RT-PCR灵敏高达1000倍。当使用重组质粒作为模板时，RPA的检测限为10 fg。使用田间样本对RT-RPA检测方法进行了验证，发现其适用于大规模筛选小豆蔻植株是否感染LCCV，以选择无病毒植株。

补充信息

在线版本包含可在10.1007/s13337-024-00861-2获取的补充材料。

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