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Development and application of new molecular markers for analysis of genetic diversity in Verticillium dahliae populations

机译:黄萎病菌群体遗传多样性分析新分子标记的开发与应用

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摘要

The aim of this study was to develop new polymorphic markers for analysis of genetic diversity in the fungal soilborne plant pathogen Verticillium dahliae. Twelve polymorphic markers (five microsatellites and seven polymorphic sequences) were developed from a genomic library enriched for microsatellites. Screening of polymorphic loci was done using a collection of 25V. dahliae isolates of diverse geographic origins, host sources and vegetative compatibility groups (VCGs). Three methods were used to score alleles: polyacrylamide gel electrophoresis (PAGE), sequencing of PCR-amplified loci, and capillary electrophoresis. The new markers were used to assess genetic differentiation between isolates associated with different host plants. Two collections of isolates were analysed, obtained from artichoke (30 isolates) and potato (20 isolates) from crops grown in rotation located in the same area in eastern-central Spain. The resolution of genetic differentiation between these two collections using the new markers was compared to that provided by other often-used markers (SCARs and VCGs). Sequence analysis of the alleles proved to be the most unambiguous technique for scoring microsatellite data. The relatively high genetic differentiation observed between isolates from different crops (genetic differentiation coefficient, GST=0·24) and their high genotypic diversity suggest a divergence between V. dahliae from artichoke and potato. It is hypothesized that evolution of V. dahliae from the local resident population in association with the two host crops has occurred. The new markers are useful for resolving population structure within V. dahliae and may contribute to a better understanding of the population biology of this fungus. © 2011 The Authors. Plant Pathology © 2011 BSPP.
机译:这项研究的目的是开发新的多态性标记,以分析真菌土壤传播的植物病原体大黄萎病菌的遗传多样性。从富含微卫星的基因组文库中开发了十二个多态性标记(五个微卫星和七个多态序列)。多态性位点的筛选是使用25V的集合进行的。大丽花的分离物具有不同的地理起源,寄主来源和营养相容性组(VCG)。三种方法用于对等位基因评分:聚丙烯酰胺凝胶电泳(PAGE),PCR扩增的基因座测序和毛细管电泳。新的标记用于评估与不同寄主植物相关的分离株之间的遗传分化。分析了两个分离株,分别是从位于西班牙中东部同一地区的轮作作物中的朝鲜蓟(30个分离株)和马铃薯(20个分离株)获得的。使用新标记将这两个集合之间的遗传分化分辨率与其他常用标记(SCAR和VCG)所提供的分辨率进行了比较。等位基因的序列分析被证明是对微卫星数据评分的最明确的技术。在不同农作物的分离株之间观察到较高的遗传分化(遗传分化系数,GST = 0·24),并且它们的高基因型多样性表明朝鲜蓟与马铃薯的差异很大。假设已经发生了大麦弧菌从当地居民种群与两种寄主作物的进化。新的标记物对于解决大隐孢子虫中的种群结构很有用,并且可能有助于更好地了解这种真菌的种群生物学。 ©2011作者。植物病理学©2011 BSPP。

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