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A multiplex PCR-based method for the detection and early identification of wood rotting fungi in standing trees

机译:基于多重PCR的立木树木腐烂真菌的检测和早期鉴定方法

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The goal of this research was the development of a PCR-based assay to identify important decay fungi from wood of hardwood tree species in northern temperate regions. Eleven taxon-specific primers were designed for PCR amplification of either nuclear or mitochondrial ribosomal DNA regions of Armillaria spp., Ganoderma spp., Hericium spp., Hypoxylon thouarsianum var. thouarsianum, Inonotus/Phellinus-group, Laetiporus spp., Perenniporia fraxinea, Pleurotus spp., Schizophyllum spp., Stereum spp. and Trametes spp. Multiplex PCR reactions were developed and optimized to detect fungal DNA and identify each taxon with a sensitivity of at least 1 pg of target DNA in the template. This assay correctly identified the agents of decay in 82% of tested wood samples. The development and optimization of multiplex PCRs allowed for reliable identification of wood rotting fungi directly from wood. Early detection of wood decay fungi is crucial for assessment of tree stability in urban landscapes. Furthermore, this method may prove useful for prediction of the severity and the evolution of decay in standing trees.
机译:这项研究的目的是开发一种基于PCR的检测方法,以从北方温带地区的阔叶树种的木材中鉴定出重要的腐烂真菌。设计了十一种分类单元特异性引物,用于PCR扩增蜜环菌属,灵芝属,猴头属,Hypoxylon thouarsianum var的核或线粒体核糖体DNA区域。 Thouarsianum,Inonotus / Phellinus-group,Laetiporus spp。,Perenniporia fraxinea,Pleurotus spp。,Schizophyllum spp。,Stereum spp。和Trametes spp。开发并优化了多重PCR反应,以检测真菌DNA并以模板中至少1 pg靶DNA的敏感性鉴定每个分类单元。该测定法正确地鉴定了82%的测试木材样品中的腐烂因子。多重PCR的开发和优化可以直接从木材中可靠地鉴定木材腐烂真菌。早期发现木材腐烂真菌对于评估城市景观中树木的稳定性至关重要。此外,该方法可用于预测站立树木的严重程度和衰退的演变。

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