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首页> 外文期刊>Journal of Virological Methods >Quantitative detection of Cucumber vein yellowing virus in susceptible and partially resistant plants using real-time PCR.
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Quantitative detection of Cucumber vein yellowing virus in susceptible and partially resistant plants using real-time PCR.

机译:使用实时PCR定量检测易感和部分耐药植物中的黄瓜静脉黄化病毒。

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摘要

A method for the detection of Cucumber vein yellowing virus (CVYV) that combines reverse transcription with real-time PCR (SYBR((R)) Green chemistry) was developed using specific primers designed from a nucleotide sequence of the RNA polymerase gene (NIb) conserved among all the available CVYV strains. This method provided a linear assay over five to six orders of magnitude and reproducibly detected titres as low as 10(3) molecules of the target CVYV cDNA. Real-time PCR gave reproducible results for the quantification of CVYV in young leaves of susceptible and resistant cucumber landraces after mechanical inoculation. Significant differences in the starting amount of target cDNA were found between the analyzed genotypes, indicating differences in viral accumulation that correlated to their different levels of resistance. Real-time PCR results validated our previous findings using slot-blot hybridization, the dominance of the strong resistance to CVYV displayed by C.sat 10, and provided improved reliability and sensitivity of detection. This method has great potential in resistance breeding for germplasm screening, characterization of resistance mechanisms and genetic studies.
机译:利用从RNA聚合酶基因(NIb)的核苷酸序列设计的特异性引物,开发了一种将逆转录与实时PCR(SYBR(R)绿色化学)相结合的黄瓜静脉黄化病毒(CVYV)的检测方法。在所有可用的CVYV菌株中均保守。该方法提供了超过五到六个数量级的线性分析,可重复检测的滴度可低至目标CVYV cDNA的10(3)个分子。实时PCR定量分析了机械接种后易感和抗性黄瓜地方品种幼叶中CVYV的定量结果。在分析的基因型之间发现了靶cDNA起始量的显着差异,表明病毒积累的差异与它们不同的抗性水平相关。实时PCR结果验证了我们以前使用缝隙印迹杂交的发现,即C.sat 10对CVYV的强抗性的优势,并提供了提高的检测可靠性和灵敏度。该方法在抗性育种,种质筛选,抗性机理鉴定和遗传研究等方面具有巨大潜力。

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