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Application of a real-time PCR method for the detection of pine wood nematode, Bursaphelenchus xylophilus, in wood samples from lodgepole pine

机译:实时荧光定量PCR方法在检测来自黑松木材样品中的松材线虫Bursaphelenchus xylophilus的应用

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摘要

A real-time PCR polymerase chain reaction (real-time PCR) method was developed to detect and differentiate Bursaphelenchus xylophilus (pine wood nematode, PWN) from other wood-inhabiting nematode species. A primer set and a specific TaqmanReg. fluorescent probe were designed to amplify target B. xylophilus heat shock protein 70 sequences. After optimization, this real-time PCR assay was shown to be highly specific and sensitive, detecting at least 0.005 ng of B. xylophilus genomic DNA, as well as DNA extracted from single nematodes. The practical application of this real-time PCR diagnostic method for the detection of B. xylophilus from actual wood samples of lodgepole pine (Pinus contorta, Dougl. var. latifolia) trees containing a heterogeneous population of nematodes, rather than pure cultures or individual nematodes, is demonstrated. This method works well in the presence of potential inhibitors associated with wood after Baermann extraction and thus eliminates the need to produce pure nematode samples through further culturing and/or isolation of nematodes with a high-power microscope..
机译:开发了一种实时PCR聚合酶链反应(real-time PCR)方法,以检测和区分嗜木Bursaphelenchus xylophilus(松木线虫,PWN)与其他居住在木材中的线虫。引物组和特定的TaqmanReg。设计了荧光探针以扩增靶标嗜木芽孢杆菌热激蛋白70序列。优化后,该实时PCR分析显示出高度特异性和敏感性,可检测至少0.005 ng的木糖双歧杆菌基因组DNA以及从单个线虫提取的DNA。这种实时PCR诊断方法从实际的含有不同种类线虫种群而不是纯培养物或单个线虫的寄主松(Pinus contorta,Dougl。var。latifolia)树的木材样品中检测木糖双歧杆菌的实际应用。演示。此方法在Baermann提取后存在与木材相关的潜在抑制剂的情况下效果很好,因此无需通过使用大功率显微镜进一步培养和/或分离线虫来生产纯线虫样品。

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