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A Method to Detect and Quantify Eutypa lata and Diplodia seriate-Complex DNA in Grapevine Pruning Wounds

机译:一种检测和量化Eutypa Lata和Diplodia Seriation-Compled DNA在葡萄树修剪伤口中的方法

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摘要

Trunk diseases are factors that limit sustainability of vineyards worldwide. Botryosphaeria and Eutypa diebacks are caused by several fungi belonging to the Botryosphaeriaceae and Diatrypaceae, respectively, with Diplodia seriata and Eutypa lata beingtwo of the most common species. Previous information indicated that the traditional isolation method used to detect these pathogens from plant samples could underestimate their incidence levels. In the present study, we designed two sets of primers thattarget the j8-tubulin gene and that are amenable for quantitative real-time PCR (qPCR) Sybr-Green assays for the detection and quantification of D. seriate-complex (DseCQF/R) and E. lata (E1QF/R) DNA. The design of a species-specific assay was achievedfor E. lata. For D. seriata, a species-specific assay could not be designed. The low interspecific diversity across ^-tubulin genes resulted in an assay that could not discriminate D. seriata from some closely related species either not yet reported orpresenting a low prevalence on grapevine, such as D. intermedia. We validated our technique on grapevine spur samples naturally and artificially infected with D. seriata and E. lata during the dormant season. Experimental grapevines were located in two counties of northern California where the incidence of both pathogens was previously reported. The qPCR assays revealed that a high frequency of pruning wound infections (65%) was achieved naturally by E. lata, while low infection frequency (less than 5%)was observed using the reisolation method. For D. seriate-complex, low (5%) to no natural infection frequencies were observed by the qPCR and the reisolation method, respectively. These results also provided evidence that our qPCR detection methods were more sensitive to assess the incidence of E. lata and D. seriate-complex in plant samples, than traditional isolation techniques. Benefits of molecular methods for the detection of canker pathogens in the field under natural conditions are discussed.
机译:中继疾病是限制全球葡萄园可持续性的因素。 Botryosphaeria和Eutypa沉着背部是由几种属于Botry ospaeriaceae和DiaTrypacea的真菌引起的,其中包含甲基锡和eutypa Lata istwo最常见的物种。以前的信息表明,用于检测来自植物样本的这些病原体的传统隔离方法可能低估其发病率。在本研究中,我们设计了两组引物,即J8-微管蛋白基因,并且可用于定量实时PCR(QPCR)SYBR-Green测定,用于检测和定量D. Seriate-Complex(DSECQF / R)和E. Lata(E1QF / R)DNA。为E. Lata实现了物种特异性测定的设计。对于D.Seriata,无法设计一种特异性的测定。 β-丁蛋白基因的低间隙多样性导致测定,不能在一些密切相关的物种中区分D.Seriata尚未报道的葡萄葡萄树脂,例如D.介质。我们在休眠期间验证了我们对葡萄葡萄样品上的葡萄刺刺样品的技术,并且在休眠期间患有D.Seriata和E. Lata。实验葡萄藤位于加利福尼亚州北部的两个县,先前报道了两种病原体的发生率。 QPCR测定显示,通过E. LATA天然达到造成伤口感染(65%)的高频率,而使用重度方法观察到低感染频率(小于5%)。对于D. QPCR分别观察到Seriate - 复合物,低(5%)至没有自然感染频率,分别观察到QPCR和再隔离方法。这些结果还提供了证据表明我们的QPCR检测方法更敏感,以评估植物样本中的E. Lata和D.Seriate-综合体的发病率比传统的隔离技术。讨论了在天然条件下检测该领域溃疡病原体的分子方法的优点。

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