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首页> 外文期刊>Journal of General Plant Pathology >Development of real-time PCR assay using TaqMan probe for detection and quantification of Rosellinia necatrix in plant and soil
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Development of real-time PCR assay using TaqMan probe for detection and quantification of Rosellinia necatrix in plant and soil

机译:使用TaqMan探针开发实时PCR检测试剂盒,以检测和定量植物和土壤中的玫瑰茄

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摘要

We developed real-time PCR assays using TaqMan probes to detect and quantify Rosellinia necatrix, the causal agent of white root rot in many plant species. Two sets of PCR primers and TaqMan probe indicated that their detection limits could be as low as 1 fg of template DNA. Using the real-time PCR assays with the TaqMan probes, we were able to quantify R. necatrix DNA in naturally diseased roots of Japanese pear and in artificially infested soil samples. Although the new assays were inadequate for use with naturally infested soil samples, nested PCR procedures improved the detectability of the new assays.
机译:我们开发了使用TaqMan探针的实时PCR测定法,以检测和定量玫瑰茄(Rosellinia necatrix),玫瑰茄是许多植物物种中白根腐烂的病原体。两组PCR引物和TaqMan探针表明,其检测限可低至1 fg模板DNA。使用TaqMan探针进行的实时PCR分析,我们能够对日本梨自然感染的根和人工感染的土壤样品中的R. necatrix DNA进行定量。尽管新方法不足以与自然侵染的土壤样品一起使用,但巢式PCR程序却提高了新方法的可检测性。

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