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Reference Gene Selection and Validation for the Early Responses to Downy Mildew Infection in Susceptible and Resistant Vitis vinifera Cultivars

机译:易感和抗性葡萄品种对霜霉病感染的早期反应的参考基因选择和验证

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摘要

The pivotal role of cultivated grapevine (Vitis vinifera L.) in many countries economy is compromised by its high susceptibility to Plasmopara viticola, the causal agent of downy mildew disease. Recent research has identified a set of genes related to resistance which may be used to track downy mildew infection. Quantification of the expression of these resistance genes requires normalizing qPCR data using reference genes with stable expression in the system studied. In this study, a set of eleven genes (VATP16, 60 S, UQCC, SMD3, EF1α, UBQ, SAND, GAPDH, ACT, PsaB, PTB2) was evaluated to identify reference genes during the first hours of interaction (6, 12, 18 and 24 hpi) between two V. vinifera genotypes and P. viticola. Two analyses were used for the selection of reference genes: direct comparison of susceptible, Trincadeira, and resistant, Regent, V. vinifera cultivars at 0 h, 6, 12, 18 and 24 hours post inoculation with P. viticola (genotype effect); and comparison of each genotype with mock inoculated samples during inoculation time-course (biotic stress effect). Three statistical methods were used, GeNorm, NormFinder, and BestKeeper, allowing to identify UBQ, EF1α and GAPDH as the most stable genes for the genotype effect. For the biotic stress effect, EF1α, SAND and SMD3 were the most constant for the susceptible cultivar Trincadeira and EF1α, GAPDH, UBQ for the resistant cultivar Regent. In addition, the expression of three defense-related transcripts, encoding for subtilisin-like protein, CYP and PR10, was analysed, for both datasets, during inoculation time-course. Taken together, our results provide guidelines for reference gene(s) selection towards a more accurate and widespread use of qPCR to study the first hours of interaction between different grapevine cultivars and P. viticola.
机译:栽培葡萄(Vitis vinifera L.)在许多国家的经济中起着举足轻重的作用,因为它对霜霉病的病原体极度疟原虫高度易感。最近的研究已经确定了一组与抗性有关的基因,可用于追踪霜霉病感染。这些抗性基因表达的定量需要使用在研究系统中具有稳定表达的参考基因对qPCR数据进行标准化。在这项研究中,评估了一组11个基因(VATP16、60 S,UQCC,SMD3,EF1α,UBQ,SAND,GAPDH,ACT,PsaB,PTB2),以在相互作用的最初几个小时内鉴定参考基因(6、12, 18和24 hpi)之间的两个酿酒葡萄基因型和葡萄。两种分析方法用于选择参考基因:在接种 P后0小时,6、12、18和24小时,直接比较易感的Trincadeira和抗性的Regent,V。vinifera品种。 viticola (基因型效应);并在接种过程中将每种基因型与模拟接种样品进行比较(生物胁迫效应)。使用三种统计方法GeNorm,NormFinder和BestKeeper,可以将 UBQ EF1α GAPDH 识别为该基因型最稳定的基因影响。对于生物胁迫效应,易感品种Trincadeira和EF1αEF1α SAND SMD3 最为恒定。 , GAPDH UBQ 用于抗病品种丽晶。此外,在接种时程中,对两个数据集分析了三种与防御相关的转录本的表达,分别编码枯草杆菌蛋白酶样蛋白 CYP PR10 。两者合计,我们的结果为选择qPCR来研究不同葡萄品种和 P之间相互作用的最初几个小时提供参考指南,以更准确和广泛地使用qPCR。葡萄

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