首页> 外文期刊>Journal of Phytopathology >Specific and Sensitive Detection of Phytophthora nicotianae by Nested PCR and Loop-mediated Isothermal Amplification Assays
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Specific and Sensitive Detection of Phytophthora nicotianae by Nested PCR and Loop-mediated Isothermal Amplification Assays

机译:巢式PCR和环介导的等温扩增法检测烟草疫霉菌的特异性和灵敏性

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摘要

Phytophthora nicotianae is an important soilborne plant pathogen. It causes black shank in tobacco and other commercially important crop diseases. Early and accurate detection of P.nicotianae is essential for controlling these diseases. In this study, primers based on the Ras-related protein gene (Ypt1) of P.nicotianae were tested for their specific detection of the pathogen using nested PCR and LAMP assays. For specificity testing, DNA extracts from 47 P.nicotianae isolates, 45isolates of 16 different oomycetes and 25 isolates of other fungal species were used; no cross-reaction with other pathogens was observed. The sensitivity assay showed that the nested PCR and LAMP assays had detection limits of 100fg and 10fg genomic DNA per 25-l reaction, respectively. Furthermore, the nested PCR and LAMP assays were used for the detection of DNA from naturally P.nicotianae-infected tobacco tissues and soil. Our results suggest that the LAMP assay has the greatest potential for the specific detection of P.nicotianae in regions that are at risk of contracting tobacco black shank disease and that the Ypt1 gene is a novel and effective target of P.nicotianae LAMP visual detection.
机译:烟草疫霉是一种重要的土壤传播植物病原体。它在烟草和其他商业上重要的农作物疾病中引起黑胫病。尽早而准确地检测到烟曲霉对于控制这些疾病至关重要。在这项研究中,使用巢式PCR和LAMP分析测试了基于烟曲霉Ras相关蛋白基因(Ypt1)的引物对病原体的特异性检测。为了进行特异性测试,使用了来自47个烟曲霉分离株,16个不同卵菌的45个分离株和其他真菌种类的25个分离株的DNA提取物。没有观察到与其他病原体的交叉反应。敏感性分析表明,巢式PCR和LAMP分析每25-l反应的检测限分别为100fg和10fg基因组DNA。此外,巢式PCR和LAMP测定法还用于检测天然感染烟草的烟草组织和土壤中的DNA。我们的结果表明,在有患烟草黑胫病风险的区域中,LAMP测定法具有最大的潜力,可用于特异性检测烟隐孢子虫,并且Ypt1基因是烟隐孢子虫LAMP视觉检测的新型有效靶标。

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