Rapid and Sensitive Detection of the Causal Agents of Postharvest Kiwifruit Rot, Botryosphaeria dothidea and Diaporthe eres, Using a Recombinase Polymerase Amplification Assay.

IF 1.8 3区农林科学 Q2 PLANT SCIENCES

Plant Pathology Journal Pub Date : 2023-10-01 DOI:10.5423/PPJ.NT.07.2023.0094

Gi-Gyeong Park, Wonyong Kim, Kwang-Yeol Yang

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Abstract

The occurrence of postharvest kiwifruit rot has caused great economic losses in major kiwifruit-producing countries. Several pathogens are involved in kiwifruit rot, notably Botryosphaeria dothidea, and Diaporthe species. In this study, a recombinase polymerase amplification (RPA) assay was developed for the rapid and sensitive detection of the pathogens responsible for posing significant threats to the kiwifruit industries. The RPA primer pairs tested in this study were highly specific for detection of B. dothidea and D. eres. The detection limits of our RPA assays were approximately two picograms of fungal genomic DNA. The optimal conditions for the RPA assays were determined to be at a temperature of 39°C maintained for a minimum duration of 5 min. We were able to detect the pathogens from kiwifruit samples inoculated with a very small number of conidia. The RPA assays enabled specific, sensitive, and rapid detection of B. dothidea and D. eres, the primary pathogens responsible for kiwifruit rots in South Korea.

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用重组酶-聚合酶扩增法快速、灵敏地检测猕猴桃采后腐烂病、斑点葡萄球菌和双孢子虫的致病因素。

猕猴桃采后腐烂病的发生给主要猕猴桃生产国造成了巨大的经济损失。几种病原体与猕猴桃腐烂有关，特别是多蒂氏菌和双孢菌。在这项研究中，开发了一种重组酶聚合酶扩增（RPA）方法，用于快速灵敏地检测对猕猴桃产业构成重大威胁的病原体。在本研究中测试的RPA引物对对检测B.dothidea和D.eres具有高度特异性。我们的RPA测定的检测限约为两皮克真菌基因组DNA。RPA测定的最佳条件是在39°C的温度下保持至少5分钟。我们能够从接种了极少量分生孢子的猕猴桃样品中检测病原体。RPA分析能够特异、灵敏、快速地检测出B.dothidea和D.eres，这是导致韩国猕猴桃腐烂的主要病原体。

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来源期刊

Plant Pathology Journal 生物-植物科学

CiteScore

4.90

自引率

4.30%

发文量

审稿时长

12 months

期刊介绍： Information not localized