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PCR detection of Pseudoperonospora humuli and Podosphaera macularis in Humulus lupulus

机译:Hum草中假单孢菌和黄斑假单胞菌的PCR检测

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Hop downy mildew (Pseudoperonospora humuli) and hop powdery mildew (Podosphaera macularis) are the most important pathogens of hop (Humulus lupulus). The early detection and identification of these pathogens are often made difficult by symptomless or combined infection with another pathogens. Molecular analysis of internal transcribed spacer (ITS) regions of rDNA is a novel and very effective method of species determination. Therefore, specific PCR assays were developed to detect the pathogens Pseudoperonospora humuli and Podosphaera macularis in naturally infected hop plants. The specific PCR primer combinations P1 + P2 and S1 + S2 amplified specific fragments from Pseudoperonospora humuli and Podosphaera macularis, respectively, and did not cross-react with hop DNA nor with DNA from other fungi. PCR primer combinations R1 + R2 and R3 + R4 could be used in multiplex PCR detection of Pseudoperonospora humuli, Podosphaera macularis, Verticillium albo-atrum and Fusarium sambucinum. Phylogenetic relationships were inferred for 42 species of the Erysiphales from nuclear rDNA (ITS1, 5.8S, ITS2). The molecular characterisation and phylogenetic analyses confirmed the species identification of hop powdery mildew. The PCR assays used in this study proved to be accurate and sensitive for detection, identification, classification and disease-monitoring of the major hop pathogens.
机译:啤酒花霜霉病(Pseudoperonospora humuli)和啤酒花白粉病(Podosphaera macularis)是啤酒花(Humulus lupulus)的最重要病原体。这些病原体的早期检测和识别通常由于无症状或与另一种病原体合并感染而变得困难。 rDNA内部转录间隔区(ITS)区域的分子分析是一种新颖且非常有效的物种确定方法。因此,开发了特异性PCR分析法以检测自然感染的啤酒花植物中的假单孢菌和黄斑假单胞菌。特异性PCR引物组合P1 + P2和S1 + S2分别扩增了来自假单孢菌和黄斑假单胞菌的特定片段,并且未与蛇麻草DNA或与其他真菌的DNA发生交叉反应。 PCR引物R1 + R2和R3 + R4组合可用于假单孢菌,黄斑假单胞菌,黄萎病菌和红枯病菌的多重PCR检测。从核rDNA(ITS1,5.8S,ITS2)推断出42种Erysiphales的亲缘关系。分子特征和系统发育分析证实了啤酒花白粉病的种类鉴定。事实证明,这项研究中使用的PCR方法对于主要啤酒花病原体的检测,鉴定,分类和疾病监测是准确而敏感的。

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