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首页> 外文期刊>Phytopathologia Mediterranea >Multiplex PCR for specific identification and determination of mating type in Togninia minima (anamorph Phaeoacremonium aleophilum), a causal agent of esca disease of grapevine
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Multiplex PCR for specific identification and determination of mating type in Togninia minima (anamorph Phaeoacremonium aleophilum), a causal agent of esca disease of grapevine

机译:多重PCR用于特异性鉴定和确定小葡萄球菌(Ecaca esca病的病原体)最小认知层(无性的Phaeoacremonium aleophilum)的交配类型

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摘要

Togninia minima is one of the fungi involved in esca disease of grapevine, worldwide. It has a biallelic heterothallic mating system. A multiplex PCR test was developed that can detect the species as well as the mating type. A T. minima-specific primer set, with expected amplicon size of 500 bp, was designed based on beta-tubulin gene sequences. A previously designed degenerate primer set (NcHMG1 and NcHMG2) was successfully used to amplify a fragment of approximately 300 bp from the Mat1-2 gene of T. minima. The obtained sequence showed substantial homology to the Mat1-2 gene sequences of other related ascomycetes. A more specific primer set, with expected amplicon size of 230 bp, was designed based on the same Mat1-2 gene sequence. The specificity of the new primer set was verified on DNA extracted from a set of Phaeoacremonium and other fungal species frequently occurring on grapevine. Both primer sets were combined in a multiplex PCR for the simultaneous identification and determination of mating types of T. minima. A 500 bp amplicon was obtained from all available T. minima isolates and none from the other Phaeoacremonium spp. A 230 bp amplicon confirmed T. minima isolates that have the Mat1-2 allele. The species-specific beta-tubulin-based primer set served as an internal control to confirm that the PCR reaction with the mating type primer set had worked properly. The efficacy of the multiplex test was evaluated on 31 isolates of T. minima from different vineyards in the Azarshahr region (East Azerbaijan province, Iran). Isolates of both mating types were found from the sampled areas; however, Mat1-2 isolates were more frequent than Mat1-1 isolates (19: 12). This multiplex PCR assay developed can facilitate rapid screening of mating types in populations of T. minima.
机译:全世界范围内,极小的Togninia是与葡萄的埃斯卡病有关的真菌之一。它具有双等位异硫杂交配系统。已开发出可以检测物种以及交配类型的多重PCR测试。基于β-微管蛋白基因序列设计了预期的扩增子大小为500 bp的最小拟南芥特异性引物组。先前设计的简并引物组(NcHMG1和NcHMG2)已​​成功用于扩增来自短螺旋体Mat1-2基因的约300 bp片段。所获得的序列显示出与其他相关子囊菌的Mat1-2基因序列基本同源。基于相同的Mat1-2基因序列,设计了一个更特异性的引物组,预期的扩增子大小为230 bp。新的引物组的特异性已在从一组葡萄球菌和其他葡萄品种上常见的真菌物种中提取的DNA上进行了验证。将两种引物组在多重PCR中组合以同时鉴定和确定最小的T.交配类型。 500 bp的扩增子是从所有可用的最小拟南芥分离株中获得的,而没有一个是从其他Phaeoacremonium spp中获得的。一个230 bp的扩增子证实了带有Mat1-2等位基因的最小T.分离株。物种特异性的基于β-微管蛋白的引物组用作内部对照,以确认与交配型引物组的PCR反应是否正常进行。在来自Azarshahr地区(东阿塞拜疆省,伊朗)不同葡萄园的31株最小的T. T.菌株中评估了多重试验的功效。从采样区域发现了两种交配类型的分离株。但是,Mat1-2分离株比Mat1-1分离株更常见(19:12)。所开发的这种多重PCR分析方法可以促进快速筛选最小隐孢子虫种群中的交配类型。

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